Application
This kit can be used for detection of Ca2+-ATPase activity in animal tissue, culture cells and other samples.
Detection significance
ATPase exists on the membrane of tissue cells and organelles. It is a kind of protease on the biological membrane which plays an important role in material transport, energy conversion and information transmission. The enzyme activity of ATPase will have a series of changes when the body in the hypoxic or diseases condition, and is also associated with some genetic diseases.
Detection principle
ATPase can decompose ATP into ADP and inorganic phosphorus. ATPase activity can be calculated by determining the content of inorganic phosphorus.
Experimental instruments
Test tube, Micropipettor
Vortex mixer
37℃ water bath
Spectrophotometer (636nm)
Sample pretreatment
1. Tissue:
Weigh the tissue accurately, add 9 times of normal saline at the ratio of Weight (g): Volume (mL) = 1:9. Make the mechanical homogenization in ice water bath to prepare 10% homogenate. Centrifuge at 2500 rpm for 10 min and take the supernatant (10% homogenate). Then dilute the 10% homogenate with normal saline for 10 times to prepare 1% homogenate for detection. Meanwhile, determine the protein concentration of supernatant (E-BC-K318, E-BC-K168, E-BC-K165). If the result of pre-experiment is too high, dilute the 1% tissue homogenate to different concentrations for pre-experiment and determine the sample concentration according to the result.
2. Culture cell samples:
Collect and centrifuge the culture cells, discard the supernatant and keep the cell sediment. Add 0.2~0.3 mL of normal saline or homogenate medium to prepare 107/mL cell suspension, then broken the cells by homogenizer, ultrasonic crusher or freezing/thawing cycles. The prepared cell suspension does not need to be centrifuged. Meanwhile, determine the protein concentration of supernatant (E-BC-K318, E-BC-K168, E-BC-K165).Then dilute the cell homogenate to different concentrations for pre-experiment and determine the sample concentration according to the result.
[Note] 1. The sample must be mix fully when test the sample.
2. Do not use phosphate buffer or phosphorus-containing reagents as homogenization media or dilute samples.
3. The absolute OD value (the OD value of sample- the OD value of control) in pre-experiment should be control about 0.2.
4. The enzyme activity will be affect when treat the cells by freezing/thawing cycles.
Operation steps
1. Enzymatic reaction
| Control tube | Sample tube |
Reagent 1 (μL) | 70 | 70 |
Reagent 2 (μL) | 20 |
|
Reagent 3 (μL) |
| 20 |
Reagent 4 (μL) | 20 | 20 |
Reagent 5 (μL) |
| 20 |
Reagent 6 (μL) | 20 |
|
Sample (μL) |
| 100 |
Mix fully and react at 37℃for 10 min exactly. | ||
Reagent 7 (μL) | 50 | 50 |
Sample (μL) | 100 |
|
Mix fully and centrifuge at 3500 rpm for 10 min and take 150 μL of the supernatant to determine phosphorus. |
2. Determination of phosphorus
| Blank tube | Standard tube | Control tube | Sample tube |
Double-distilled water (mL) | 0.15 |
|
|
|
0.02 μmol/mL phosphorus standard application solution (mL) |
| 0.15 |
|
|
Supernatant (mL) |
|
| 0.15 | 0.15 |
Phosphorus determination reagent (mL) | 0.5 | 0.5 | 0.5 | 0.5 |
Mix fully and stand for 2 min at room temperature. | ||||
Stop solution (mL) | 0.5 | 0.5 | 0.5 | 0.5 |
Mix fully and stand for 5 min at room temperature. Set to zero with double-distilled water and measure the OD values at 636 nm with 0.5 cm diameter cuvette. |
Note: the cuvette should be rinse with running water for 10 times and then wash with double distilled water for 4~5 times. It will avoid the contamination of phosphorus.
Notes
1. This kit is for research use only.
2. Please progress strictly with operation procedures.
3. Do not use components from different batches of kit.
4. The valid period of kit is 6 months and the expiration date is on the packing box.
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