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An Assay to Evaluate Immunodominance in Cytotoxic T Lymphocyte Responses

An Assay to Evaluate Immunodominance in Cytotoxic T Lymphocyte Responses

筆記録

For injection of the target cells, first, gently vortex the source tubes and pool the three CFSE-labeled cell suspensions into a new tube at equal ratios. Top up the tube contents with sterile PBS, and collect the cells by centrifugation for counting. Then, adjust the volume to a 1 x 107 mixed target cells per 200 microliters of PBS per recipient concentration, and inject 200 microliter volumes of the cell suspension into the tail vein of each recipient C57-Black-6 mouse.

Two or four hours after the injection, remove and process the spleen of each recipient animal as demonstrated, and resuspend the isolated white blood cells in 3 milliliters of PBS per spleen. Transfer approximately 1 times 10 to the 7th cells from each processed spleen into a clean FACS tube, and immediately run the cells on the flow cytometer as demonstrated to gate the CFSE low, intermediate, and high target cell populations.

Then, acquire a total of 2,000 CFSE low events in the fluorescence one channel, and calculate the specific lysis of each cognate target cell population, according to the formula detailed in the text.

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