Caspase 1 Activity Assay Kit
SKU: 69574973757

Caspase 1 Activity Assay Kit

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Description

Caspase 1 Activity Assay KitProduct Specification Usage 1. Preparatory work 1. After the lysate is dissolved, mix well and put on an ice bath for later use. 2. After the detection buffer is dissolved, mix well and place it on an ice bath for later use. 2. Determination of pNA standard curve 1. Preparation of standard diluent: Prepare an appropriate amount of standard diluent according to the ratio of 0. 1 ml of lysate per 0. 9 ml of detection buffer. 2. The pNA provided in the

Product Specification

Usage 1. Preparatory work
1. After the lysate is dissolved, mix well and put on an ice bath for later use.
2. After the detection buffer is dissolved, mix well and place it on an ice bath for later use.

2. Determination of pNA standard curve
1. Preparation of standard diluent: Prepare an appropriate amount of standard diluent according to the ratio of 0.1 ml of lysate per 0.9 ml of detection buffer.
2. The pNA provided in the kit (10 mM) was diluted to 0, 10, 20, 50, 100 and 200 uM with a standard diluent as a standard.
3. Take 100ul of each concentration and detect it with a microplate reader, or take an appropriate amount and detect it with a spectrophotometric detection cup with a capacity of no more than 100ul to determine A405.
4. A405 of each standard was subtracted from A405 of the blank control without pNA to calculate the actual absorbance due to pNA, and a standard curve of pNA concentration versus A405 was created. The pNA standard curve has a good linear relationship in the range of 0-20uM, as shown in the figure below.Note: The experimental data may vary due to different experimental conditions, testing instruments, etc. The data in the figure is for reference only.

3. Sample collection
1. Suspended cells: Centrifuge the control sample that did not induce apoptosis and the sample that induced apoptosis at 600g at 4 º C for 5 minutes to collect the cells, carefully aspirate the supernatant, and ensure that no cells are aspirated as much as possible, and wash once with PBS. After the supernatant was aspirated as before, the lysate was added at a ratio of 100 ul of lysate per 2 million cells, the pellet was resuspended, and lysed in an ice bath for 15 minutes. Go down to Step 4.
2. Adherent cells: suck the cell culture medium for later use. The adherent cells were digested with trypsin and collected into a spare cell culture medium. Collect cells by centrifugation at 600 g at 4 º C for 5 minutes, carefully aspirate the supernatant while ensuring that no cells are aspirated as much as possible, and wash once with PBS. After the supernatant was aspirated as before, the lysate was added at a ratio of 100 ul of lysate per 2 million cells, the pellet was resuspended, and lysed in an ice bath for 15 minutes. Go down to Step 4.
3. Tissue samples: Add lysate at a ratio of 100ul lysate per 3-10mg tissue, and homogenize with a glass homogenizer on an ice bath. The homogenate was then transferred to a 1.5 ml centrifuge tube and lysed in an ice bath for an additional 5 minutes.
4. Centrifuge at 4 º C 16,000-20,000 g for 10-15 minutes.
5. Transfer the supernatant to an ice bath precooled centrifuge tube.
6. The enzyme activity of Caspase 1 was determined immediately or the sample was stored at − 80 ° C. At the same time, a small amount of sample can be taken to measure the protein concentration by Bradford method, and try to make the protein concentration reach 1-3mg/ml, which is equivalent to at least 10-30ug of protein per 10ul of the sample to be tested. If there are fewer cells, the amount of cells can be appropriately increased.

4. Detection of Caspase 1 enzyme activity
1. Take out an appropriate amount of Ac-YVAD-pNA (2mM) and place it on an ice bath for later use.
2. Set up the reaction system as follows:
  Blank control Sample
Assay buffer 40ul 40ul
Sample to be measured 0ul 50ul
Lysate 50ul 0ul
Ac-YVAD-pNA (2 mM) 10ul 10ul
Total Volume 100ul 100ul

Note: When setting the reaction system, add the detection buffer first, then add the sample to be tested, and mix properly. Be careful to avoid bubbles during mixing. An additional 10 ul of Ac-YVAD-pNA (2 mM) was then added.

3. Add Ac-YVAD-pNA (2mM) and mix well, taking care to avoid bubbles during mixing. Incubate at 37 º C for 60-120 minutes. A405 can be measured when the color change is obvious. If the color change is not obvious, the incubation time can be appropriately extended, or even overnight.
4. A405 of the sample minus A405 of the blank control is the absorbance produced by pNA catalyzed by Caspase 1 in the sample. The amount of pNA catalytically produced in the sample can be calculated by comparing it with the standard curve obtained in step 2.
5. Refer to the definition of Caspase 1 enzyme activity unit from Chemicon: One unit is the amount of enzyme that will clear 1.0 nmol of the colorimetric substrate Ac-YVAD-pNA per hour at 37 º C under saturated substrate concentrations. That is, an enzyme activity unit is defined as the amount of caspase 1 enzyme that can cleave 1 nmol of Ac-YVAD-pNA to produce 1 nmol of pNA within one hour at 37 º C when the substrate is saturated. In this way, it is possible to calculate how many enzyme activity units of Caspase 1 are contained in the sample. Note: In the detection system of this kit, the initial concentration of the substrate is 0.2 mM, at which time the substrate is saturated. For many samples, the substrate is saturated within 2 hours of incubation at 37 º C; If the activity of caspase 1 enzyme in the sample is particularly high, the sample must be properly diluted with lysate before determination.
6. Use the Bradford method to detect the protein concentration in the sample to be tested (because the lysate contains a high concentration of DTT, it is not suitable to use the BCA method for protein concentration determination). In this way, the enzyme activity unit of Caspase 1 contained per unit weight of protein in a sample can be calculated.
Synonym interkeukin 1β conberting enzyme,ICE,caspase-1,caspase 1
Detection Type Mammalian tissues, cells
Description

Caspase 1 Activity Detection Kit is a kit for detecting Caspase 1 enzyme activity or purified Caspase 1 enzyme activity in cell or tissue lysates by spectrophotometry. Caspase is a family of proteases involved in the process of apoptosis and contains more than 10 members. Among them, Caspase-1 is the only Caspase that can cleave IL-1b and IL-18 precursors to produce active cytokines. Caspase-11 cleaves the 45 kD Caspase-1 precursor protein to produce 20 kD and 10 kD fragments, which can form heterodimers and further tetramers. This tetramer has protease activity. Caspase-1 regulates apoptosis by cleaving Bcl-XL, and regulates related cytokine-mediated immune inflammatory responses by cleaving cytokine precursors.
This kit is based on the fact that Caspase 1 can catalyze the substrate Ac-YVAD-pNA to produce yellow pNA (p-nitroaniline), so that the activity of Caspase 1 can be detected by measuring absorbance. pNA has strong absorption near 405nm. This kit can detect 20 samples (20T) or 100 samples (100T) in addition to the standard curve when detected with a microplate reader or a spectrophotometric detection cup with a capacity not exceeding 100ul.
Product Components:

Product composition 20T 100T
Lysate Lysis buffer 8ml 30ml
Assay buffer 8ml 20ml
Ac-YVAD-pNA (2 mM) 200ul 1ml
pNA (10 mM) 200ul 1ml

 

Storage Temp. When stored at-20 °C, Ac-YVAD-pNA and pNA need to be stored in the dark.
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SKU: 69574973757

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