Sandalwood Basic Biology, Tissue Culture, and Genetic PDF
Sandalwood Basic Biology, Tissue Culture, and Genetic PDF
DOI 10.1007/s00425-015-2452-8
REVIEW
Received: 27 July 2015 / Accepted: 16 December 2015 / Published online: 8 January 2016
Ó Springer-Verlag Berlin Heidelberg 2016
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The historical, cultural, medicinal, and economic              reviews (Rai and Sarma 1990; Ganeshaiah et al. 2007;
importance of sandalwood as a basis                            Arun Kumar et al. 2012; Rashkow 2014). Indian sandal-
for conservation                                               wood was extensively exploited in the Pacific throughout
                                                               the first half of the 19th century although initial evidence of
Sandalwood trees of the genus Santalum belong to the           sandalwood trade originated much earlier, with the begin-
Santalaceae. This family is composed of 29 genera with         ning of Buddhism into China from India (Ritter 1836;
approximately 400 species, 19 of which are specific to the     Thomson et al. 2005a). This occurred in the first century
Santalum genus (Fox 2000; Harbaugh 2007; Harbaugh and          AD typified by smoldering sandalwood incense in temples.
Baldwin 2007; Harbaugh et al. 2010; Butaud 2015;               Trade then extended to the Pacific when Americans and
Table 1). Encyclopedia Britannica online (2013) lists 36       Australians began to trade with China, leading to the dis-
genera. Harbaugh and Baldwin (2007) placed those num-          covery of sandalwood in the Pacific, including Hawaii, and
bers as ‘‘15 extant species, approximately 14 varieties, and   Australia (Thomson et al. 2005a). Commercial exploitation
one recently extinct species, distributed throughout India,    of sandalwood has, however, resulted in the acute degra-
Australia, and the Pacific Islands.’’ Nageswara Rao et al.     dation of natural populations of many species, including
(2011) listed 16 species and several varieties. According to   those in India (Rashkow 2014), Indonesia (Ora 2012),
The Plant List (2015), currently only 12 species names are     Papua New Guinea (Gunn et al. 2002), and Vanuatu
accepted, while 41 remain unresolved (Supplementary            (Gillieson et al. 2008).
Table 1). These discrepancies suggest that some attention          Heartwood does not exist in young trees of S. album and
to the taxonomy of the Santalum genus is required.             only mature trees (30–50 years old) produce the heartwood
    The economically most prominent species include            rich in fragrant essential oil (Burdock and Carabin 2008;
Indian sandalwood or East Indian sandalwood (Santalum          Zhang et al. 2012b). The concentration of essential oil
album L.), and Australian sandalwood [S. spicatum (R.Br.)      within the heartwood of mature sandalwood varies between
A.DC.]. Indian sandalwood has various levels of impor-         trees, ranging from 0.5 to 5 % in S. album (Sindhu
tance in cosmetic, perfumery, and aromatherapy industries,     Veerendra and Anantha Padmanabha 1996), 0.05–8 % in S.
in religion, as well as in traditional medicine (reviewed in   austrocaledonicum (Page et al. 2010b), and 0.1–8.2 % in S.
Dhanya et al. 2010; Arun Kumar et al. 2012; Heena Kausar       lanceolatum (Page et al. 2007). Phytochemical analyses of
et al. 2014). Indian sandalwood was used for carving           the heartwood of several sandalwood species (S. album, S.
wooden idols, the manufacture of richly carved boxes,          spicatum, S. austrocaledonicum, and S. insulare) reveal
work tables, and cabinets (Chada 1972), and for burning in     that more than 230 compounds, mainly terpenoids, have
certain Hindu and Buddhist rituals or to carve deities and     been identified so far (reviewed by Baldovini et al. 2011).
temples (Kushalapa 1998). The wood paste was also used         The Flavor and Extract Manufacturers’ Association, the
as an ointment to dissipate heat (Ral 1990). Sandalwood        United States Food and Drug Administration, as well as the
essential oil, which has a rich tradition of uses spanning     Council of Europe have approved sandalwood essential oil
more than 4000 years as mentioned in Sanskrit texts, is an     for use in food-based products (Burdock and Carabin
important ingredient of cosmetic produces, herbal medi-        2008). The essential oils of sandalwood, including biore-
cine, and perfumes (Ritter 1836; Burdock and Carabin           actors, will be reviewed separately (Teixeira da Silva et al.
2008). The ancient Egyptians imported the wood and used        unpublished review).
it in medicine, embalming and ritual burning to venerate           Excessive exploitation of natural stands and the lack of
the gods (Arun Kumar et al. 2012). Historically, sandal-       initiatives to establish, until fairly recently, artificial stands
wood has a rich tradition of trade with the East, dating as    has led to a decrease in natural stocks and thus an increase
far back as the 5th century BC (Edwards 1951) when its         in market prices (Gillieson et al. 2008; Arun Kumar et al.
aromatic heartwood and oils were already recognized as         2012; Subasinghe 2013). Anantha Padmanabha (2000,
prized commodities. Sandalwood trade in India was started      2014) described a decline in sandalwood production in
as early as the 13th century by Indian rulers trying to        India over several decades: 4000 t (1950) ? 2000
monopolize Indian sandalwood resources to ensure eco-          t (1990) ? *1000 t (1999). More recent figures regarding
nomic strength for power and warfare, the classic case         sandalwood supply in India are difficult to determine, since
being the mighty Vijaya Nagara Empire (13–16 century           much of the traded wood comes from illegally harvested
AC) of the Deccan region (Ganeshaiah et al. 2007). Real-       sources, and estimates suggest around 1000 tonnes of
izing the value of sandalwood, Tippu Sultan, the King of       legally traded wood (AAG 2006; McKinnell 2011). In
Mysore (India), declared the sandalwood tree as a royal        Indonesia, the sandalwood trade in East Nusa Tenggara
tree in 1772 (Buchanan 1884; Adkoli 1977). More histor-        Province decreased rapidly during the 1990s contributing
ical details on Indian sandalwood are available in other       almost 50 % of total regional revenue for the early 1990s to
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Table 1 Santalum species and distribution: modified from Harbaugh and Baldwin (2007), Harbaugh et al. (2010) and Butaud (2015)
Species number        Species                                Variety                                  Distribution
13 % in the late 1990s, and total production continued to                 using Traditionaloven.com (2015)]; (AAG 2006; McKin-
decline from 7465 tonnes in the 9 years 1987–1997 to just                 nell 2011). The average auction price for the heartwood of
2178 tonnes in the 6 years 2001–2007 (Ora 2012).                          wild Indian sandalwood rose from $9,400/tonne in 1990
   According to the Tropical Forestry Services, essential                 (Ral 1990) to approximately $150,000/tonne in July 2014
oil is extracted from the heartwood of Indian sandalwood                  (on small volumes based on an auction held in Tamilnadu,
by distillation and trades for over $5000/kg on the inter-                India), which indicates a significant annual compounded
national market (TFS 2015a). The annual supply of wild-                   growth rate (TFS 2015b). A 12 % annual increase in the
harvested Australian sandalwood species approaches 2000                   minimum price paid to landowners for S. austrocale-
tonnes of S. spicatum (McKinnell 2011), and while a                       donicum in Vanuatu has also been recorded, from an
500 m3 license exists for S. lanceolatum (DPI&F 2004;                     equivalent of US$4/kg in 2000 (Mele 2001; Berry 2005) to
Timber-Queensland 2012), others suggests that actual                      US$20/kg in 2015 (Tosul 2015). The price of S. spicatum
annual yields fluctuate between 120 and 400 tonnes                        varies considerably between product grades, and in
[equivalent to between 49.86 and 166.21 m3; conversion                    2007–2008, export prices ranged from USD 3000 to
                                                                                                                                 123
850                                                                                               Planta (2016) 243:847–887
10,000/tonne (McKinnell 2011), which has increased to         FPC) pers. comm. 2015). Planted sandalwood in Vanautu
USD 8000 to 17,000/tonne in 2014–2015 (Zauba.com              (S. austrocaledonicum) comprises largely small-scale
2015). The price of Indian sandalwood is ten times higher     woodlots with an estimated area of approximately 550 ha
than that of Australian sandalwood while the heartwood of     planted by 2006 with planting continuing to date (Page
Indian sandalwood yields more essential oil with a higher     et al. 2010a).
proportion of a- and b-santalols—important constituents of       This review aims to explore the basic biology and
sandalwood oil fragrance—than other sandalwood species        propagation of the genus Santalum, how in vitro tissue
(Baldovini et al. 2011; FAO 2015; TFS 2015a). This pos-       culture has been used to produce clonal plant material, and
itive economic perspective makes Indian sandalwood an         what promises this technology holds in aiding the conser-
attractive option for commercial growers aiming at inter-     vation and mass propagation of threatened Santalum
national perfumery, cosmetic, and pharmaceutical markets      germplasm.
(Christian 2015).
    Indian sandalwood tree is a hemi-parasitic plant that
requires a host for sustained growth (discussed in more       Basic biology and propagation
detail in the section ‘‘Hemi-parasitism and host plant
dependence’’), making cultivation practices highly spe-       Basic biology, flowering control, reproductive
cialized. These factors, together with its strong demand in   mechanisms, and breeding
Asia and the Middle East for the global fragrance industry,
have led to the mass deforestation of Indian sandalwood       Sexual reproduction
from natural habitats. Indian sandalwood was first classi-
fied as vulnerable by the International Union for Conser-     The onset of reproductive maturity in several sandalwood
vation of Nature (IUCN) in 1998 (IUCN 2015a). The             species (S. album, S. austrocaledonicum, S. macgregorii, S.
Convention on International Trade in Endangered Species       spicatum, and S. yasi) occurs between 2 and 5 years (Jiko
(CITES) also considers closely related S. austrocale-         1993; Barrett and Fox 1995; Doran and Brophy 2005).
donicum, S. yasi, and S. insulare as endangered (CITES        Sexual reproduction in sandalwood may be considered to
2013). Four Santalum species, namely S. album (vulnerable     be opportunistic with several species flowering across most
due to factors like fire, grazing, exploitation of wood and   months of the year, with two (sometimes three) peak
smuggling; IUCN 2015a), S. fernandezianum (extinct due        periods following favorable rainfall events/periods. In S.
to cutting for the aromatic wood; IUCN 2015b), S. mac-        austrocaledonicum (Doran and Brophy 2005), S. macgre-
gregorii (endangered due to overexploitation of the scented   gorii (Bosimbi 2005), and S. yasi (Bulai and Nataniela
wood for incense; IUCN 2015c), and S. haleakalae (vul-        2005), a low level of reproduction may be found across
nerable; IUCN 2015d), are listed in the IUCN Red Data         most months of the year. The periods of peak fruit pro-
List. The use of traditional technologies such as seed ger-   duction occur in both wet and dry seasons with the most
mination, as well as the use of applied biotechnologies,      prominent of these two peaks occurring in the wet months
such as tissue culture, would allow production to be stan-    for S. album (in India and Timor) (Suriamihardja and
dardized, and perhaps even reverse species decline through    Suriamihardja 1993) and S. yasi (in Fiji) (Bulai and
the production of cultivated stands.                          Nataniela 2005) and the dry months for S. austrocale-
    In southern China, great efforts are being made to        donicum (in Vanuatu) (Daruhi 1993; Doran and Brophy
increase production (Zhang et al. 2007) while plantations     2005). Reproduction in S. spicatum (Applegate et al. 1990;
have expanded in India, China, Indonesia, and Australia       Loneragan 1990) and S. lanceolatum (Applegate and
over the past 20 years (Dhanya et al. 2010; Lu 2011).         McKinnell 1993) is highly dependent upon rainfall events,
Indian sandalwood (S. album) plantings in Australia are       and the timing and location of seed crops are highly vari-
currently approaching 11,000 ha with two main producers       able. The period of fruit development in tropical sandal-
Tropical Forestry Services (TFS 2015c) having just over       wood species typically occurs over a 2- to 3-month period
9000 hectares and Santanol who acquired Elders Forestry       (Corrigan et al. 2005), whereas it can take up to 6 months
estate in 2013 (Jackman 2013) comprising approximately        for the fruit to mature in S. spicatum (Barrett and Fox
1800 ha (Werren 2011). In South China, plantation of S.       1995).
album on a large scale began in 2013 increasing rapidly          The general breeding system of Santalum species may
to 5000 ha, planted mainly in mountain areas (Guohua          be described as facultatively allogamous (incompletely
Ma, unpublished data). According to Western Australian        outbreeding), with variation between families and indi-
Forest Products Commision (FPC), the 2015 Australian          viduals at the level of self-incompatibility (Ma et al. 2006;
sandalwood (S. spicatum) plantings in Australia are           Muir et al. 2007; Tamla et al. 2011) and with no capacity
approaching 20,000 ha (Erasmus (General Manager of            for apomixis or parthenocarpy (Ma et al. 2006; Tamla et al.
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the exception in this genus. This feature of the breeding       karyotypes belonged to the 2B type of Stebbins’ karyotypic
system can facilitate the introgression of traits between       symmetry (Stebbins 1971), suggesting that S. album was a
species and the development of hybrids. Introduction of         primitive taxon. Somatic cells of S. yasi and the sponta-
exotic sandalwood species within the natural range of a         neous F1 hybrid, S. album 9 S. yasi, were diploid, with
compatible species will likely result in uncontrolled gene      2n = 20 (Zhang et al. unpublished data). These results
flow between them and modify the genetic structure and          allow species and this hybrid in Santalum to be exploited
diversity of the local species.                                 and utilized in future plant breeding programs.
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Planta (2016) 243:847–887                                                                                                 853
coconut dust (1:1:1, w/w), including 2 % calcium super-         a source of scions improved graft success (60 %) more than
phosphate, resulted in 98 % survival (as well as greater        scions obtained directly from field-grown trees. The suc-
height and biomass than other substrates) of S. album           cess rate of in vitro grafting was also affected by scion size
seedlings when Kuhnia rosmarinifolia Vent. was used as          and rootstock age. Under suitable conditions, scions and
the primary host plant and after treating surface-sterilized    hypocotyls united to form complete plants with 2–4 leaves
(0.1 % mercuric chloride for 5–6 min and three washes in        within 6–8 weeks (Sanjaya et al. 2006a). Grafting of S.
distilled water) seeds with 1 mg/L GA3 for 24 h. Lu et al.      austrocaledonicum has also been demonstrated using a top-
(2013) soaked S. album seeds in 0.1 % GA3 for 12 h using        wedge graft with actively growing semi-hardwood stems
the protocol of Radomiljac (1998) then surface-sterilized       (Tate et al. 2006). These authors suggested that the success
them with 3 % NaOCl for 5 min, washed them with dis-            of grafting was dependent upon the skill of the propagator
tilled water, and then germinated them on sterilized sand       with the percentage of successfully grafted unions varying
soaked with distilled water at 28–30 °C for 3–4 weeks.          between 60 and 90 %.
When germination conditions are suitable and in associa-           Thus, techniques for the establishment of a seedling
tion with an appropriate host, this method can be useful for    stock are well established, although mechanization of the
the large-scale seed germination of S. album (Ral 1990), as     process is less explored. To address this gap, St. Jack et al.
summarized in Fig. 1 (specific for Karnataka, India).           (2013) devised a seed metering device that would optimize
Athelstone et al. (1994) assessed the effects of plant growth   the mechanization of seed planting and germination.
regulators (ethrel, silver thiosulfate, 6-benzyladenine,
kinetin, GA3, and GA4) on S. accuminatum seed germi-            Vegetative propagation
nation. They found that cracking seed and treatment with
580 lM GA3 (duration of treatment not reported) resulted        Various authors have reported on successful vegetative
in 90 % seed germination within 43 days. Jayawardena            propagation of S. album by cuttings. Uniyal et al. (1985)
et al. (2015) found that scarification and 500 mg/L GA3         demonstrated that S. album can be propagated by root
could increase germination to 100 % from near-zero levels       cuttings with 60 % success when they used Seradix B2Ò at
in non-scarified control S. album seeds. Chauvin and Ehr-       the time of planting during the first week of April under
hart (1998) observed differences in germination rates of        Indian conditions. S. lanceolatum can be propagated by
two provenances of S. austrocaledonicum var. austro-            root suckers (Warburton et al. 2000). Havea (2012)
caledonicum: 55 % germination in the ‘‘Ile des Pins’’           reported that S. yasi, S. album, and their hybrids can be
provenance after 2 years and 0 % germination in the             vegetatively propagated using apical cuttings from younger
‘‘Mare’’ provenance with the exception of 19 % germina-         seedlings (up to 12 months of age). They recommended
tion in one lot after 15 months. Nasi (1995) had noted that     treating the cuttings with indole-3-butyric acid and a-
25 % germination of S. austrocaledonicum var. pilosulum         naphthaleneacetic acid (1.0 mg/L each) and using a sub-
was possible without pre-treatment, but only after 1 year;      strate composed of sand:peatmoss (30:70, w/v).
however, removing the endocarp, nicking the seeds, not             Batabyal et al. (2014) proposed that S. album can be
storing seeds, and soaking seeds in 100 mg/L GA3 all            propagated using 15-cm-long stem cuttings from 3- to
increased the germination percentage at 28 °C. Natural          4-year-old trees by treatment with 1.5 mg/L indole-3-acetic
stands of S. album growing in East Nusa Tenggara Pro-           acid (IAA) and 1.5 mg/L GA3, resulting in most leaves per
vince in Indonesia showed regeneration percentages rang-        branch, although rooting percentages among the treatments
ing widely from 4.85 to 48.4 % (Wawo 2008).                     were not reported. These authors were also able to increase
    In vivo or in vitro germinated seedlings can be used as     the number of branches per cutting by applying 1.5 mg/L
ideal rootstock for grafting (Sanjaya and Rai 2003). San-       IBA and kinetin. Rao and Srimathi (1977) attempted air
jaya et al. (2006a) managed to attain a 50 % in vivo            layering to clonally propagate S. album, in which branches
micrografting rate of success in S. album when 4- to 5-cm-      of 2 cm thick from different seasons’ growth were used,
long scions, collected from a candidate plus tree (CPT) of      observing that March–April (rainy season) were most
50–60 years of age, were grafted onto 90-day-old nursery-       favorable for air layering under Indian conditions. Collins
grown rootstock. Sanjaya et al. (2006a) reported that scion     et al. (2000) found substantial variation in the percentage
size, rootstock age, and scion collection season are vital      of stem cuttings with adventitious roots between experi-
factors that affect graft success. Grafted plants were kept     ments, genotypes and species. Differences between
under greenhouse conditions for 6–8 weeks to allow for          experiments were recorded for S. album (9.5 and 0 %
graft union. In vitro micrografts were accomplished by          rooting), S. austrocaledonicum (63.5 and 20.2 %), and S.
placing 1- to 2-cm-long scions collected from nodal cut-        yasi (46.1 and 10.1 %). Differences were observed
tings (obtained from CPT) onto the hypocotyl of 45-day-         between 15 S. austrocaledonicum genotypes with root
old in vitro rootstocks. The use of in vitro-grown shoots as    induction ranging from 25 to 88.9 %. It has been proposed
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Ready for transplanting to the field Seeds available (April-May and Sept-Oct)
GA3-treated seeds
that S. yasi and S. austrocaledonicum are more amenable to                    many species of the Fabaceae, Mimosaceae, Casuari-
stem cutting propagation than S. album, S. lanceolatum,                       naceae, Meliaceae, Myrtaceae, Apocynaceae, and Rham-
and S. macgregorii (Collins et al. 2000; Thomson et al.                       naceae are proven good hosts. However, not all species in
2005b). The differences observed in the series of experi-                     these families are good hosts. For example, in the Faba-
ments conducted by Collins et al. (2000) indicate that it is                  ceae, many species, including Butea monosperma and
difficult to generalize the optimum conditions required for                   Tamarindus indica, are poor hosts (Table 2).
successful stem cutting propagation across the Santalum                          Annapurna et al. (2004) noticed that the container size
genus.                                                                        for potting influenced the success of pot growth, with
                                                                              600 ml pots being an ideal size for S. album seedlings,
Hemi-parasitism and host plant dependence                                     producing plantlets 20 cm high within 6 months when in
                                                                              the presence of pigeon pea [Cajanus cajan (L.) Millsp.] as
First noted by Scott (1871), and further confirmed by                         the host plant. These authors also recommended a potting
Brandis (1903), Santalum species are hemi-parasitic,                          mixture of sand, soil, compost, burnt rice husk, and char-
whereby they derive part of their water and nutrient                          coal (5:3:10:1:1). Despite these optimized conditions, the
requirements from a host plant. Under cultivation, sandal-                    authors noted that root development was quite poor, indi-
wood species require hosts during all stages of production                    cating that one possible reason might be the use of an
including the pot stages, in the first years of establishment                 inappropriate host. Radomiljac (1998) had previously used
and at maturity (Ehrhart and Fox 1995; Fox et al. 1996;                       Alternanthera nana R.Br. and Sesbania formosa (F.
Radomiljac et al. 1998a, 1999a; Annapurna et al. 2006),                       Muell.) N. Burb. as the primary host in pot experiments
although the choice of potting medium can also be an                          that used 1500 ml pots in a substrate consisting of sand,
influencing factor (Annapurna et al. 2005). Sandalwood                        peat, and perlite (3:2:2), successfully increasing the sur-
can potentially be grown across a range of environments                       vival, height, and diameter of S. album plants; in that study,
provided locally adapted host species can be identified for                   Atalaya hemiglauca (F.Muell.) F.Muell. ex Benth, Acacia
each stage of cultivation (Table 2). Among these families,                    hemignosta F.Muell, and Crotalaria retusa L. were not
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      Table 2 Host plants (suitable and unsuitable) for sandalwood (chronological listing)
      Species         Country of      Suitable hosts                              Family          Unsuitable hosts                Family        References
                      test
      S. album        India           Azadirachta indica A.Juss                   Meliaceae       Butea monosperma (Lam.) Taub.   Fabaceae      Parthasarathi et al.
                                      Cassia fistula L.                           Fabaceae        Dodonea viscosa Jacq.           Sapindaceae    (1974)
                                      C. siamea (Lam.) lrwin et Barneby           Fabaceae        Gmelina arborea Roxb.           Lamiaceae
                                      Dalbergia latifolia Roxb.                   Fabaceae        Melia azedarach L.              Meliaceae
                                                                                                                                                                          Planta (2016) 243:847–887
123
      Table 2 continued
                                                                                                                                                                                   856
123
      S. acuminatum   Australia    Acacia rostellifera Benth.             Mimosaceae         NR                                                        Tennakoon et al. (1997b)
                                   A. pulchella R. Br.                    Mimosaceae
                                   Allocasuarina campestris (Diels) L.    Casuarinaceae
                                    Johnson
                                   Alyogyne hakeaefolia (Giord.) Alef.    Malvaceae
                                   Anthocercis viscosa R. Br.             Solanaceae
                                   Baeckea tetragona Benth.               Myrtaceae
                                   Cryptandra mutila Reisseck.            Rhamnaceae
                                   Dodonaea aptera Miq.                   Sapindaceae
                                   Exocarpos sparteus R. Br.              Santalaceae
                                   Leucopogon ovalifolius Sonder.         Epacridaceae
                                   Lysinema ciliatum R. Br.               Epacridaceae
                                   Melaleuca viminea Lindley              Myrtaceae
                                   Spyridium cordatum (Turca.) Benth.     Rhamnaceae
      S. spicatum     Australia    Acacia acuminata Benth.                Fabaceae           Allocasuarina huegeliana (Miq.) L.A.S.    Casuarinaceae   Brand et al. (1998, 2000,
                                                                                              Johnson                                                   2003); Brand (2009)
                                                                                             Eucalyptus loxophleba subsp. loxophleba   Myrtaceae
      S. album        Australia    Acacia trachycarpa E. Pritzal          Mimosaceae         Eucalyptus camaldulensis Dehnh.           Myrtaceae       Radomiljac et al. (1998b,
                                   A. ampliceps Maslin.                   Mimosaceae                                                                    1999a,b,c)
                                   Sesbania formosa (F. Muell) N. Burb.   Papilionaceae
      S. acuminatum   Australia    Melia azedarach L.                     Meliaceae          NR                                                        Loveys et al. (2001a)
                                   Myoporum parvifolium R.Br.             Scrophulariaceae
      S. acuminatum   Australia    Acacia pycnantha Benth.                Mimosaceae         Eucalyptus fasciculosa F. Mueller         Myrtaceae       Loveys et al. (2001b)
                                   Atriplex vesicaria Benth.              Amaranthaceae      Eucalyptus camaldulensis Dehnh.           Myrtaceae
                                   Heterodendrum oleifolium Desf.         Sapindaceae
                                   Pittosporum phylliraeoides DC.         Pittosporaceae
                                   Rhagodia spinescens var. deltaphylla   Amaranthaceae
      S. acuminatum   Australia    Acacia cyclops A Cunn. Ex G. Don       Mimosaceae         NR                                                        Loveys et al. (2002)
                                   Atriplex nummularia Lindl.             Amaranthaceae
                                   Myoporum parvifolium R. Br.            Scrophulariaceae
                                   Templetonia retusa (Vent.) R. Br.      Fabaceae
      S. acuminatum   Australia    Acacia acuminata Benth.                Mimosaceae         NR                                                        Woodall and Robinson
                                                                                                                                                        (2002)
                                                                                                                                                                                   Planta (2016) 243:847–887
      Table 2 continued
      Species         Country of   Suitable hosts                            Family            Unsuitable hosts                           Family           References
                      test
      S. acuminatum   Australia    Acacia acuminata Benth.                   Mimosaceae        Acacia cyclops A.Cunn. ex G. Don           Mimosaceae       Woodall and Robinson
                                   A. asepala Maslin                         Mimosaceae        A. jibberdingensis Maiden & Blakely        Mimosaceae        (2003)
                                   A. assimilis S.Moore                      Mimosaceae        Alyxia buxifolia R.Br.                     Apocynaceae
                                   A. cochlearis (Labill.) H.L.Wendl.        Mimosaceae        Astroloma prostratum R.Br.                 Epacridaceae
                                                                                                                                                                                  Planta (2016) 243:847–887
                                   A. declinata R.S. Cowan & Maslin          Mimosaceae        A. epacridis (DC.) Druce                   Epacridaceae
                                   A. erinacea Benth.                        Mimosaceae        Dichopogon fimbriatus (R.Br.) J.F.Macbr.   Anthericaceae
                                   A. glaucoptera Benth.                     Mimosaceae        Dryandra armata R.Br.                      Proteaceae
                                   A. lasiocalyx C.R.P.Andrews               Mimosaceae        Enchylaena tomentosa R.Br.                 Chenopodiaceae
                                   A. microbotrya Benth.                     Mimosaceae        Eucalyptus perangusta Brooker              Myrtaceae
                                   A. patagiata R.S. Cowan & Maslin          Mimosaceae        E. salmonophloia F.Muell.                  Myrtaceae
                                   A. pulviniformis Maiden & Blakely         Mimosaceae        E. tetragona (R.Br.) F.Muell               Myrtaceae
                                   A. saligna H. Wendl.                      Mimosaceae        Grevillea nudiflora Meisn.                 Proteaceae
                                   A. sulcata R.Br.                          Mimosaceae        Hybanthus floribundus (Lindl.) F.Muell.    violaceae
                                   Allocasuarina campestris (Diels)          Casuarinaceae     Melaleuca pentagona Labill.                Myrtaceae
                                    L.A.S.Johnson
                                   A. huegeliana (Miq.) L.A.S.Johnson        Casuarinaceae     Nemcia hookeri (Meisn.) Crisp              Papilionaceae
                                   A. humilis (Otto & F.Dietr.)              Casuarinaceae     Opercularia spermaocea                     Rubiaceae
                                    L.A.S.Johnson
                                   A. microstachya (Miq.) L.A.S.Johnson      Casuarinaceae     Oxylobium microphyllum Benth.              Papilionaceae
                                   A. thuyoides (Miq.) L.A.S.Johnson         Casuarinaceae     Petrophile fastigiata R.Br.                Proteaceae
                                   Banksia attenuate R.Br.                   Proteaceae        P. seminuda Lindl.                         Proteaceae
                                   Dampiera lavandulacea Lindl.              Goodeniaceae      Rhagodia baccata (Labill.) Moq.            Henopodiaceae
                                   Daviesia incrassate Sm.                   Papilionaceae     Spyridium majoranifolium (Fenzl) Rye       Rhamnaceae
                                   D. teretifolia Benth.                     Papilionaceae     Synaphea petiolaris R.Br.                  Proteaceae
                                   Dodonaea humifusa Miq.                    Sapindaceae
                                   D. ptarmicaefolia Turcz.                  Sapindaceae
                                   Gastrolobium parviflorum (Benth.) Crisp   Papilionaceae
                                   Hakea lissocarpha R.Br.                   Proteaceae
                                   H. nitida R.Br.                           Proteaceae
                                   H. preissii Meisn.                        Proteaceae
                                   H. trifurcata (Sm.) R. Br.                Proteaceae
                                   Halgania cyanea Lindl.                    Boraginaceae
                                   Hibbertia rupicola (S.Moore)              Dilleniaceae
                                    C.A.Gardner
                                   Jacksonia furcellata (Bonpl.) DC.         Papilionaceae
                                   Labichea lanceolata Benth.                Caesalpiniaceae
                                                                                                                                                                                  857
123
      Table 2 continued
                                                                                                                                                                                      858
123
                              Lasiopetalum rosmarinifolium (Turcz.)          Sterculiaceae
                               Benth.
                              Olearia axillaris (DC.) Benth.                 Asteraceae
                              O. muelleri Benth.                             Asteraceae
                              Senna artemisioides subsp. filifolia Randell   Caesalpiniaceae
                              Templetonia retusa (Vent.) R. Br.              Papilionaceae
                              Thomasia angustifolia Steud.                   Sterculiaceae
      S. album   India        Azadirachta indica A. Juss                     Meliaceae         Artocarpus integrifolia L.                     Moraceae        Nagaveni and
                              Cajanus cajan (L.) Millsp.                     Papilionaceae     Acacia auriculiformis A. Cunn. Ex Benth.       Fabaceae         Vijayalakshmi (2003)
                              Casuarina equisetifolia L.                     Casuarinaceae     Swietenia mahogani L.                          Meliaceae
                              Eucalyptus camaldulensis Dehnh.                Myrtaceae
                              Pongamia pinnata L.                            Fabaceae
                              Tectona grandis L.                             Verbenaceae
                              Wrightia tinctoria (Roxb.)R.Br.                Apocynaceae
      S. album   China        Acacia auriculaeformis A. Cunn.                Fabaceae          Artocarpus heterophyllus (Wall.) R. N. Park.   Moraceae        Li (2003)
                              Acacia confusa Merr.                           Fabaceae          Camellia odorata Abel.                         Theaceae
                              Albizia lebbek (L.) Benth.                     Fabaceae          Mangifera indica Linn                          Anacardiaceae
                              Caesalpinia pulcherrima L.                     Caesalpiniaceae   Ormosia fordiana Oliv.                         Papilionaceae
                              Casuarina junghuhniana Miq.                    Casuarinaceae     Pterocarpus echinatus Pers.                    Fabaceae
                              Cajanus cajan (L.) Mill sp.                    Fabaceae          Syzygium cumini (L.) Skeels                    Myrtaceae
                              Kuhnia rosmarnifolia Vent.                     Asteraceae
                              Lantana camara L.                              Verbenaceae
      S. album   China        Gardenia jasminoides Ellis                     Rubiaceae         NR                                                             Ma et al. (2005)
                              Hibiscus rosa-sinensis L.                      Malvaceae
                              Phyllanthus reticulatus Poir.                  Euphorbiaceae
      S. album   China        Acacia confusa Merr.                           Fabaceae          Bischofia polycarpa (H. Lévl.) Airy Shaw      Euphorbiaceae   Lu (2011); Lu et al.
                              Dalbergia odorifera T. Chen                    Fabaceae          Dracontomelon duperreranum Pierre              Anacardiaceae    (2013, 2014)
      S. album   China        Kuhnia rosmarnifolia Vent.                     Asteraceae        NR                                                             Zhang et al. (2012a)
                              Acacia confusa Merr.                           Fabaceae          Bauhinia blakeana Dunn                         Leguminosae     Chen et al. (2014)
                              Calliandra haematocephala Hassk.               Mimosaceae        Delonix regia (Hook.) Raf.                     Leguminosae
                              Caesalpinia sappan L.                          Fabaceae          Leucaena leucocephala Lam.                     Mimosaceae
                              Erythrina corallodendron L.                    Papilionaceae     Ormosia pinnata (Lour.) Merr.                  Papilionaceae
                                                                                                                                                                                      Planta (2016) 243:847–887
Planta (2016) 243:847–887                                                                                                                                                                                                 859
                                                                                                                                                                 good host for 1–2 years until the parasitized host dies. At
                                                                                                                                                                 this stage, some shrubs (Tephrosia candida Roxb. DC,
                                                                                                                                                                 Calliandra haematocephala, Cajanus cajan Millsp) and
                                                                                                                                                                 small trees (Caesalpinia sappan Linn, Cerasus yedoensis
                                                                                                                                                                 Matsum.) need to be cultivated near sandalwood trees.
                    Unsuitable hosts
China
                                                                                                                                                                 spheric soil of almost all fine hosts ranged from 5.0 to 6.0
                                       India
                    test
                                                                                                                                                                                                                   123
860                                                                                                 Planta (2016) 243:847–887
differences among different N2-fixing hosts (Chen et al.        the hemi-parasitism by haustoria that form between San-
2014).                                                          talum species and the host root. Sahai and Shivanna (1984)
   A recent comparative study showed that a suitable host       observed that the addition of 30 lg/ml xenognosin, the
among leguminous and non-leguminous trees could pro-            active fraction of tragacanth gum (an exudate of a legume,
mote the growth of S. album. Ouyang et al. (2015) found         Astragalus sp.), could effectively induce haustoria in
that net photosynthetic rate, stomatal conductance, tran-       3-month-old S. album seedlings in the absence of the host.
spiration rate, and plant height in S. album in China were         Tennakoon et al. (1997a) found that S. acuminatum
similar in two suitable hosts, D. sissoo, a leguminous tree,    derived nitrogen primarily from woody N2 fixers (legumes
and Lonicera japonica, a non-leguminous vine. It was            and Allocasuarina), although each host transported a
suggested that black-stained material (BSM) in the inter-       characteristic set of organic nitrogenous solutes, but little
action of haustoria penetrating into hosts might play an        or no nitrate. They concluded that only a limited direct flow
important role in establishing the sandalwood host con-         of amino compounds took place between xylem streams of
nection. In the good hosts, L. japonica and D. sissoo, the      hosts and S. acuminatum (Tennakoon et al. 1997b). There
connection between the finger parenchymal cells of the          were close resemblances between S. album and legume
haustoria and the host root cell was tight and was related to   hosts (S. formosa, A. trachycarpa, A. ampliceps) in con-
the presence of a prominent BSM while BSM in the poor           centration and composition of xylem sap amino acids, and
host Aquilaria sinensis was thin. The origin of BSM and its     in the amino acid spectra of the corresponding parasite
functions remain unclear. Thus, the metabolism underlying       endophytic tissue, and low N levels in xylem sap of
the host preference of sandalwood needs further                 E. camaldulensis and dissimilarities between its amino acid
investigation.                                                  composition and that of partnered S. album (Radomiljac
   The dry matter gains of S. album grown at 33 weeks           et al. 1998b). The analyses of net C and N gains of S.
were significantly improved when S. album was separately        album and the C: N ratios of xylem solutes of S. album
partnered with the three legume hosts, Sesbania formosa,        between the parasite-host associations showed that the
Acacia trachycarpa, and A. ampliceps compared with the          heterotrophic gains of C from xylem of the three legume
hemi-parasite grown with Eucalyptus camaldulensis or            hosts was highest in S. album partnered with A. ampliceps
without a host (Radomiljac et al. 1999b). They proposed S.      (57.9 % of total carbon) and lowest in S. album and S.
formosa to be best host, followed by A. ampliceps, A.           formosa (34.6 %) over a 9-week period (Radomiljac et al.
trachycarpa, and E. camaldulensis (Radomiljac et al.            1999b). This is similar to the study of Tennakoon et al.
1999b). Based on assays of leaf, stem, bark, and root tissue    (1997b) in which S. acuminatum probably would gain more
of S. album and its hosts, net increases in mineral contents    than one-third of its C requirement for dry matter pro-
of S. album over the first 9 weeks were obtained when           duction heterotrophically from the xylem of its hosts.
attached to a beneficial host. In particular, some elements     Foliar N concentrations of S. album were significantly
such as Ca, K, P, and Na were greatest when associated          greater than corresponding hosts and higher when on the
with hosts richest in corresponding elements. S. album          N2-fixing hosts than on E. camaldulensis, or without a host
foliage became more abundant in Na and in some cases            (Radomiljac et al. 1999c). When S. austrocaledonicum,
also in P and N compared with associated hosts. By con-         distributed in New Caledonia, was associated with A.
trast, net losses or only small gains of P, K, Ca over the      spirorbis, psydrax odorata, Diospyros pustulata, or Cleis-
study interval in S. album grown alone or associated with       tanthus stipitatus, an analysis of foliar mineral composition
E. camaldulensis indicated poor nutrient uptake ability         showed that nitrogen levels were particularly high when A.
through its own root system. A previous study on mineral        spirorbis served as the host (Veillon and Jaffré 1995).
nutrition of S. spicatum with its preferred host, Acacia        These results indicate that Santalum directly gained xylem
acuminata, showed high levels of K and Na, a high K/Ca          N and C from N2-fixing legumes hosts and that the parasite
ratio, and low levels of Zn in the parasite compared to the     obtained little N and C from the xylem sap of non-bene-
host plant (Struthers et al. 1986). In this interaction, host   ficial hosts such as E. camaldulensis.
seedlings are planted in the first year while untreated seeds      In addition, xylem sap of hosts contained variable
of S. spicatum are sown directly in the second or third year,   amounts of sucrose, glucose, and fructose, whereas that of
although Woodall and Robinson (2002) found that simul-          matching parasites was dominated by fructose in S. album
taneous sowing of both S. spicatum and A. acuminata             (Radomiljac et al. 1998b). Similarly, the levels of sucrose,
improved germination, survival, and growth of the former.       fructose, glucose, malate, and citrate were high in all saps,
Woodall and Robinson (2003) noted that S. spicatum par-         and fructose was especially prominent in S. acuminatum
asitized 68 hosts in remnant populations in Western Aus-        (Tennakoon et al. 1997b). Using 14C, glucose was found to
tralia (Table 2). These studies provide some evidence that      move from the host Myoporum parvifolium to S. acumi-
a beneficial host can supply nutrients as a direct result of    natum (Loveys et al. 2001a). Dissimilarities were also
123
Planta (2016) 243:847–887                                                                                                 861
                                                                                                                   123
      Table 3 Explant source, size, and surface sterilization procedures for preparation of tissue culture studies of sandalwood (chronological listing)
                                                                                                                                                                                                  862
Species Explant source Explant type, size and density; culture vessel Surface sterilization and preparation References
123
      S. album     Mature fruit. Age of mother plant NR               Seeds, ZEs, endosperms. Exact size of explant        Fruits ? CW 10 min                            Rangaswamy and Rao
                                                                       NR. Culture tube and dimensions NR. 15 ml                                                          (1963); Rao (1965);
                                                                       media/tube. Explant density NR                                                                     Rao and Rangaswamy
                                                                                                                                                                          (1971)
      S. album     Stem segments from 4-week-old in vitro             Stem segments (size NR). 5 mm long                   NR                                            Rao and Bapat (1978);
                     seedlings. Age of mother plant NR                  hypocotyls segments from seedlings for plant                                                      Bapat and Rao (1979);
                                                                        regeneration and callus culture. Culture vessels                                                  Shekhawat et al.
                                                                        NR (tubes from photos). Explant density NR                                                        (2008, 2010)
      S. album     Shoot segments and shoot tips of [20-year-old      5–6 mm diameter shoots cut into 5–6 mm long          Shoot segments and shoot tips ? DW ? 0.1 %    Lakshmi Sita et al.
                    trees                                               explants (shoot segments). Shoot                    HgCl2 10 min ? SDW (multiple washes)          (1979, 1980b);
                                                                        tips = 5 mm. Culture vessels NR (text tubes                                                       Lakshmi Sita and
                                                                        and Petri dishes from photos). Explant density                                                    Sobha Rani (1983);
                                                                        NR                                                                                                Lakshmi Sita (1986)
      S. album     Green seeds (6-8 mm). Age of mother plant NR       Endosperm from seeds. Other conditions, as for       NR                                            Lakshmi Sita et al.
                                                                       Lakshmi Sita et al. 1979                                                                           (1980a); Lakshmi Sita
                                                                                                                                                                          (1986)
      S. album     NR                                                 Achlorophyllous shoots derived from callus           NR                                            Bhaskar and Rao (1983)
      S. album     Juvenile shoots from mature tree, green fruits,    The cut ends of shoot segments were sealed with      Shoot segments, green fruit and mature        Rao and Raghava Ram
                     mature seeds                                      molten wax, Explant size, explant density,           seeds ? detergent soap (conc. and duration    (1983)
                                                                       culture vessel type and dimensions NR (test          NR) ? tap water (duration NR) ? 0.1 %
                                                                       tubes and Petri dishes assumed from photos)          HgCl2 (w/v) 5-8 min ? SDW (multiple
                                                                                                                            washes)
      S. album     Seeds ? in vitro seedlings. Age of mother plant    5 mm hypocotyl segments from 4-week-old              HgCl2 (conc. NR) 5 min ? SDW (6X) ?           Bapat and Rao (1984)
                    NR                                                  in vitro seedlings (shoot bud initiation).          sown on BM
                                                                        Hypocotyl segments with excised regenerated
                                                                        shoot buds (for SE). Culture vessel NR (tubes
                                                                        from photos). Explant density NR
      S. album     Juvenile shoots from 30-year-old trees. Cut        1 cm long nodal segments; 1.5 cm long                Shoots ? detergent water ? RTW ?              Rao et al. (1984)
                     ends immediately sealed by molten wax.             internode segments. Culture vessel and explant      0.1 % HgCl2 8 min ? 6X SW
                                                                        density NR
      S. album     4-week-old in vitro seedling. Juvenile shoots      Protoplasts from 5 mm long hypocotyls                Protocol for seedling and stems NR. Leaves:   Bapat et al. (1985)
                     from 30-year-old tree; first 3–4 young leaves     segments of seedlings, callus culture of stem        0.1 % HgCl2 ? SDW (multiple washes)
                     from apex. Age of mother plant NR                 and leaves. Culture vessel NR (tubes and Petri
                                                                       dishes from photos). Explant density NR
      S. album     Shoot segments of 20-year-old trees                Shoot segments ? callus ? suspension                 NR                                            Ozias-Akins et al.
                                                                       culture ? protoplast isolation ? protoplast                                                        (1985)
                                                                       culture ? SEs. Explant size, culture vessel
                                                                       and explant density NR
      S. album     Shoot segments of 20-year-old trees.               Protoplast from 4 to 5-days-old suspension           NR                                            Rao and Ozias-Akins
                    Embryogenic cell suspension cultures from          culture. Subculture in 100 ml Erlenmeyer flask                                                     (1985)
                    3-year-old callus cultures                         containing 6–8 ml suspension/14 ml medium
                                                                       (cell suspension culture). 2 ml/6 cm Petri dish.
                                                                       1–5 9 105 protoplasts/ml (protoplast culture)
                                                                                                                                                                                                  Planta (2016) 243:847–887
      Table 3 continued
      Species      Explant source                                  Explant type, size and density; culture vessel      Surface sterilization and preparation          References
      S. album     Young shoots from 20-year-old mother plant      Internode segments (5 mm long). Density and         HgCl2 (conc. NR) 7–8 min ? SDW (multiple       Bapat and Rao (1988)
                    immediately sealed at both cut ends              culture vessel NR. SEs embedded and                washes)
                                                                     suspended at 10 beads/flask (100 ml)
      S. album     Stem internodes of young shoots from 20-year-   Details not available from original protocol        Details not available from original protocol   Bapat and Rao (1992a);
                     old tree                                       (Bapat and Rao 1989)                                (Bapat and Rao 1989)                           Bapat et al. (1996)
                                                                                                                                                                                               Planta (2016) 243:847–887
      S. album     4-week-old fruits. Age of mother plant NR       Endosperm. Exact size of explants, explant          NR                                             Sankara Rao et al.
                                                                    density and culture vessels NR                                                                     (1996); Shiri and Rao
                                                                                                                                                                       (1998)
      S. album     Tender and thicker stem shoots. Age of mother   Shoot tips, nodal explants, and leaves. Test tube   RTW ? few drops detergent ? 1-2 DW wash        Muralidharan (1997)
                    plant NR                                        (borosilicate glass, 150 mm 9 25 mm or              (for all explants) ? 0.05 % HgCl2 5 min for
                                                                    100 mm 9 25 mm). Explant density NR                 tender stem; 0.1 % HgCl2 5 min for thicker
                                                                                                                        stem and leaves; 0.5–1.0 % HgCl2 5–10 min
                                                                                                                        for shoot tip and nodal explants. Rinses NR
      S. album     Seeds. Age of mother plant NR                   Zygotic embryo from 10 days in vitro                NR                                             Rai and McComb
                                                                    germinated seeds                                                                                   (1997)
      S. album     Nodes and hypocotyls from in vitro-germinated   Explant size, density NR. Culture vessel NR         NR                                             Das et al. (1998)
        ‘Elite      seedlings. Age of mother plant NR
        Kerala’
      S. album     Seeds and nodes from mature, superior tree.     To compare with field-derived explants, in vitro-   Seeds without pericarp ? single nodal          Rugkhla and Jones
        614, S.     Seeds harvested from fruit with a green to      derived leaves and nodal segments were also         segments: commercial soap (1 %)                (1998)
        spicatum    reddish pericarp                                used. Exact size of explants and age of mother      5–10 min ? 1 % NaOCl 15 min ? 5X SDW
        S107                                                        plants NR. Explant density and culture vessels
                                                                    NR
      S. album     Stem of 30-year-old tree.                       Stem and hypocotyl segments: size NR                NR                                             Bapat and Rao (1999)
                     Age of seedlings NR
      S. album     Seeds ? in vitro seedlings.                     Seedling hypocotyls (10–15 mm long). Density        NR                                             Das et al. (1999)
                    Age of mother plant NR                          and culture vessel NR for embryogenic callus
                                                                    production. Embryogenic callus used for
                                                                    bioreactor (liquid media) and test tube (solid
                                                                    media) trials
      S. album     Seeds ? in vitro seedlings.                     Seedling hypocotyls (size NR). Density and          NR                                             Das et al. (2001)
                    Age of mother plant NR                          culture vessel NR for embryogenic callus
                                                                    production. Embryogenic callus used for liquid
                                                                    media trials in 250-ml Erlenmeyer flasks
      S. album     Endosperm. Age of mother plant NR               Endosperm callus. Culture vessel and explant        NR                                             Anil and Rao (2000)
                                                                    density NR
      S. album     Endosperm from 4-week-old fruit                 Endosperm ? callus ? callus proliferation and       NR                                             Anil et al. (2000)
                                                                    SE induction ? PEM ? SE maturation.
                                                                    Culture vessel and explant density NR in
                                                                    suspension culture. Torpedo and cotyledonary
                                                                    stage SE at 21 days used
                                                                                                                                                                                               863
123
      Table 3 continued
                                                                                                                                                                                                      864
Species Explant source Explant type, size and density; culture vessel Surface sterilization and preparation References
123
      S. album    20-year-old candidate plus tree                     Nodal segments (1.5–2.0 cm, trimmed to            RTW 30 min ? soap ? 4 % NaOCl                     Radhakrishnan et al.
                                                                       1–1.5 cm after disinfection)                      4 min ? 0.1 % HgCl2 10 min ? SDW                  (2001)
                                                                                                                         2–3 min
      S. album    Seeds ? in vitro seedlings. Age of mother plant     Hypocotyls and stem nodes (size NR). Culture      NR                                                Ilah et al. (2002)
                   NR                                                  vessel NR
      S. album    Mature seeds from 50 to 60-year-old elite tree      Zygotic embryos. 200-ml glass jars with 35 ml     Seeds: deionized water overnight ? 2 %            Rai and McComb
                                                                       medium/jar for induction of somatic               NaOCl ? 0.005 % Tween-20                          (2002)
                                                                       embryogenesis. 25 9 100 mm test tubes with        10-15 min ? 3X SDW. Seeds air-dried in
                                                                       15 ml medium/test tube for somatic embryo         laminar flow bench for 10 min prior to
                                                                       conversion to plantlets                           excision of zygotic embryos
      S. album    Seeds. Age of mother plant NR                       GA3 treated seeds. Culture vessel and density     Seeds ? 0.15 % HgCl2for 8 min ? SDW               Sanjaya and Rai (2003)
                                                                       NR
      S. album    Leaves from 3 to 4-week-old in vitro seedlings      Intact leaves or half leaves (sections cut        Seeds: 0.1 % HgCl2 4 min ? 3X SDW                 Mujib (2005)
                                                                        perpendicular to the mid-vein) 5–15 mm long;
                                                                        adaxial and abaxial surfaces of the laminae
                                                                        tested separately
      S. album    In vitro shoots derived from in vitro subcultured   Shoot tip size and age of donor plant NR. Jam     NR                                                Primawati (2006)
                    shoots. Age of mother plant NR                     bottles (13 cm high, 7 cm diameter)
      S. album    Nursery seeds (for rootstocks; 2006a) and           Nodal shoot segments (2.5–3.5 cm long) with       Decoated seeds for in vitro rootstocks (2006a):   Sanjaya et al. (2006a, b)
                   50–60-year-old tree (high-yielding oil:             dormant axillary buds, harvested in Nov-Jan.      0.05 % GA3 overnight ? 0.075 % HgCl2
                   4–5 %; 2006a, 2006b) for scions                     25 9 100 mm test tubes (one seed/tube; 25 ml      6-7 min ? 6-8X SDW. Nodal segments from
                                                                       medium/tube)                                      50-60-y-old tree for scions (2006a, 2006b):
                                                                                                                         70 % EtOH 30-40 s ? 0.075 % HgCl2
                                                                                                                         6–7 min ? 6-8X SDW
      S. album    Mature stem segments from elite tree (age NR)       1 cm long stem segments (nodes or internodes?).   0.1 % HgCl2 5 min ? 2-3X SDW                      Shekhawat et al. (2008)
                                                                        100 ml Erlenmeyer flasks: 200 mg of friable
                                                                        embryogenic callus tissue in 20 ml of liquid
                                                                        medium
      S. album    Young shoots from elite mature tree (age NR)        1 cm long stem segments, 80 9 150-mm              Young shoots ? RTW 30 min ? 0.1 % HgCl2           Ma et al. (2008)
                                                                        (diameter 9 height) culture jars, explant        10 min ? SDW 3X
                                                                        density NR
      S. album    Top shoots, young leaves, and seeds. Age of         Top shoots, leaves of 0.5 cm2, seeds              Top shoots and leaves ? 0.1 % HgCl2               Mo et al. (2008)
                   mother plant NR                                                                                       10 min ? SDW 5X
                                                                                                                        Seeds ? RTW ? peel pericarps ? 0.1 %
                                                                                                                         HgCl2 10 min ? SDW 5-6X
      S. album    Fruits collected in May from tree (age NR)          Seed. Viability tested with 2,4,5-triphenyl       Fruits soaked overnight in water ? DW             Nikam and Barmukh
                                                                       tetrazolium chloride (TTC) before use. 1 or 2     3X ? soap solution 30 min ? 0.1 % HgCl2           (2009)
                                                                       seeds/culture tube                                3 min ? SDW 3X. Seeds ? 0.1 % HgCl2
                                                                                                                         3 min ? SDW 3X ? 4 mM GA3
                                                                                                                         12 h ? SDW 3X
                                                                                                                                                                                                      Planta (2016) 243:847–887
      Table 3 continued
      Species      Explant source                                    Explant type, size and density; culture vessel      Surface sterilization and preparation              References
      S. album     Immature seeds and mature seeds, 10-year-old      ZEs                                                 Seeds ? peel pericarps ? 70 % EtOH                 Mo et al. (2010)
                    tree                                                                                                  1 min ? 5-10 % NaClO 5–20 min ? 0.1 %
                                                                                                                          HgCl2 5-15 min ? SDW 4-5X
      S. album     Seeds of 8-year-old plants ? in vitro seedlings   Internodes (8–10 mm) from 2-months-old              Seeds: RTW 20 min ? * 2 % Tween-20                 Janarthanam and
                                                                       seedlings. 25 9 150 mm culture tubes.              1 min ? SDW ? 0.1 % HgCl2 5 min ? 4X                Sumathi (2011);
                                                                                                                                                                                                      Planta (2016) 243:847–887
123
866                                                                                                                                                                                                                                                                                                                                                               Planta (2016) 243:847–887
                                                                                                                         BM basal medium (in mg/l: KINO3 (1900), NH4NO3 (1650) CaC12.2H2O (440), MgSO47H2O (370), KH2PO4 (170), MnSO44H2O (25), H3BO3 (10), ZnSO47H2O (13.9), Na2EDTA (18.6),
                                                                                                                         myo-inositol (100), nicotinic acid (5), folic acid (5), glycine (2), pyridoxine–HCl (0.5), thiamine-HCI (0.5), biotin (0.05), sucrose (20 g/l), Difco bacto agar (6 g/l) modified WB according to
                                                                                                                         chloride, NaOCl sodium hypochlorite, NR not reported in the study, PEM pro-embryogenic masses, rpm revolutions per minute, RTW running tap water, SDW sterilized (by autoclaving)
                                                                                                                         Rangaswamy (1961)), CW chlorine water, DAG day(s) after germination, DW distilled water, DDW double distilled water, EtOH ethyl alcohol (ethanol), GA3 gibberellic acid, HgCl2 mercury
                                                                                                                                                                                                                                                                                                                             et al. (2014) found that the inter-collapsed layers, an
                                                                                                                                                                                                                                                                                                                             important structure within haustoria, might be involved in
                                                                     Peeris and Senarath                                                                                                                                                                                                                                     cell inclusion and energy concentration at the inner
                                                                                                                                                                                                                                                                                                                             meristematic region and these cell inclusions and energy
                    References
                                                                                                                                                                                                                                                                                                                             Applied biotechnologies
Table 3 continued
123
      Table 4 In vitro conditions for tissue culture studies of sandalwood (chronological listing)
      Studied        Culture medium, PGRs, additives, subculturesb       Culture conditionsc                   Experimental outcome, maximum productivity,          References
      sandalwooda                                                                                              acclimatization and variation
      S. album       mWM ? 20 % CM ? 400 mg/l CH (SGM).                  PP NR. Diffused light (LI NR).        SG produced seedlings in 5 weeks. In seed            Rangaswamy and Rao
                      mWM ? 2 mg/l 2,4-D ? 5 mg/l Kin ? 0.25 %            25 ± 2 °C. 50–60 % RH                 culture, 30–40 % of seeds initially started to       (1963); Rao (1965)
                      YE (seed culture). pH 5.8. 4 % sucrose. Difco                                             germinate but did not convert to seedlings.
                      bacto agar 0.8 %                                                                          60–70 % of cultures showed no sign of
                                                                                                                                                                                               Planta (2016) 243:847–887
123
      Table 4 continued
                                                                                                                                                                                                 868
      Studied       Culture medium, PGRs, additives, subculturesb     Culture conditionsc                          Experimental outcome, maximum productivity,          References
      sandalwooda                                                                                                  acclimatization and variation
123
      S. album      MS ? 1-2 mg/l 2,4-D or MS ? 0.5–2 mg/l            As for Lakshmi Sita et al. 1979              Embryoid formation in 4–6 weeks. Organogenesis       Lakshmi Sita et al.
                     BA ? 1 mg/l NAA (CIM). MS ? 1 mg/l 2,4-D                                                       not quantified. Acclimatization NP                   (1980a)e, b; Lakshmi
                     (callus subculture). MS ? 1–2 mg/l GA3                                                                                                              Sita (1986)
                     (SEIM). MS ? 0.3 mg/l BA ? 1 mg/l
                     IAA ? 0.3 mg/l Kin ? 1 mg/l GA3 (SEMM).
                     WB ? 0.5 mg/l IAA (RIM). Shake cultures
                     using callus in 250-ml flasks at 70 rpm and pH
                     5.2 (1980b). Other conditions as for Lakshmi
                     Sita et al. (1979), or unclear
      S. album      1–3 mg/l NAA (RIM). Other conditions NR           NR                                           In vitro-derived shoots cultured in pots with host   Bhaskar and Rao (1983)
                                                                                                                     Cassia siamea, leading to plantlet formation
      S. album      MS ? 1 mg/l 2,4-D alone or in combination with    Continuous light. 1000 lux. 25 ± 2 °C.       Within 3 weeks, callus formed on surface of          Rao and Raghava Ram
                     0.2 mg/l Kin (CIM). MS ? 1 mg/l                   55 % RH. At SE germination stage,            endosperm. During 6 weeks, callus proliferated       (1983)
                     IAA ? 1 mg/l BA (SEIM). MS ? 1 mg/l               cultures kept in dark for 72 h then          well. SE formation observed within 4 weeks
                     IAA ? 0.5 mg/l IBA ? 0.5 mg/l GA3 (SE             transferred to continuous light for 4–6      from callus obtained on CIM. Plantlets with 2–3
                     germination). pH, 5.8. 2 % sucrose (CIM) or       weeks                                        pairs of leaves with roots developed within 4
                     5 % (SEIM, SE germination). 0.6 % agar                                                         weeks and transferred to vermiculite then
                                                                                                                    acclimatized in earthen pots with soil
      S. album      mBM ? 1 mg/l NAA or 1 or 2 mg/l BA (SIM).         PP NR. CWFT. 1000 lux. 25 ± 2 °C. RH         Normal plantlets produced (time period NR).          Bapat and Rao (1984)e
                     mBM ? (0.5 mg/l NAA ? 5 mg/l IBA) or              55–60 %                                      Acclimatized for 3 w in Hoagland’s nutrient
                     1 mg/l BA (RIM). mBM ? 0.5 mg/l or 1 mg/l                                                      solution (Hoagland and Arnon 1938). 10 %
                     IAA (SEIM). mBM ? 0.4 % YE ? 400 mg/l                                                          survived in field without host plant. 90 % of the
                     CH ? 400 mg/l CA (SEMM). mBM ? 1 mg/l                                                          basal region of hypcotyl explants differentiated
                     IAA or NAA (PCM)                                                                               into buds. Insignificant effect of seedling age.
                                                                                                                    Rapid response on liquid medium than on agar
                                                                                                                    medium. 100 % response on hypocotyl explant
                                                                                                                    orientated with root end in direct contact with
                                                                                                                    medium. 20 cm long plantlets obtained on RIM.
                                                                                                                    4 % sucrose ? 1650 mg/l NH4NO3 best for SE
                                                                                                                    induction
      S. album      MS ? 0.5 or 1 mg/l BA (SIM). MS ? 1 mg/l 2,4-     Initial 72 h darkness for root induction.    Shoot buds obtained from nodes did not respond       Rao et al. (1984)e
                     D or MS ? 1 mg/l 2,4-D ? 0.2 mg/l Kin              All other conditions as in Bapat and Rao    to rooting. Shoots obtained from SEs of
                     (CIM). MS ? 1 mg/l IAA ? 1 mg/l BA                 (1984)                                      internode-derived callus resulted in successful
                     (SEIM). 2 % sucrose. 0.7 % agar. pH 5.6.                                                       plantlet conversion and 10 % survival in field
                     MS ? 1 mg/l IAA ? 0.5 mg/l IBA ? 0.5 mg/l                                                      conditions
                     GA3 (SEMM). 5 % sucrose. 0.6 % agar
                                                                                                                                                                                                 Planta (2016) 243:847–887
      Table 4 continued
      Studied       Culture medium, PGRs, additives, subculturesb         Culture conditionsc                        Experimental outcome, maximum productivity,          References
      sandalwooda                                                                                                    acclimatization and variation
      S. album      MS ? 1 mg/l 2,4-D or BA (CIM for hypocotyl).          As for Bapat and Rao (1984)                Effect of explant source on protoplast isolation     Bapat et al. (1985)e
                     MS ? 1 mg/l 2.4-D or 1 mg/l 2,4-D ? 0.5 mg/l                                                     efficiency. Maximum number of SEs induced on
                     Kin (CIM for stem). MS ? 1 mg/l 2,4-D (PCM                                                       stem-derived callus cultured on  MS ? 1 mg/l
                     for hypocotyl callus). MS ? 1 mg/l                                                               IAA. Plantlet conversion from stem callus-
                                                                                                                                                                                                       Planta (2016) 243:847–887
                     IAA ? 1 mg/l BA (SEIM from stem callus).                                                         derived SEs. No SE induction from leaf- and
                     Modified V47 medium ? 1 mg/l 2,4-                                                                hypocotyl-derived callus
                     D ? 1 mg/l NAA ? 1 mg/l BA (protoplast
                     proliferation medium for stem callus).
                     MS ? 1 mg/l IAA or MS ? 1 mg/l
                     IAA ? 1 mg/l BA, or  MS ? 1 mg/l IAA or
                      MS ? 10 % CM ? 500 mg/l CH (SEIM
                     from stem callus). SEMM NR. Medium for leaf-
                     derived protoplast culture NR
      S. album      CIM NR ? suspension culture (composition              NR                                         SEs obtained from protoplast derived culture.        Ozias-Akins et al. (1985)e
                     NR) ? subculture (0.5 or 1 mg/l 2,4-                                                             Organogenesis not NR but complete plants
                     D) ? liquid or gelled media (0.1–2 mg/l BA)                                                      claimed to have formed from SEs
                     (details NR) ? protoplast isolation ? V47
                     medium (750 mOs/kg H2O, adjusted using
                     mannitol) (PCM) ? MS medium (IBA ? BA
                     conc. NR). Gelling agent, pH, carbon source and
                     other conditions NR
      S. album      MS ? 2,4-D (0.5–2.5 mg/l) ? 1 mg/l folic acid         PP NR. Continuous diffused light. LI NR.   Club and heart shaped stages of SE obtained from     Rao and Ozias-Akins
                     (liquid SEIM). 3.4 % sucrose (CSC). Liquid MS         26 °C. Gyrotary shaker at 150 rpm (for     different callus cell lines on media with BA and     (1985)
                     or MS ? agar either with Zea (0.2, 0.35 mg/l),        suspension culture)                        2,4-D. Secondary SEs obtained from cell
                     BA (0.1, 0.5, 1.0, 2.0 mg/l) or BA (0.1, 0.5, 1.0,                                               suspension culture on MS containing 0.1 and
                     2.0 mg/l) ? 0.01 mg/l 2,4-D (SEM). MS or                                                        1 mg/l BA. SE successfully converted to
                     MS, alone or MS or  MS ? BA (0.1 or 1 mg/                                                       plantlets. SEs from protoplast did not form roots
                     1) or 1 mg/1 IAA or 1 mg/1 GA3 ? 0.2 mg/l
                     BA (SEMM). MS ? agar or filter-paper bridge
                     on mWBM ? 0.5 mg/l IAA or combination of
                     0.1 mg/l IAA ? 0.5 mg/l IBA ? 0.5 mg/l GA3
                     (SGM). Protoplast culture: V47 medium (750
                     mOs/kg H2O). pH 5.8 (PCM). MS ? 1 mg/l
                     IAA ? 1 mg/l BA or 400 mg/l casamino acid
                     (SEIM from protoplasts). MS ? 1 mg/l BA
                     (SEMM from protoplasts). WM ? 0.5 mg/l
                     IAA (plantlet conversion from callus-derived
                     SE).  MS (only major elements?) or
                     WM ? 1 mg/l IAA or 0.5 mg/l IBA or 1/3 mg/l
                     GA3 ? 4 or 5 % sucrose ? 0.6 % agar
                     (germination for SE from protoplasts).
                     Subculture cell suspension cultured every 4–5
                     days
                                                                                                                                                                                                       869
123
      Table 4 continued
                                                                                                                                                                                                    870
      Studied       Culture medium, PGRs, additives, subculturesb      Culture conditionsc                     Experimental outcome, maximum productivity,             References
      sandalwooda                                                                                              acclimatization and variation
123
      S. album      MS ? 1 mg/l 2,4-D (CIM). MS ? 0.3 mg/l IAA         Suspension of beads under continuous    Embryogenic cells encapsulated in 3 % alginate          Bapat and Rao (1988)e
                     or 0.5 mg/l GA (SEIM, as a suspension culture).    light. 950 lux. 25 ± 2 °C               bead showed plantlet conversion after 16 weeks.
                     MS ? 0.5 mg/l BA ? 0.5 mg/l IAA (secondary                                                 However, low synseed germination (10 %)
                     SEs). Gelling agent and pH NR. 5 % sucrose for
                     SE germination
      S. album      MS ? 87.6 lM sucrose ? 4.52 lM 2,4-D (CIM).        Suspension of beads under continuous    SEs isolated and desiccated for 10, 20 or 30 days.      Bapat and Rao (1992a);
                     MS ? IAA 2.85 lM ? BA                              light. 1000 lux. 25 ± 2 °C. 80 rpm      One lot of desiccated SEs encapsulated in 3 %           Bapat et al. (1996)e
                     2.22 lM ? 87.6 lM sucrose (SEM).                                                           sodium alginate gel (control = non-                     (using protocol
                     MS ? 87.6 lM sucrose or WM ? 58.4 lM                                                       encapsulated SEs). Both encapsulated and non-           originally from Bapat
                     sucrose (SEIM) for 4 w. WM ? 58.4 lM                                                       encapsulated SEs showed revived growth after            and Rao (1989)
                     sucrose ? 18.92 lM ABA (plantlet conversion)                                               rehydration on WM and developed into plants.
                    2. Synthetic seed: Encapsulation of SE according                                            The desiccation tolerance and regeneration of
                      to Bapat and Rao (1988)                                                                   plants was dependent on the pre-treatment given
                                                                                                                to SEs. In Bapat et al. 1996, the addition of a
                                                                                                                cyanobacterial extract (Plectonema boryanum
                                                                                                                strain UTX594) promoted callus formation in
                                                                                                                the absence of PGRs
      S. album      MS ? 1 mg/l 2,4-D ? 1 mg/l BA or 2 mg/l 2,4-       NR                                      4 stages of somatic embryogenesis claimed, with         Sankara Rao et al. (1996)e
                     D ? 0.5 mg/l Kin (CIM). MS ? 1 mg/l 2,4-                                                    distinct biochemical profiles
                     D ? 3 % sucrose (SEIM). PGR-free MS ? 2 %
                     mannitol (SE differentiation). PGR-free MS
                     with or without mannitol (SE maturation). 0.6 %
                     agar
      S. album      MS ? 0.5 lM BA ? 0.5 lM Kin (SIM).                 16-h PP. CWFT. 18 lE m-2 s-1.           Callus produced from intermodes on CIM. 4 shoot         Muralidharan (1997)
                     MS ? 0.5-4 lM 2,4-D (CIM). MS ? 0.5–2 lM           25 ± 2 °C                               buds/nodal explant on SIM. Shoot tips failed to
                     IBA (RIM). pH 5.7. 2 % sucrose. 0.5 % agar.                                                respond. Plant regeneration was not possible
                     Subcultured every 4 weeks
      S. album      MS ? 20 % CM ? CH or 1 lg/l Kin (SGM;              16-h PP. Light source NR. 40 lmol m-2   91.6 % of explants induced SEs, forming 14.23           Rai and McComb 1997e,
                     1997). MS ? 2 mg/l BA (1997) or 4.5 lM TDZ         s-1. 25 ± 1 °C                          SEs/explant after 8 w. 91.6 % of primary SEs            (2002)e
                     (2002) (SEIM). PGR-free MS (SEMM).                                                         formed secondary SEs, forming 20.5 SEs/
                     MS ? 0.5 mg/l IAA (1997) or 2.8 lM GA3                                                    primary SE after 8 weeks. 81.2 % of SEs
                     (2002) (SE conversion). pH 5.8. 3 % sucrose.                                               germinated after 8 w. From the same treatment,
                     0.8 % agar (SEIM, SEMM) or 0.15 % Phytagel                                                 72.3 % of plants survived in the field after initial
                     (SE conversion)                                                                            acclimatization in sand ? soil ? FYM (2:1:1)
                                                                                                                and 1-2 seeds of red gram (Cajanus cajan) as the
                                                                                                                primary pot host. Most details not explained in
                                                                                                                1997 paper
      S. album      MS minerals ? B5 vitamins ? 0.5 mg/l BA            PP NR. CWFLT. 1500 lux. 26 ± 2 °C.      25–60 shoots/SEs from hypocotyls, and only 3–5          Das et al. (1998)e
        ‘Elite       (SIM). MS minerals ? B5 vitamins ? 0.5 mg/l        60–70 % RH                              from nodes
        Kerala’      BA ? 0.5 mg/l IAA (SEIM). pH 6.0. 4 %
                     sucrose
                                                                                                                                                                                                    Planta (2016) 243:847–887
      Table 4 continued
      Studied       Culture medium, PGRs, additives, subculturesb         Culture conditionsc                         Experimental outcome, maximum productivity,          References
      sandalwooda                                                                                                     acclimatization and variation
      S. album      MS ? 5 lM BA (SIM). MS ? 5 lM                         SEIM: PP and light source NR.               S. album nodal segments: 100 % explants formed       Rugkhla and Jones (1998)
        614, S.      BA ? 2 lM GA3 (for leaf enlargement).                 2 lmol m-2 s-1. SEMM: 16-h PP.               green SEs, 72 % formed white SEs (2 lM
        spicatum     MS ? 1-2 lM TDZ (SEIM). MS ? 6 lM                     Light source NR. 50 lmol m-2 s-1.            TDZ), 64 % formed friable embryogenic tissue
        S107         IAA ? 1 lM Kin (SEMM). MS ? 6 lM GA3                  25 ± 1 °C                                    (2 lM TDZ). S. album seed: 0 % explants
                                                                                                                                                                                                      Planta (2016) 243:847–887
                     (SE germination) ? 3 lM GA3 (SE elongation)                                                        formed green SEs, 96 % formed white SEs and
                     (S. album) and with 250 mg/l CH ? 5 % CW                                                           friable embryogenic tissue (2 lM TDZ). S.
                     (S. spicatum). 6-w subculture in SEIM, then 3-w                                                    spicatum nodal segments: 20 % of explants
                     subculture during SE maintenance. pH 5.8. 2 %                                                      formed primary and secondary SEs. Rooting
                     sucrose. 0.2 % gelrite                                                                             was problematic but overall plantlet growth was
                                                                                                                        improved on liquid medium. Acclimatization
                                                                                                                        NP
      S. album      MS ? 1 mg/l 2,4-D ? 1 mg/l BA (CIM).                  14-h PP. CWFT. 5 (callus, SEs) ? 200        Pricked torpedo–cotyledonary stage SEs               Shiri and Rao (1998)e
                     MS ? 1 mg/l 2,4-D for 3 w (SEIM). PGR-free            (plantlets) lE m-2 s-1. 26 ± 2 °C           (0.75–1.2 cm) from a Sankara Rao et al. (1996)-
                     MS ? 2 % mannitol (SE differentiation). PGR-                                                      derived line. Plantlets ardened to the greenhouse
                     free MS with or without                                                                          simply by growing on paper bridges overlaying
                     mannitol ? WB ? 0.5 mg/l IAA                                                                      liquid WB. SEs genetically transformed with
                     (SE ? plantlets). 3 % sucrose. Agar conc. NR                                                      Agrobacterium tumefaciens harboring
                                                                                                                       LBA4404/pKIWI105 (see text for details).
                                                                                                                       Success of regeneration and genetic
                                                                                                                       transformation not quantified
      S. album      MS ? 1 mg/l IAA (SEIM). No other SEIM                 16-h PP. CWFT. 24 lmol m-2 s-1.             3000 seedlings derived from bioreactor in 6 w (vs    Das et al. (1999)e
                     conditions described. Initial pH (bioreactor) 5.8.    24 ± 2 °C. 60–70 % RH                       800 in 12 w on solid medium): 59.3 % vs
                     2000 ml in a 3.5-L airlift bioreactor (25 g                                                       88.9 % abnormality and 31.1 vs 7.7 SEs/10 ml
                     embryogenic callus/l). MS ? 1 mg/l                                                                in former vs latter, respectively
                     BA ? 0.5 mg/l ABA (bioreactor). Air-flow = 1
                     vvm. 3 % sucrose
      S. album      MS ? 1 mg/l BA ? 1 mg/l 2,4-D (CIM).                  PP and light source NR. Diffused light of   Embryogenic callus consisted of two types of         Anil and Rao (2000)
                     MS ? 1 mg/l 2,4-D (SEIM). Liquid MS (PGR-             5 lEm-2 S-2. 26 °C ± 2 °C                   cells: (a) more cytoplasm that formed clumps;
                     free) ? 2 % mannitol (SEMM). Orbital shaker                                                       (b) less cytoplasm and elongated shape. Torpedo
                     at 100 rpm. 3 % sucrose. 3.9 mM CaCl2.                                                            and bipolar stages of SE collected after 21 days
                     Gelling agent and pH NR                                                                           of culture from first type of cells
      S. album      MS ? 4.52 mM 2,4-D (CIM; 2-w subcultures).            Light conditions NR. 25 ± 2 °C              57.35 % optimization of SE production. SEs           Das et al. (2001)e
                     MS ? 2.85 mM IAA ? 3.99 mM BA (SEIM 1;                                                            produced in 14 days
                     subcultures NR). WPM ? 2.85 mM
                     IAA ? 3.99 mM BA ? 40 mM
                     glutamine ? 0.33 M mannitol ? 11.6 mM
                     nitrate ? 7.89 mM ammonium ? 1.31 mg/l
                     ABA (SEIM 2; subcultures NR). 50 ml medium
                     in 250-ml Erlenmeyer flasks (12 g embryogenic
                     callus/l; 75 rpm). 3 % sucrose (CIM, SEIM 1) or
                     4 % (SEIM 2). pH NR
                                                                                                                                                                                                      871
123
      Table 4 continued
                                                                                                                                                                                              872
      Studied       Culture medium, PGRs, additives, subculturesb     Culture conditionsc                     Experimental outcome, maximum productivity,            References
      sandalwooda                                                                                             acclimatization and variation
123
      S. album      MS ? 4 mg/l BA (CIM, SIM). MS ? 3 mg/l IBA        16-h PP. Light source NR. 1000 lux.     Callus induced after 3 weeks. The inclusion of a       Radhakrishnan et al.
                     (RIM). pH 5.7. 2 % sucrose. 0.9 % agar            25 ± 2 °C                               seed extract of Cajanus cajan (red gram) in RIM        (2001)
                                                                                                               did not improve rooting
      S. album      BM NR ? 2.26 lM 2,4-D or 2.68 lM pCPA             PP and light source NR. 24 lmol m-2     2-w-old initial callus induced on CIM transferred      Ilah et al. (2002)e
                     (CIM). BM NR ? 2.70 lM NAA ? 2.22 lM              s-1. 24 ± 2 °C. 70–80 % RH               to SEIM. Liquid medium superior to solid
                     BA (SEIM). WPM (PGR-free) (SEMM).                                                          medium (depending on stage of SE). 53–68 %
                     5.71 lM IAA (RIM). pH, carbon source, gelling                                              of cultures showed abnormalities (aggregation
                     agent NR                                                                                   of pro-embryos and SEs, growth arrest,
                                                                                                                browning of SEs, SEs with no or poorly
                                                                                                                developed roots, roots with undeveloped shoot).
                                                                                                                83 % rooting
      S. album      PGR-free MS (seed germination).                   16-h PP. Light source NR. 40 lmol m-2   45-d-old seedlings used as rootstock in                Sanjaya and Rai (2003)
                     MS ? 11.12 lM BA (SIM). 3 % sucrose. 0.6 %        s-1. 25 ± 2 °C                          micrografting. The larger the scion used, the
                     agar                                                                                      more successful the micrograft: 1-2 cm scions
                                                                                                               resulted in 60 % graft success
      S. album      MS ? 0.44 and 2.22 lM BA (SIM). pH 5.8 (MS)       16-h PP. CWFT. LI NR. 25 ± 2 °C         Direct shoot formation from leaf explants              Mujib (2005)
                     or 5.2 (WPM). WPM ? 5.71 lM IAA (RIM).                                                    (13–20/explant) within 20–25 days. No auxins
                     3 % sucrose. 0.8 % agar                                                                   could induce shoots. Approx. 4-fold higher
                                                                                                               shoot bud production in liquid medium than in
                                                                                                               solid medium. Epiphyllous shoots produced
                                                                                                               when explants placed in horizontal position, but
                                                                                                               not when in the vertical position, but shoots
                                                                                                               from these buds developed slowly
      S. album      MS ? 1.5 mg/l BA ? 0.2 mg/l Kin ? 100 mg/l        NR.                                     1.4 shoots/shoot tip. No rooting or acclimatization    Primawati (2006)
                     glutamine (shoot tip development medium). 3 %                                              experiments. 17 % browning and contamination
                     sucrose
      S. album      PGR-free MS (SGM for rootstocks).                 12-h PP. CWFT. 60 lmol m-2 s-1.         Seeds were germinated in vivo and in vitro to          Sanjaya et al. (2006a)
                     MS ? 0.53 lM NAA ? 11.09 lM BA (SIM).             28 ± 1 °C                               assess micrografting, and 45-days-old seedlings
                     MS (liquid) ? 2 % sucrose on paper bridges                                                served as rootstocks. In vitro shoots (0.5–2.0 cm
                     (post-grafting). Subculture every 4 w. pH 6.0.                                            long) derived from third subculture were used as
                     3 % sucrose. 0.6 % agar                                                                   scions. 60 % of grafts were successful. 8-week-
                                                                                                               old grafted plantlets were successfully
                                                                                                               acclimatized (% success NR) in sterilized
                                                                                                               soilrite (60 lmol m-2 s-1; 25 ± 1 °C)
      S. album      MS ? 0.53 lM NAA ? 11.09 lM BA (SIM).             12-h PP. CWFT. 60 lmol m-2 s-1.         4.92 shoots/sterilized nodal shoot segment in          Sanjaya et al. (2006b)
                     SIM ? 283.93 lM AA ? 118.1 lM                     28 ± 1 °C. 60–65 % RH                    initial culture and 4.63 shoots/in vitro nodal
                     CA ? 104.04 lM cysteine ? 342.24 lM                                                        shoot segment during shoot multiplication.
                     glutamine ? 10 % CM (SMM). MS ? 2 %                                                       41.7 % of shoots could root in vitro. 50 % of
                     sucrose after 48-h pulse in 98.4 lM IBA.                                                   shoots could root in soilrite after treatment with
                     Subculture every 4 w. pH 6.0. 3 % sucrose.                                                 1230 lM IBA. 100 % survival of field-grown
                     0.6 % agar                                                                                 plantlets
                                                                                                                                                                                              Planta (2016) 243:847–887
      Table 4 continued
      Studied       Culture medium, PGRs, additives, subculturesb      Culture conditionsc                     Experimental outcome, maximum productivity,            References
      sandalwooda                                                                                              acclimatization and variation
      S. album      MS ? 5.0 lM BA ? 0.5 lM NAA (adventitious          14-h PP. CWFT. 40 lmol m-2 s-1.         5.7 shoots/shoot explant after 1 month of culture.     Ma et al. (2008)
                     shoot propagation) ? monthly subculture.           25 ± 2 °C                                Some adventitious roots within 1–3 months.
                     MS ? 250 lM IBA (RIM). pH 5.6. 3 %                                                          8 % of shoots formed roots. 95 % survival of
                     sucrose. 0.6 % agar                                                                         acclimatized plantlets in sand: peat soil: organic
                                                                                                                                                                                                Planta (2016) 243:847–887
123
      Table 4 continued
                                                                                                                                                                                                874
      Studied        Culture medium, PGRs, additives, subculturesb   Culture conditionsc                     Experimental outcome, maximum productivity,            References
      sandalwooda                                                                                            acclimatization and variation
123
      S. album       MS ? 4.44 lM BA ? 2.69 lM NAA (SGM).            16-h PP. CWFT. 2000 lux. 25 ± 2 °C      80 % SG. 60 % of internodes showed an                  Revathy and Arumugam
                      MS ? 13.5 lM 2,4-D (SEIM). MS ? 2.22 lM                                                 embryogenic response on SEIM within 4–6                (2011)e
                      BA ? 1.44 lM GA3 (SEM). MS ? 2.46 lM                                                   weeks. 65 % shoot elongation after 25 days.
                      IBA (RIM). pH 5.6. 3 % sucrose. 0.9 % agar                                              60 % of shoots rooted in RIM. 60 % survival of
                                                                                                              acclimatized plantlets in sterile
                                                                                                              soil ? sand ? vermiculite (1:1:1)
      S. album, S.   PGR-free MS (SIM). MS ? 2 lM                    16-h PP. CWFT. 30 lmol m-2 s-1. 25 °C   Shoot formation in 8 m. 13.5 % survival after          Baiculacula (2012)
        yasi, R1      BA ? 0.02 lM NAA (RIM). pH 5.7. 2 %                                                     shoot formation for S. yasi (results for S. album
        hybrids       sucrose. 0.7 % agar                                                                     and R1 hybrids NR). 19.1 % survival after root
                                                                                                              formation for S. album (results for S. yasi and
                                                                                                              R1 hybrids NR)
      S. album       MS ? 1 mg/l 2,4-D ? 0.5 mg/l TDZ (direct and    Darkness for 1 w. 16-h (CIM, SIM) or    Direct somatic embryogenesis (11.44 %), indirect       Bele et al. (2012)e
                      indirect SEIM). MS ? 2 mg/l 2,4-D ? 0.5 mg/l    12-h (plantlets) PP. CWFT. LI and       somatic embryogenesis (54.23 %): 160.08
                      TDZ (indirect SIM). MS ? 2 mg/l 2,4-            source NR. 25 ± 2 °C                    SEs/explant; indirect organogenesis (20.38 %);
                      D ? 0.5 mg/l NAA (direct SIM; plantlet                                                  direct organogenesis (9.48 %); regeneration of
                      regeneration via direct organogenesis).                                                 plantlets via direct organogenesis (36.69 %);
                      MS ? 2 mg/l TDZ ? 1.0 mg/l GA3 (plantlet                                                plant regeneration via somatic embryogenesis
                      regeneration via somatic embryogenesis).                                                (163.63 %) or 141.25 % via indirect
                      MS ? 1 mg/l TDZ ? 0.5 mg/l GA3 ? 0.5 mg/l                                               organogenesis. Roots could not be induced from
                      NAA (plantlet regeneration via indirect                                                 any medium. Acclimatized plantlets in
                      organogenesis). pH 5.8. 3 % sucrose. 0.75 %                                             sand ? soil ? FYM (sterilized mixture; 1:1:1),
                      agar                                                                                    but survival not quantified. Protocol very
                                                                                                              complex and values [100 % difficult to
                                                                                                              interpret
      S. album       B5 ? 3 % sucrose. 0.78 % Bacto agar (SGM).      16-h PP. CWFT ? purple photosynthetic   96 % SG in vitro. 1 % infection. 2 %                   Crovadore et al. (2012)
                      MS ? 0.5 lM 2,4-D ? 10 lM Kin (CIM).            lamps. 6000 lux. 27 °C                  polyembryony (discarded). No in vitro rooting
                      B5 ? 0.5 lM 2,4-D ? 10 lM Kin (CMM).                                                    possible from callus-derived shoots. Seedlings
                      MS ? 2.5 lM Kin (SIM from green callus). pH                                             planted with grafted 2-year-old Citrus as pot
                      5.7. 3 % sucrose. 0.78 % Bacto agar                                                     host. GC–MS used to analyze the composition
                                                                                                              of callus following extraction with pentane
      S. album       WPM ? 990 mg/l K2SO4 ? 100 mg/l myo-            16-h PP. CWFT. 36 lmol m-2 s-1.         2013: 100 % of explants formed callus; 24.6 shoot      Singh et al. (2013, 2015)
                      inositol ? 0.4 mg/l TDZ (CIM).                  25 ± 2 °C. 40–60 % RH                   buds/callus; 20.7 shoots/explant; 91.7 % of
                      WPM ? 2.5 mg/l BA ? 0.4 mg/l NAA (SIM).                                                 shoots rooted. 2015: 100 % of explants formed
                      WPM ? 1.5 mg/l IBA (RIM). pH 5.8. 3 %                                                   callus; 16 shoot buds/callus; 82.37 % of shoots
                      sucrose. 0.8 % agar                                                                     rooted. [90 % of plantlets acclimatized in
                                                                                                              sterile soil and coco-peat (1:1) (2013) or 85 %
                                                                                                              of plantlets acclimatized in sterile soil, sand and
                                                                                                              coco-peat (1:1:1) (2015) survived after 4–5
                                                                                                              weeks
                                                                                                                                                                                                Planta (2016) 243:847–887
      Table 4 continued
      Studied         Culture medium, PGRs, additives, subculturesb       Culture conditionsc                          Experimental outcome, maximum productivity,           References
      sandalwooda                                                                                                      acclimatization and variation
      S. album        MS ? 2.5 mg/l 2,4-D ? 3 mg/l Kn (CIM).              25 ± 1 °C, LI ? source NR Dark for           Callus induction observed with 8 weeks and SEs        Peeris and Senarath
                       MS ? 0.5 mg/l BA ? 1 mg/l IAA ? 0.5 mg/l            callus and SE induction. PP = 16 h for       within 2 weeks. About 58 % of SEs germinated          (2015)
                       Kn (SEIM). MS ? 2 mg/l GA3 (SGM).                   SE germination and plant development         within 2 weeks. About 76 % of plantlets
                       MS ? 0.4 mg/l BA ? 0.2 mg/l IAA (plantlet                                                        produced with healthy shoots and roots.
                                                                                                                                                                                                           Planta (2016) 243:847–887
123
876                                                                                                   Planta (2016) 243:847–887
greater detail in Tables 3 and 4. The most recent reviews       the source of disinfected floral tissues for either in vitro
on sandalwood tissue culture and related biotechnologies        breeding experiments or more specialized in vitro tech-
were published by Rao and Bapat (1992), (1993), (1995),         niques such as anther or ovary culture. The latter two
Bapat and Rao (1992a), and Bapat (1993)                         techniques have not yet been applied to any Santalum
                                                                species. The establishment of an in vitro propagation pro-
Perspectives and culture establishment                          tocol traditionally requires several stages: culture initiation
                                                                (including the appropriate choice of explant, surface ster-
Most in vitro studies have been conducted on S. album with      ilization, culture conditions and medium composition),
only one report on S. spicatum (Tables 3, 4). In vitro tissue   multiplication, rooting (in vitro and ex vitro), acclimati-
culture and micropropagation are popular methods for the        zation, and field establishment. These are outlined next for
large-scale propagation and improvement of existing plant       Santalum spp.
genotypes, serving as the basal method for genetic trans-
formation experiments, often cutting the time to obtain         Choice of explant and surface sterilization
novel germplasm through conventional breeding. By pro-
viding a sterile culture environment, in vitro tissue culture   The choice of an explant depends primarily on the desired
also allows for developmental events to be studied, more so     objective (e.g., shoot tips or nodal explants for the pro-
when thin cell layers are used (Teixeira da Silva and           duction of true-to-type clonal plants) or on the availability
Dobránszki 2013), and for the production of in vitro           of healthy (disease-free) material. The age and physiolog-
flowers (Teixeira da Silva et al. 2014), which can serve as     ical status of the mother plant need to be considered, such
123
Planta (2016) 243:847–887                                                                                                   877
as actively growing vs dormant shoots, which often               (Table 3). Even though the choice of sterilant, its concen-
depends on seasonal availability. For the micropropagation       tration, treatment time and rinses are all essential aspects of
of sandalwood, various explants have been used. Details          a surface sterilization protocol (Teixeira da Silva et al.
about explant source, the type of explant used, and their        2015), such basic information is frequently missing from
size are described in Table 3. In general, the micropropa-       many protocols, as is a description of the efficiency of the
gation of any plant species employs explants with a pre-         sterilization protocol and the quantification of infection
determined meristem such as a node or a shoot tip, either        (Table 3).
from mature trees or from in vitro or ex vitro germinated
seedlings; other explants such as internodes, stem seg-          Culture conditions
ments, or leaves of leaf disks are generally utilized to
induce adventitious shoots or somatic embryos. In sandal-        Specific and tested culture conditions are required to ini-
wood, the explants used encompassed nodes and shoot tips         tiate a plant tissue culture because photoperiod, light
from mature trees or seedlings (Rao et al. 1984; Muralid-        intensity, light source, and temperature play important
haran 1997; Das et al. 1998; Rugkhla and Jones 1998;             roles in the successful establishment of an in vitro culture.
Radhakrishnan et al. 2001; Ilah et al. 2002; Primawati           The most commonly used conditions in the tissue culture of
2006; Sanjaya et al. 2006a, b; Revathy and Arumugam              S. album were 16-h photoperiod and temperatures between
2011; Peeris and Senarath 2015; Singh et al. 2015), zygotic      24 and 28 °C (Table 4), although some protocols used a
embryos and seed endosperm (Rangaswamy and Rao 1963;             12-h photoperiod (Lakshmi Sita et al. 1979, 1980a, b;
Rao 1965; Rao and Rangaswamy 1971; Rao and Raghava               Sanjaya et al. 2006a, b) or very rarely a 14-h photoperiod
Ram 1983; Sankara Rao et al. 1996; Rai and McComb                (Shiri and Rao 1998). Rao et al. (1984) used a 72-h dark
1997; Shiri and Rao 1998; Anil et al. 2000; Anil and Rao         treatment for root induction. Optimal (recommended)
2000; Rai and McComb 2002; Mo et al. 2008), mature and           in vitro regeneration protocols for S. album would be Singh
immature seeds as well as seedling-derived explants such         et al. (2013, 2015) for callus induction, Rugkhla and Jones
as internodes, hypocotyls, leaves, and stem segments (Rao        (1998) for somatic embryogenesis, and Sanjaya et al.
and Bapat 1978; Bapat and Rao 1979, 1984; Lakshmi Sita           (2006a, b) for direct shoot induction from leaf explants.
et al. 1980a; Bapat et al. 1985; Das et al. 1999, 2001;
Sanjaya and Rai 2003; Mujib 2005; Mo et al. 2008, 2010;          Medium composition
Shekhawat et al. 2008; Nikam and Barmukh 2009; She-
khawat et al. 2010; Revathy and Arumugam 2011; Janar-            Medium composition includes the type of basal medium
thanam and Sumathi 2011; Bele et al. 2012; Crovadore             used or the composition and concentration of macro- and
et al. 2012; Janarthanam et al. 2012), and explants such as      micronutrients, carbon source, gelling agent (type and
leaves, stem segments, and internodes from mature trees          concentration) or liquid culture, plant growth regulators
(Lakshmi Sita et al. 1979; 1980b; Lakshmi Sita and Shobha        (PGRs), and additives. Mostly Murashige and Skoog
Rani 1983; Rao and Raghava Ram 1983; Ozias-Akins et al.          (1962) (MS) basal medium was used for S. album culture
1985; Rao and Ozias-Akins 1985; Lakshmi Sita 1986;               initiation, multiplication and rooting (Table 4). Only one
Bapat and Rao 1988, 1992b, 1999; Bapat et al. 1996; Ma           study (Singh et al. 2013) used woody plant medium
et al. 2008; Shekhawat et al. 2008; Singh et al. 2013). In       (WPM) (Lloyd and McCown 1980). Singh et al. (2013)
rare cases (Bhaskar and Rao 1983), in vitro-raised shoots        used WPM with 990 mg/L K2SO4 to induce callus from
derived from callus were used explants although details          leaves of S. album while WPM with PGRs was used to
about callus induction were not reported.                        induce shoots and roots (Table 4). Crovadore et al. (2012)
   Surface sterilization, an essential step for the initiation   used B5 medium (Gamborg et al. 1968) for in vitro seed
of an aseptic culture, varies depending on the explant type      germination, while MS medium was used for callus cul-
and source (Table 3). In sandalwood, surface-sterilized          ture, shoot induction, and rooting. In general, 3 % sucrose
fruits can be used for aseptic seed germination and to           was used as the preferred carbon source, but 4–5 % sucrose
isolate endosperm (Rao and Bapat 1978, 1979; Bapat et al.        was also reported in a few cases (Table 4). In most studies,
1985; Das et al. 1999; Ilah et al. 2002; Mujib 2005; Cro-        semisolid medium was used and gelled with agar (Table 4),
vadore et al. 2012). Once an aseptic seedling has germi-         although Laxmi Sita et al. (1980a, b) used liquid culture
nated, it can be used as a source of explants that does not      medium for S. album somatic embryogenesis. Adventitious
require further surface sterilization (Rangaswamy and Rao        S. album shoots can be induced on MS medium supple-
1963; Rao 1965; Rao and Rangaswamy 1971, 1999; Anil              mented with 5.0 lM BA and 0.5 lM NAA, subcultured on
et al. 2000; Anil and Rao 2000). For surface sterilization,      MS medium supplemented with 5.0 lM BA and 5.0 lM
HgCl2 in concentrations ranging from 0.05 to 0.5 % (w/v)         IBA, and rooted in the presence of 250 lM IBA (Fig. 2).
are most frequently used, irrespective of the explant            Optimal basal medium for S. album would be WPM
                                                                                                                     123
878                                                                                            Planta (2016) 243:847–887
supplemented with 0.4 mg/l TDZ for callus induction          1980a, b; Rao and Raghava Ram 1983; Rao et al. 1984;
(Singh et al. 2013, 2015), or MS supplemented with 5 lM      Bapat et al. 1985; Ozias-Akins et al. 1985; Rao and
BA for the induction of somatic embryos (Rugkhla and         Ozias-Akins 1985; Lakshmi Sita 1986; Bapat and Rao
Jones 1998) or 0.53 lM NAA and 11.09 lM BA for direct        1988, 1992; Bapat et al. 1990, 1996; Sankara Rao et al.
shoot induction from leaf-derived explants (Sanjaya et al.   1996; Rai and McComb 1997; Das et al. 1998, 1999;
2006a, b).                                                   Shiri and Rao 1998; Rugkhla and Jones 1998; Anil and
                                                             Rao 2000; Das et al. 2001; Ilah et al. 2002; Rai and
Somatic embryogenesis                                        McComb 2002; Mo et al. 2008; Shekhawat et al. 2008,
                                                             2010; Revathy and Arumugam 2011; Bele et al. 2012;
Somatic embryogenesis, an important in vitro plant           Singh et al. 2013, 2015; Peeris and Senarath 2015).
regeneration pathway, is utilized for large-scale propaga-   Details about culture conditions and media composition to
tion and has various applications in cryoconservation,       induce somatic embryogenesis are provided in Table 4.
synthetic seed production, and as a source of protoplasts.   Despite these prolific reports, mainly for S. album, many
A total of 33 in vitro Santalum propagation studies have     have not been supported by very strong, or convincing,
claimed somatic embryogenesis (Rao and Rangaswamy            proof, such as histology, cytology, flow cytometry, or
1971; Bapat and Rao 1979; Lakshmi Sita et al. 1979,          molecular markers.
123
Planta (2016) 243:847–887                                                                                               879
   Anil and Rao (2000) claimed that a Ca2?-mediated              and 0.55 M sorbitol. That study appears to have been a pre-
signaling pathway may be involved in somatic embryoge-           amble for the more comprehensively reported study by Rao
nesis after callus induced in the presence of 2,4-D took up      and Ozias-Akins (1985) in which the authors reported the
four-fold levels of labeled Ca2? resulting in the formation      same ideal enzyme cocktail for protoplast isolation from
of pro-embryogenic cell masses. Spherical organelles in the      embryogenic cell suspension cultures derived from shoot
endosperm are oil bodies in which calcium-dependent              segments of a 20-year-old S.album tree.
protein kinase (CDPK) (first purified in somatic embryos
by Anil and Rao (2001), and termed swCDPKs) is                   Genetic transformation
expressed during seed development (Anil et al. 2003). As a
result of the action of CDPK, the existence of these oil         There are only three reports on the genetic transformation
bodies and the Ca2?-mediated signaling pathway, as much          of sandalwood, all three targeting S. album and using
as 30 % of the dry weight of the endosperm was made up           Agrobacterium tumefaciens-mediated gene transfer. Shiri
of oil (Anil et al. 2003). Earlier studies by this group (Anil   and Rao (1998) used LBA4404/pKIWI105 to introduce
et al. 2000) indicated that CDPK could not be detected in        gusA and nptII genes into somatic embryos, confirming
somatic embryos, or in the soluble proteins of shoots and        integration using a range of biochemical assays and
flowers, but only in zygotic embryos, seedlings, and             molecular tools [GUS histochemical staining, NPTII
endosperm. S. album callus suspension that develops in MS        expression assay, PCR, Southern blot, dot blot (equivalent
liquid medium supplemented with 4.5 lM 2,4-D can be              to Northern blot)]. Disarmed A. tumefaciens strain EHA105
induced to form embryogenic callus on solid MS medium            (Hood et al. 1993) harboring the pCAMBIA 1301 binary
supplemented with 5.0 lM TDZ and 0.5 lM IBA, while               vector carrying the gusA gene driven by single CaMV 35S
somatic embryos form on MS medium supplemented with              promoter and an hptII gene driven by a double-enhanced
5.0 lM TDZ and 0.5 lM IBA (Fig. 3).                              35S promoter was used to transform embryogenic S. album
                                                                 callus (Shekhawat et al. 2008). Gene integration was con-
Protoplasts                                                      firmed by PCR, RT-PCR and Southern blot analysis, and
                                                                 GUS activity was shown to be stable over 7 months of
There are only four studies available in which protoplast        culture. In an ensuing study, Shekhawat et al. (2010)
culture was used for the regeneration of plants. Laxmi Sita      transformed embryogenic cell suspension cultures—also
and Sobha Rani (1983) isolated protoplasts from young            with EHA105—with a hepatitis B small surface antigen
leaves of mature S. album trees. In their protocol, leaves       (HBsAg) gene, encoding for a pharmaceutically important
were incubated in 2 % cellulase R10, 0.5 % macerozyme,           recombinant protein. Using electroporation and selection
0.5 % pectinase, and 1 % hemicellulase in cell protoplast        on kanamycin-supplemented medium, the authors con-
washing (CPW) salts with 10 % mannitol at pH 5.6,                firmed transgene expression using RT-PCR, Western blot
incubated for 16 h at 25 °C with shaking. Protoplasts could      analysis, and ELISA. Supplementing medium with 30 mM
be isolated by using only 1 % cellulase R10 and 0.5 %            trehalose almost doubled the level of HBsAg expressed.
pectinase in V47 medium (Binding 1974). Leaves and               Genetic transformation is thus weakly explored in sandal-
callus yielded 2 9 105 and 3 9 106 protoplasts/ml,               wood species. However, the introduction of biotic (dis-
respectively. Protoplasts formed cellular colonies in            eases, pests, viruses) and abiotic (drought, cold, frost,
6 weeks after culture in liquid MS medium containing             salinity) resistance through transgenic means would widen
2 mg/l 2,4-D, 0.2 mg/L BA and 10 % mannitol. The                 the possible niches where sandalwood could be cultivated,
regeneration of organs or plantlets was not reported. Also       taking advantage of usually hostile conditions to harvest
in S. album, Bapat et al. (1985) used 1 % cellulase R10,         sandalwood products.
0.5 % macerozyme, and 0.5 M sorbitol or mannitol to
isolate protoplasts from stem callus, 2 % cellulase R10,
1 % pectinase, 1 % hemicellulase, 0.9 % CaCl22H2O, and          Conclusions and future perspectives
0.55 M sorbitol for hypocotyl callus and 2 % cellulase
R10, 1 % macerozyme, 1 % hemicellulase and 0.8 M                 Sandalwood from several Santalum species is a commer-
sorbitol for leaf mesophyll, all in V47 medium. The highest      cially important forest product that has been traded for
yield was from stem callus (8.73 9 106), and the authors         many centuries. International trade has been based on the
claimed the production of somatic embryos and the sub-           harvest of wild stands, resulting in excessive exploitation
sequent development into plantlets. Ozias-Akins et al.           and severe reductions in abundance and biodiversity across
(1985) also claimed to derive somatic embryos from callus        most species. This has led to sustained price rises for
induced from protoplasts derived from shoot segments             sandalwood products and increasing interest in sandalwood
using 1 % cellulase, 1 % macerozyme, 0.5 % driselase,            cultivation, both as an industrial crop and on a smaller
                                                                                                                  123
880                                                                                                               Planta (2016) 243:847–887
scale within agroforestry systems. Successful cultivation of           Guangdong Province Science and Technology Program (number:
sandalwood will depend on a clear understanding of its                 2015B020231008). The authors thank the assistance of Dr. Budi
                                                                       Winarto (IOCRI, Indonesia) with assistance in the interpretation of
basic biology and propagation, details of which have been              Indonesian literature and Dr. Robert Nasi (Director, Center for
examined in depth in this review. The hemi-parasitic nature            International Forestry Research (CIFOR), Indonesia) for providing
of sandalwood necessitates the planting of host plants to              difficult-to-access literature. TP recognizes the generous contributions
support its growth. While this makes cultivation of san-               of the Australian Center for International Agricultural Research
                                                                       (ACIAR). The authors are thankful to the anonymous reviewers for
dalwood more complex relative to other forestry species,               constructive comments and suggestions.
many suitable species have been recorded in the literature
to support sandalwood growth during the three main stages              Compliance with ethical standards
of its rotation (pot, intermediate, and final hosts). Sandal-
                                                                       Conflict of interest   The authors declare no conflicts of interest.
wood can potentially be grown across a range of environ-
ments provided locally adapted suitable host species are
used from the nursery phase until harvest. It is evident that
Santalum spp. preferentially form haustorial connections               References
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