Method for evaluating DNA (Deoxyribose Nucleic Acid) damages of peripheral blood lymphocytes caused by ionizing radiation
A technology for DNA damage and lymphocytes, applied in measuring devices, individual particle analysis, scientific instruments, etc., can solve problems such as poor repeatability of experiments and large differences between different individuals
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[0020] 1) Take 0.9ml of peripheral blood from a healthy person using a heparin anticoagulant tube, and divide it into 3 parts, each 0.3ml, of which the first part is not irradiated, the second part is irradiated with 2Gy gamma rays, and the third part is irradiated with 6Gy gamma rays;
[0021] 2) Add 1.5ml of fixative solution (2% paraformaldehyde solution) to the blood sample and let it react for 30 minutes at room temperature;
[0022] 3) Centrifuge at room temperature (500g) for 5 minutes, remove the supernatant;
[0023] 4) Wash the cell pellet with 1.5ml PBS buffer, centrifuge (500g) for 5 minutes at room temperature, remove the supernatant, and keep the pellet;
[0024] 5) Add 1.5ml Triton-100 solution with a concentration of 0.4%, mix the cell pellet, and let it react at room temperature for 15 minutes;
[0025] 6) Centrifuge (500g) for 5 minutes at room temperature, and remove the supernatant;
[0026] 7) Add 1.5ml PBS buffer solution to wash the cells, centrifuge a...
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