TECHNICAL BULLETIN
CellTiter-Glo Luminescent
Cell Viability Assay
Instructions for Use of Products
G7570, G7571, G7572 and G7573
Revised 3/15
TB288
�CellTiter-Glo Luminescent
Cell Viability Assay
All technical literature is available at: www.promega.com/protocols/
Visit the web site to verify that you are using the most current version of this Technical Bulletin.
E-mail Promega Technical Services if you have questions on use of this system: [email protected]
1. Description.......................................................................................................................................... 1
2. Product Components and Storage Conditions......................................................................................... 5
3. Performing the CellTiter-Glo Assay...................................................................................................... 6
3.A. Reagent Preparation.................................................................................................................... 6
3.B. Protocol for the Cell Viability Assay............................................................................................... 6
3.C. Protocol for Generating an ATP Standard Curve (optional)............................................................. 7
4. Appendix............................................................................................................................................. 8
4.A. Overview of the CellTiter-Glo Assay............................................................................................ 8
4.B. Additional Considerations............................................................................................................ 9
4.C. References................................................................................................................................ 11
4.D. Related Products....................................................................................................................... 12
5. Summary of Change........................................................................................................................... 14
1. Description
The CellTiter-Glo Luminescent Cell Viability Assay(ad) is a homogeneous method to determine the number of viable
cells in culture based on quantitation of the ATP present, which signals the presence of metabolically active cells. The
CellTiter-Glo Assay is designed for use with multiwell-plate formats, making it ideal for automated high-throughput
screening (HTS) and cell proliferation and cytotoxicity assays. The homogeneous assay procedure (Figure 1) involves
adding a single reagent (CellTiter-Glo Reagent) directly to cells cultured in serum-supplemented medium. Cell
washing, removal of medium or multiple pipetting steps are not required.
The homogeneous add-mix-measure format results in cell lysis and generation of a luminescent signal proportional
to the amount of ATP present (Figure 2). The amount of ATP is directly proportional to the number of cells present in
culture in agreement with previous reports (1). The CellTiter-Glo Assay relies on the properties of a proprietary
thermostable luciferase (Ultra-Glo Recombinant Luciferase), which generates a stable glow-type luminescent
signal and improves performance across a wide range of assay conditions. The luciferase reaction for this assay is
shown in Figure 3. The half-life of the luminescent signal resulting from this reaction is greater than five hours
(Figure 4). This extended half-life eliminates the need for reagent injectors and provides flexibility for continuous or
batch-mode processing of multiple plates. The unique homogeneous format reduces pipetting errors that may be
introduced during the multiple steps required by other ATP-measurement methods.
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TB288 Revised 3/15
�1.
Description (continued)
CellTiter-Glo
Substrate
CellTiter-Glo
Buffer
CellTiter-Glo
Reagent
Luminometer
3170MA12_0A
Mix
Figure 1. Flow diagram showing preparation and use of CellTiter-Glo Reagent.
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�System Advantages
Homogeneous: Add-mix-measure format reduces the number of plate-handling steps to fewer than that
required for similar ATP assays.
Fast: Data can be recorded 10 minutes after adding reagent.
Sensitive: Measures cells at numbers below the detection limits of standard colorimetric and fluorometric assays.
Flexible: Can be used with various multiwell formats. Data can be recorded by luminometer or CCD camera or
imaging device.
Robust: Luminescent signal is very stable, with a half-life >5 hours, depending on cell type and culture medium
used.
Able to Multiplex: Can be used with reporter gene assays or other cell-based assays from Promega (2,3).
3.5 106
r = 0.99
R = 0.999
3.0 106
2.5 106
2.0 106
50,000
1.5 106
30,000
40,000
1.0 106
20,000
0.5 106
r = 0.99
10,000
10,000
20,000
30,000
Cells per Well
100
40,000
200
300
50,000
400
60,000
3171MA12_0A
Luminescence (RLU)
4.0 106
Figure 2. Cell number correlates with luminescent output. A direct relationship exists between luminescence
measured with the CellTiter-Glo Assay and the number of cells in culture over three orders of magnitude. Serial
twofold dilutions of HEK293 cells were made in a 96-well plate in DMEM with 10% FBS, and assays were performed
as described in Section3.B. Luminescence was recorded 10minutes after reagent addition using a GloMax-Multi+
Detection System. Values represent the mean S.D. of four replicates for each cell number. The luminescent signal
from 50HEK293 cells is greater than three times the background signal from serum-supplemented medium without
cells. There is a linear relationship (r2 = 0.99) between the luminescent signal and the number of cells from 0to 50,000
cells per well.
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TB288 Revised 3/15
�Description (continued)
HO
COOH
Ultra-Glo Recombinant
Luciferase
+ATP+O2
Mg2+
Beetle Luciferin
O
+AMP+PPi+CO2+Light
Oxyluciferin
1399MD03_6A
1.
100
90
80
70
60
50
40
30
20
10
0
CHO-K1
BHK-21
HepG2
50
100 150 200 250 300
Time (minutes)
3173MA12_0A
Relative Luminescence (%)
Figure 3. The luciferase reaction. Mono-oxygenation of luciferin is catalyzed by luciferase in the presence of Mg2+,
ATP and molecular oxygen.
Figure 4. Extended luminescent half-life allows high-throughput batch processing. Signal stability is shown
for three common cell lines. HepG2 and BHK-21 cells were grown and assayed in MEM containing 10% FBS, while
CHO-K1 cells were grown and assayed in DME/F-12 containing 10% FBS. CHO-K1, BHK-21 and HepG2 cells, at
25,000 cells per well, were added to a 96-well plate. After an equal volume of CellTiter-Glo Reagent was added, plates
were shaken and luminescence monitored over time with the plates held at 22C. The half-lives of the luminescent
signals for the CHO-K1, BHK-21 and HepG2 cells were approximately 5.4, 5.2 and 5.8 hours, respectively.
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�2.
Product Components and Storage Conditions
PRODUCT
S I Z E C A T. #
CellTiter-Glo Luminescent Cell Viability Assay
10ml
G7570
Substrate is sufficient for 100 assays at 100l/assay in 96-well plates or 400 assays at 25l/assay in 384-well
plates. Includes:
1 10ml CellTiter-Glo Buffer
1 vial CellTiter-Glo Substrate (lyophilized)
PRODUCT
CellTiter-Glo Luminescent Cell Viability Assay
S I Z E C A T. #
10 10ml
G7571
Each vial of substrate is sufficient for 100 assays at 100l/assay in 96-well plates or 400 assays at 25l/assay
in 384-well plates (1,000 to 4,000 total assays). Includes:
10 10ml CellTiter-Glo Buffer
10 vials CellTiter-Glo Substrate (lyophilized)
PRODUCT
CellTiter-Glo Luminescent Cell Viability Assay
S I Z E C A T. #
100ml
G7572
Substrate is sufficient for 1,000 assays at 100l/assay in 96-well plates or 4,000 assays at 25l/assay in
384-well plates. Includes:
1 100ml CellTiter-Glo Buffer
1 vial CellTiter-Glo Substrate (lyophilized)
PRODUCT
CellTiter-Glo Luminescent Cell Viability Assay
S I Z E C A T. #
10 100ml
G7573
Each vial of substrate is sufficient for 1,000 assays at 100l/assay in 96-well plates or 4,000 assays at
25l/assay in 384-well plates (10,000to 40,000 total assays). Includes:
10 100ml CellTiter-Glo Buffer
10 vials CellTiter-Glo Substrate (lyophilized)
Storage Conditions: For long-term storage, store the lyophilized CellTiter-Glo Substrate and CellTiter-Glo Buffer
at 20C. For frequent use, the CellTiter-Glo Buffer can be stored at 4C or room temperature for 48hours without
loss of activity. See product label for expiration date information. Reconstituted CellTiter-Glo Reagent (Buffer plus
Substrate) can be stored at room temperature for up to 8hours with <10% loss of activity, at 4C for 48hours with
~5% loss of activity, at 4C for 4days with ~20% loss of activity or at 20C for 21weeks with ~3% loss of activity.
The reagent is stable for up to ten freeze-thaw cycles, with less than 10% loss of activity.
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TB288 Revised 3/15
�3.
Performing the CellTiter-Glo Assay
Materials to Be Supplied by the User
opaque-walled multiwell plates adequate for cell culture
multichannel pipette or automated pipetting station for reagent delivery
device (plate shaker) for mixing multiwell plates
luminometer, CCD camera or imaging device capable of reading multiwell plates
optional: ATP for use in generating a standard curve (Section 3.C)
3.A. Reagent Preparation
1.
Thaw the CellTiter-Glo Buffer, and equilibrate to room temperature prior to use. For convenience the
CellTiter-Glo Buffer may be thawed and stored at room temperature for up to 48hours prior to use.
2.
Equilibrate the lyophilized CellTiter-Glo Substrate to room temperature prior to use.
3.
Transfer the appropriate volume (10ml for Cat.# G7570 and G7571, or 100ml for Cat.# G7572 and G7573) of
CellTiter-Glo Buffer into the amber bottle containing CellTiter-Glo Substrate to reconstitute the lyophilized
enzyme/substrate mixture. This forms the CellTiter-Glo Reagent.
4.
Mix by gently vortexing, swirling or inverting the contents to obtain a homogeneous solution. The CellTiter-Glo
Substrate should go into solution easily in less than 1minute.
3.B. Protocol for the Cell Viability Assay
We recommend that you perform a titration of your particular cells to determine the optimal number and ensure that
you are working within the linear range of the CellTiter-Glo Assay. Figure2 provides an example of such a titration of
HEK293 cells using 0 to 50,000 cells per well in a 96-well format.
1.
Prepare opaque-walled multiwell plates with mammalian cells in culture medium, 100l per well for 96-well
plates or 25l per well for 384-well plates.
Multiwell plates must be compatible with the luminometer used.
2.
Prepare control wells containing medium without cells to obtain a value for background luminescence.
3.
Add the test compound to experimental wells, and incubate according to culture protocol.
4.
Equilibrate the plate and its contents at room temperature for approximately 30 minutes.
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�5.
Add a volume of CellTiter-Glo Reagent equal to the volume of cell culture medium present in each well (e.g.,
add 100l of reagent to 100l of medium containing cells for a 96-well plate, or add 25l of reagent to 25l of
medium containing cells for a 384-well plate).
6.
Mix contents for 2 minutes on an orbital shaker to induce cell lysis.
7.
Allow the plate to incubate at room temperature for 10 minutes to stabilize luminescent signal.
Note: Uneven luminescent signal within standard plates can be caused by temperature gradients, uneven
seeding of cells or edge effects in multiwell plates.
8.
Record luminescence.
Note: Instrument settings depend on the manufacturer. An integration time of 0.251 second per well should
serve as a guideline.
3.C. Protocol for Generating an ATP Standard Curve (optional)
It is a good practice to generate a standard curve using the same plate on which samples are assayed. We recommend
ATP disodium salt (Cat.# P1132, Sigma Cat.# A7699 or GE Healthcare Cat.# 27-1006). The ATP standard curve
should be generated immediately prior to adding the CellTiter-Glo Reagent because endogenous ATPase enzymes
found in sera may reduce ATP levels.
1.
Prepare 1M ATP in culture medium (100l of 1M ATP solution contains 1010 moles ATP).
2.
Prepare serial tenfold dilutions of ATP in culture medium (1M to 10nM; 100l contains 1010 to 1012 moles
of ATP).
3.
Prepare a multiwell plate with varying concentrations of ATP standard in 100l medium
(25l for a 384-well plate).
4.
Add a volume of CellTiter-Glo Reagent equal to the volume of ATP standard present in each well.
5.
Mix contents for 2 minutes on an orbital shaker.
6.
Allow the plate to incubate at room temperature for 10 minutes to stabilize the luminescent signal.
7.
Record luminescence.
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�4. Appendix
4.A. Overview of the CellTiter-Glo Assay
The assay system uses the properties of a proprietary thermostable luciferase to enable reaction conditions that
generate a stable glow-type luminescent signal while simultaneously inhibiting endogenous enzymes released during
cell lysis (e.g., ATPases). Release of ATPases will interfere with accurate ATP measurement. Historically, firefly
luciferase purified from Photinus pyralis (LucPpy) has been used in reagents for ATP assays (1,47). However, it
has only moderate stability in vitro and is sensitive to its chemical environment, including factors such as pH and
detergents, limiting its usefulness for developing a robust homogeneous ATP assay. Promega has successfully
developed a stable form of luciferase based on the gene from another firefly, Photuris pennsylvanica (LucPpe2), using
an approach to select characteristics that improve performance in ATP assays. The unique characteristics of this mutant
(LucPpe2m) enabled design of a homogeneous single-reagent-addition approach to perform ATP assays with cultured
cells. Properties of the CellTiter-Glo Reagent overcome the problems caused by factors, such as ATPases, that
interfere with ATP measurement in cell extracts. The reagent is physically robust and provides a sensitive and stable
luminescent output.
Sensitivity and Linearity: The ATP-based detection of cells is more sensitive than other methods (810). In
experiments performed by Promega scientists, the luminescent signal from 50HEK293 cells is greater than three
standard deviations above the background signal from serum-supplemented medium without cells. There is a linear
relationship (r2 = 0.99) between the luminescent signal and the number of cells from 0 to 50,000 cells per well in the
96-well format. The luminescence values in Figure 2 were recorded after 10 minutes of incubation at room temperature
to stabilize the luminescent signal as described in Section3.B. Incubation of the same 96-well plate used in the
experiment shown in Figure 2 for 360minutes at room temperature had little effect on the relationship between
luminescent signal and number of cells (r2 = 0.99).
Speed: The homogeneous procedure to measure ATP using the CellTiter-Glo Assay is quicker than other ATP assay
methods that require multiple steps to extract ATP and measure luminescence. The CellTiter-Glo Assay also is faster
than other commonly used methods to measure the number of viable cells (such as MTT, alamarBlue or Calcein-AM)
that require prolonged incubation steps to enable the cells metabolic machinery to convert indicator molecules into a
detectable signal.
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�4.B. Additional Considerations
Temperature: The intensity and decay rate of the luminescent signal from the CellTiter-Glo Assay depends on the
luciferase reaction rate. Environmental factors that affect the luciferase reaction rate will change the intensity and
stability of the luminescent signal. Temperature is one factor that affects the rate of this enzymatic assay and thus the
light output. For consistent results, equilibrate assay plates to a constant temperature before performing the assay.
Transferring eukaryotic cells from 37C to room temperature has little effect on ATP content (5). We have demonstrated that removing cultured cells from a 37C incubator and allowing them to equilibrate to 22C for 12 hours had
little effect on ATP content. For batch-mode processing of multiple assay plates, take precautions to ensure complete
temperature equilibration. Plates removed from a 37C incubator and placed in tall stacks at room temperature will
require longer equilibration than plates arranged in a single layer. Insufficient equilibration may result in a temperature
gradient effect between wells in the center and at the edge of the plates. The temperature gradient pattern also may
depend on the position of the plate in the stack.
Chemicals: The chemical environment of the luciferase reaction affects the enzymatic rate and thus luminescence
intensity. Differences in luminescence intensity have been observed using different types of culture media and sera. The
presence of phenol red in culture medium should have little impact on luminescence output. Assaying 0.1M ATP in
RPMI medium without phenol red resulted in ~5% increase in luminescence output (in relative light units [RLU])
compared to assays in RPMI containing the standard concentration of phenol red, whereas assays in RPMI medium
containing twice the normal concentration of phenol red showed a ~2% decrease in luminescence.
Solvents for the various test compounds may interfere with the luciferase reaction and thus the light output from the
assay. Interference with the luciferase reaction can be detected by assaying a parallel set of control wells containing
medium without cells. Dimethylsulfoxide (DMSO), commonly used as a vehicle to solubilize organic chemicals, has
been tested at final concentrations of up to 2% in the assay and only minimally affects light output.
Plate Recommendations: We recommend using standard opaque-walled multiwell plates suitable for luminescence
measurements. Opaque-walled plates with clear bottoms to allow microscopic visualization of cells also may be used;
however, these plates will have diminished signal intensity and greater cross talk between wells. Opaque white tape
may be used to decrease luminescence loss and cross talk.
Cellular ATP Content: Different cell types have different amounts of ATP, and values reported for the ATP level in
cells vary considerably (1,4,1113). Factors that affect the ATP content of cells may affect the relationship between cell
number and luminescence. Anchorage-dependent cells that undergo contact inhibition at high densities may show a
change in ATP content per cell at high densities, resulting in a nonlinear relationship between cell number and
luminescence. Factors that affect the cytoplasmic volume or physiology of cells also will affect ATP content. For
example, oxygen depletion is one factor known to cause a rapid decrease in ATP (1).
Mixing: Optimal assay performance is achieved when the CellTiter-Glo Reagent is mixed completely with the
cultured cells. Suspension cell lines (e.g., Jurkat cells) generally require less mixing to achieve lysis and extract ATP
than adherent cells (e.g., L929 cells). Tests were done to evaluate the effect of shaking the plate after adding the
CellTiter-Glo Reagent. Suspension cells cultured in multiwell plates showed only minor differences in light output
whether or not the plates were shaken after adding the CellTiter-Glo Reagent. Adherent cells are more difficult to lyse
and show a substantial difference between shaken and nonshaken plates.
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TB288 Revised 3/15
�4.B. Additional Considerations (continued)
Several additional parameters related to reagent mixing include the force of delivery of CellTiter-Glo Reagent, sample
volume and dimensions of the well. All of these factors may affect assay performance. The degree of reagent mixing
required may be affected by the method used to add the CellTiter-Glo Reagent to the assay plates. Automated
pipetting devices using a greater or lesser force of fluid delivery may affect the degree of subsequent mixing required.
Complete reagent mixing in 96-well plates should be achieved using orbital plate shaking devices built into many
luminometers and the recommended 2-minute shaking time. Special electromagnetic shaking devices that use a radius
smaller than the well diameter may be required to efficiently mix contents of 384-well plates. The depth of medium and
geometry of the multiwell plates may have an effect on mixing efficiency. We recommend that you take these factors
into consideration when performing the assay and empirically determine whether a mixing step is necessary for the
individual application.
Luminometers
For highly sensitive luminometric assays, the luminometer model and settings greatly affect the quality of data
obtained. Luminometers from different manufacturers will vary in sensitivities and dynamic ranges. We recommend
the GloMax products because these instruments do not require gain adjustments to achieve optimal sensitivity and
dynamic range. Additionally, GloMax instruments are preloaded with Promega protocols for ease of use.
If you are not using a GloMax luminometer, consult the operating manual for your luminometer to determine the
optimal settings. The limits should be verified on each instrument before analysis of experimental samples. The assay
should be linear in some portion of the detection range of the instrument used. For an individual luminometer there
may be different gain settings. We recommend that you optimize the gain settings.
10
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�4.C. References
1.
Crouch, S.P. et al. (1993) The use of ATP bioluminescence as a measure of cell proliferation and cytotoxicity.
J. Immunol. Methods 160, 818.
2.
Farfan, A. et al. (2004) Multiplexing homogeneous cell-based assays. Cell Notes 10, 25.
3.
Riss, T., Moravec, R. and Niles, A. (2005) Selecting cell-based assays for drug discovery screening. Cell Notes
13, 1621.
4.
Kangas, L., Grnroos, M. and Nieminen, A.L. (1984) Bioluminescence of cellular ATP: A new method for
evaluating cytotoxic agents in vitro. Med. Biol. 62, 33843.
5.
Lundin, A. et al. (1986) Estimation of biomass in growing cell lines by adenosine triphosphate assay. Methods
Enzymol. 133, 2742.
6.
Sevin, B.U. et al. (1988) Application of an ATP-bioluminescence assay in human tumor chemosensitivity testing.
Gynecol. Oncol. 31, 191204.
7.
Gerhardt, R.T. et al. (1991) Characterization of in vitro chemosensitivity of perioperative human ovarian
malignancies by adenosine triphosphate chemosensitivity assay. Am. J. Obstet. Gynecol. 165, 24555.
8.
Petty, R.D. et al. (1995) Comparison of MTT and ATP-based assays for the measurement of viable cell number.
J. Biolumin. Chemilumin. 10, 2934.
9.
Cree, I.A. et al. (1995) Methotrexate chemosensitivity by ATP luminescence in human leukemia cell lines and in
breast cancer primary cultures: Comparison of the TCA-100 assay with a clonogenic assay. AntiCancer Drugs 6,
398404.
10. Maehara, Y. et al. (1987) The ATP assay is more sensitive than the succinate dehydrogenase inhibition test for
predicting cell viability. Eur. J. Cancer Clin. Oncol. 23, 2736.
11. Stanley, P.E. (1986) Extraction of adenosine triphosphate from microbial and somatic cells. Methods Enzymol.
133, 1422.
12. Beckers, B. et al. (1986) Application of intracellular ATP determination in lymphocytes for HLA-typing.
J. Biolumin. Chemilumin. 1, 4751.
13. Andreotti, P.E. et al. (1995) Chemosensitivity testing of human tumors using a microplate adenosine
triphosphate luminescence assay: Clinical correlation for cisplatin resistance of ovarian carcinoma. Cancer Res.
55, 527682.
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www.promega.com
TB288 Revised 3/15
11
�4.D. Related Products
Cell Proliferation Products
Product
Size Cat.#
ApoLive-Glo Multiplex Assay
10ml
G6410
ApoTox-Glo Triplex Assay
10ml
G6320
CellTiter-Fluor Cell Viability Assay (fluorescent)
10ml
G6080
CellTiter-Blue Cell Viability Assay (resazurin)
CellTiter 96 AQueous One Solution Cell Proliferation Assay (MTS, colorimetric)
CellTiter 96 AQueous Non-Radioactive Cell Proliferation Assay (MTS, colorimetric)
CellTiter 96 AQueous MTS Reagent Powder
CellTiter 96 Non-Radioactive Cell Proliferation Assay (MTT, colorimetric)
20ml
G8080
200 assays
G3582
1,000 assays
G5421
1g
G1111
1,000 assays
G4000
Additional sizes available.
Cytotoxicity Assays
Product
Size Cat.#
CytoTox-Glo Cytotoxicity Assay (luminescent)*
10ml
G9290
Mitochondrial ToxGlo Assay*
10ml
G8000
MultiTox-Glo Multiplex Cytotoxicity Assay (luminescent, fluorescent)*
10ml
G9270
MultiTox-Fluor Multiplex Cytotoxicity Assay (fluorescent)*
10ml
G9200
CytoTox-Fluor Cytotoxicity Assay (fluorescent)*
10ml
G9260
200800 assays
G7890
1,0004,000 assays
G7892
1,000 assays
G1780
GSH-Glo Glutathione Assay
10ml
V6911
50ml V6912
GSH/GSSG-Glo Assay
10ml
50ml V6612
CytoTox-ONE Homogeneous Membrane Integrity Assay (LDH, fluorometric)*
CytoTox-ONE Homogeneous Membrane Integrity Assay, HTP
CytoTox 96 Non-Radioactive Cytotoxicity Assay (LDH, colorimetric)*
V6611
*Additional sizes available.
12
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TB288 Revised 3/15
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�Luminometers
Product
Size Cat.#
GloMax-Multi+ Detection System with Instinct Software:
Base Instrument with Shaking
1 each
E8032
GloMax -Multi+ Detection System with Instinct Software:
Base Instrument with Heating and Shaking
1 each
E9032
GloMax-Multi+ Luminescence Module
1 each
E8041
Apoptosis Products
Product
Size Cat.#
Caspase-Glo 2 Assay*
10ml
G0940
Caspase-Glo 6 Assay*
10ml
G0970
Caspase-Glo 3/7 Assay*
2.5ml
G8090
Caspase-Glo 8 Assay*
2.5ml
G8200
Caspase-Glo 9 Assay*
2.5ml
G8210
1ml
G7792
Apo-ONE Homogeneous Caspase-3/7 Assay
DeadEnd Fluorometric TUNEL System
60 reactions
G3250
DeadEnd Colorimetric TUNEL System
20 reactions
G7360
Anti-ACTIVE Caspase-3 pAb
50l
G7481
Anti-PARP p85 Fragment pAb
50l
G7341
Anti-pS473 Akt pAb
40l
G7441
Caspase Inhibitor Z-VAD-FMK, 20mM
50l
G7231
125l G7232
*Additional sizes available.
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TB288 Revised 3/15
13
�5.
Summary of Change
The following change was made to the 3/15 revision of this document:
Removed an expired patent statement.
(a)
U.S. Pat. Nos. 6,602,677 and 7,241,584, European Pat. No. 1131441, Japanese Pat. Nos. 4537573 and 4520084 and other patents pending.
(b)
(c)
U.S. Pat. No. 7,741,067, Japanese Pat. No. 4485470 and other patents pending.
U.S. Pat. No. 7,700,310, European Pat. No. 1546374 and other patents pending.
(d)
U.S. Pat. Nos 7,083,911, 7,452,663 and 7,732,128, European Pat. No. 1383914 and Japanese Pat. Nos. 4125600 and 4275715.
20012015 Promega Corporation. All Rights Reserved.
Anti-ACTIVE, Apo-ONE, Caspase-Glo, CellTiter 96, CellTiter-Blue, CellTiter-Glo, CytoTox 96 and GloMax are registered trademarks of Promega
Corporation. ApoTox-Glo, ApoLive-Glo, CellTiter-Fluor, CytoTox-Fluor, CytoTox-Glo, CytoTox-ONE, DeadEnd, GSH-Glo, GSH/GSSG-Glo, Instinct, ToxGlo
and Ultra-Glo are trademarks of Promega Corporation.
alamarBlue is a registered trademark of Trek Diagnostic Ssystems, Inc.
Products may be covered by pending or issued patents or may have certain limitations. Please visit our Web site for more information.
All prices and specifications are subject to change without prior notice.
Product claims are subject to change. Please contact Promega Technical Services or access the Promega online catalog for the most up-to-date
information on Promega products.
14
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