Three Effective Assays in One Single Product
The ApoTox-Glo™ Triplex Assay combines three assay chemistries to easily assess viability, cytotoxicity and apoptosis events in the same cell-based assay well. First, viability and cytotoxicity are determined by measuring two differential protease biomarkers simultaneously with the addition of a single nonlytic reagent containing two peptide substrates. The live-cell protease activity is restricted to intact viable cells and is measured using a fluorogenic, cell-permeant peptide substrate (GF-AFC Substrate). The substrate enters intact cells, where it is cleaved to generate a fluorescent signal proportional to the number of living cells. This live-cell protease activity marker becomes inactive upon loss of membrane integrity and leakage into the surrounding culture medium.
A second, cell-impermeant, fluorogenic peptide substrate (bis-AAF-R110 Substrate) is used simultaneously to measure dead-cell protease activity that has been released from cells that have lost membrane integrity. This results in ratiometric, inversely correlated measures of cell viability and cytotoxicity. The ratio of viable cells to dead cells is independent of cell number and, therefore, can be used to normalize data. A second reagent containing luminogenic DEVD-peptide substrate for caspase-3/7 and Ultra-Glo™ Recombinant Thermostable Luciferase is added. Caspase-3/7 cleavage of the substrate releases luciferin, which is a substrate for luciferase and generates light. The light output, measured with a luminometer, correlates with caspase-3/7 activation as a key indicator of apoptosis.
Cat.# G6320 contains sufficient reagents for 100 assays in a 96-well plate format or 400 assays in a 384-well format. Cat.# G6321 contains sufficient reagents for 500 assays in a 96-well plate format or 2,000 assays in a 384-well format.
Measure Viability, Cytotoxicity, and Apoptosis in the Same Sample Well
Ionomycin treatment of Jurkat cells for 6 hours results in dose-dependent decrease in viability and increase in cytotoxicity with no caspase-3/7 activation, consistent with primary necrosis.
ApoTox-Glo™ Triplex Assay with suspension Jurkat cells treated with staurosporine. Staurosporine treatment for 6 hours results in a dose-dependent decrease in viability and increase in cytotoxicity with an increase in caspase-3/7 activity consistent with apoptosis.
Camptothecin treatment of Jurkat cells for 48 hours results in dose-dependent decrease in viability, no cytotoxicity and increase in caspase-3/7 activity, consistent with cell-cycle arrest and early-phase apoptosis.
Protocols
Complete Protocol
Quick Protocols
Specifications
Catalog Number:
What's in the box
| Item | Part # | Size |
|---|---|---|
|
GF-AFC Substrate |
G608A | 1 × 10μl |
|
bis-AAF-R110 Substrate |
G609A | 1 × 10μl |
|
Assay Buffer |
G610A | 1 × 10ml |
|
Caspase-Glo® 3/7 Buffer |
G810A | 1 × 10ml |
|
Caspase-Glo® 3/7 Substrate |
G811A | 1 × 1 bottle |
SDS
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Use Restrictions
For Research Use Only. Not for Use in Diagnostic Procedures.Storage Conditions
What's in the box
| Item | Part # | Size |
|---|---|---|
|
GF-AFC Substrate |
G608B | 1 × 50μl |
|
bis-AAF-R110 Substrate |
G609B | 1 × 50μl |
|
Assay Buffer |
G610A | 2 × 10ml |
|
Caspase-Glo® 3/7 Buffer |
G810A | 5 × 10ml |
|
Caspase-Glo® 3/7 Substrate |
G811A | 5 × 1 bottle |
SDS
Search for SDSCertificate of Analysis
Use Restrictions
For Research Use Only. Not for Use in Diagnostic Procedures.Storage Conditions
Resources
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