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Caspase 2 Activity Assay Kit (Colorimetric Method)– MSE Supplies LLC

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Caspase 2 Activity Assay Kit (Colorimetric Method)

SKU: E-CK-A382-100

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Caspase 2 Activity Assay Kit (Colorimetric Method)

 

Introduction

Elabscience® Caspase 2 Activity Assay Kit uses spectrophotometry to detect the caspase 2 activity of cells, tissue lysates or other samples.

 

Product Details

Properties

Application Caspase
Assay type Qualitative or quantitative
Detection method Colorimetric Method
Sample type Cell and tissue samples
Assay time 4-6 hours
Detection instrument Spectrophotometer
Other reagents required PBS(E-BC-R187),Bradford Protein Determination Kit(E-BC-K168-S or E-BC-K168-M)
Storage -20°C, shading light
Shipping Ice bag
Expiration date 12 months

 

Detection Principle

Caspase 2, also known as Ich-1(ICE and CED-3 homolog 1) or Nedd-2, can be activated during signal transduction of apoptosis. Caspase 2 mRNA can be cleaved into two different forms. The mRNA product of full-length caspase 2 can be promote apoptosis, while the protein product of short mRNA can inhibit apoptosis. Caspase 2 can be activated by caspase 1, caspase 3 and granzyme B in vitro. This caspase 2 activity assay kit is based on caspase 2 that can catalyze the substrate Ac-VDQQD-pNA to generate yellow pNA (p-Nitroaniline). The pNA has a strong absorption near 405 nm, The activity of caspase 2 can be calculated by determining the absorbance at 405 nm.

 

Storage

Store at -20°C for 1 year. It is recommended to aliquot the AcVDQQD-pNA (4 mM) into smaller quantities and store in the dark. Avoid repeated freezing and thawing.

 

Notes

  1. This kit is for research use only.
  2. Please take safety precautions and follow the procedures of laboratory reagent operation.
  3. The pNA (4-nitroaniline) is toxic to the human body. Please be careful during operating, and pay attention to avoid direct contact with the human body or inhalation. The pNA will solidify at a lower temperature and stick to the bottom, wall or cap of centrifuge tube. It can be used until it is completely melted in a water bath at 20~25°C for a moment.
  4. When the level of activated caspase in the sample is low, first confirm whether apoptosis is obvious. If cell apoptosis is obvious and it is confirmed that the caspase can be activated, the time of inducing cells can be adjusted properly to find a time point when the caspase activation is relatively strong, so as to detect the activation of the caspase. It is recommended to plot a time curve, such as 0, 2, 4, 8, 16, and 24 hours of induction, or 0, 1, 2, 4, 8, and 16 hours, or 0, 1, 2, 4, 6, and 8 hours. Specific induction time needs to be determined according to the specific situation.
  5. In the reaction system of this kit, the initial concentration of the substrate is 0.2 mM. For most samples, the substrate is saturated within 2 hours of incubation at 37°C. For a few samples that the enzyme vitality is particularly high, it is necessary to use Cell Lysis Buffer to dilute the sample appropriately before determination.