| 发布日期: 2012-09-25 16:07 | 文章来源: 丁香园 |
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细胞 细胞培养 技术专题 义翘神州 丁香园 丁香通
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DNA Flow Cytometry (Cell Cycle Analysis)
Stock Solution
Trisodium citrate dehydrate Na3C6H5O7.2H2O 柠檬酸三钠 500 mg
Nonidet P40 (NP40) 0.5 ml
Spermine tetrahydrochloride 四氢氯化精胺 261 mg
Tris (hydroxymethyl)-aminomethane (Tris base) 30 mg
2d-H2O Total 500 ml
Titrate pH to 7.6, Store at 4℃
Citrate Buffer
Sucrose 蔗糖 42.75 g (250 mM)
Trisodium citrate dehydrate Na3C6H5O7.2H2O 2.88 g (40 mM)
DMSO 25 ml
2d-H2O Total 500 ml
Titrate pH to 7.6, Store at 4℃
Solution A:
Trypsin 胰蛋白酶 0.6 mg
Stock soln 100 ml
Titrate pH to 7.6, Store at 4℃
Solution B:
Trypsin inhibitor 胰蛋白酶抑制剂 50 mg
RNase A 10 mg
Stock soln 100 ml
Titrate pH to 7.6, Store at 4℃
Solution C:
Propidium iodide 50 mg
Spermine tetrahydrochloride 116 mg
Stock soln 100 ml
Titrate pH to 7.6, Store at 4℃. Avoid from light exposure
Procedures of DNA Flow Cytometry (Cell Cycle Analysis)
- Cell pellet (2-5X105 cells/sample)
- Resuspend and fix cells in cold citrate buffer for 5-10 min at 4℃to make the cell density 2X105 cells/200 ml citrate buffer. (May keep cells at 4℃for up to 3-5 days)
- Prewarm solutions A and B at room temperature.
- Transfer cells to a Falcon tube (Becton Dickinson FCM tube, #2052 or #2054).
- Add 450 ml Soln A for 10 min at room temp. vigorous vortexing.
- Add 375 ml Soln B for 10 min at room temp. vigorous vortexing.
- Add 100 ml cold Soln C to stain the nuclei. Brief vortexing.
- Run FAScan
The method is according to Vindelov, et al. (Cytometry 1983; 3:323-7) with some modifications.
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