CASPASSY-RO
Roche
Homogeneous Caspases Assay, fluorimetric
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About This Item
Fabricant/nom de marque
Roche
Conditions d'expédition
dry ice
Température de stockage
−20°C
Description générale
The Homogeneous Caspases Assay is a fluorimetric assay for the quantitative in vitro determination of caspases activity in microplates, which makes it especially useful for high-throughput screening.
Spécificité
Enzyme activity of natural and recombinant caspase is detected by this homogeneous caspases assay. Activated caspases 2, 3, 6, 7, 8, 9, and 10 can be analyzed with different sensitivity.
Application
Specific, quantitative in vitro determination of caspases in microplates.
During apoptosis, the activation of specific proteases, called Caspases (cysteinyl-aspartic-acid-proteases), is one of the initial intracellular biochemical events. The Homogeneous Caspases Assay can be used to detect caspase activity in life-science research applications:
During apoptosis, the activation of specific proteases, called Caspases (cysteinyl-aspartic-acid-proteases), is one of the initial intracellular biochemical events. The Homogeneous Caspases Assay can be used to detect caspase activity in life-science research applications:
- for sensitive quantification of activated caspases
- for screening of caspase inhibitors
- as an automatable one-step assay for high-throughput screening
Caractéristiques et avantages
- Determine a specific stage of apoptosis
- Detect caspases of human and animal origin
- Perform high-throughput screening
- Minimize hands-on time; use this automatable one-step assay
Conditionnement
1 kit containing 4 components
Principe
The Homogeneous Caspases Assay is a fluorimetric one-step assay for the quantitative in vitro determination of caspase activity in microplates. Cells are cultured in microplates and apoptosis is induced, causing an activation of caspases. After an appropriate incubation period, caspases substrate (DEVD-R110), diluted in incubation buffer, is added and incubated for 1 - 2 hours. During this incubation period, the cells are lysed by the Incubation buffer and the caspases substrate is cleaved in proportion to the amount of activated caspases. The fluorescent dye Rhodamine 110 is released and fluorometrically determined at λmax = 521nm.
The developed fluorochrome is proportional to the concentration of activated caspases, and can be quantified in a calibration curve.
The total assay time is approximately 1.5 hours (excluding cell culturing).
The developed fluorochrome is proportional to the concentration of activated caspases, and can be quantified in a calibration curve.
The total assay time is approximately 1.5 hours (excluding cell culturing).
Autres remarques
For life science research only. Not for use in diagnostic procedures.
Composants de kit seuls
Réf. du produit
Description
- Substrate (DEVD-R110) Stock Solution 500 μM
- Positive Control 10x concentrated
- R 110 Standard
- Incubation Buffer
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