B cells are activated and proliferate upon activation by specific antigens, anti-Ig antibodies, and/or mitogens.
Principle
B The basic principle of cell activation is that activation and proliferation can occur following activation by specific antigens, anti-Ig antibodies, and/or mitogens.
Operation method
B Cell activation
Materials and Instruments
Reagents: (1) Purified B cells. (2) Anti-IgM antibody, bacterial LPS (E. coli; Difco #011B4). (3) Soluble CD40L, anti-mouse or human CD40 antibody. (4) RPMI 1640 culture medium containing 10% FCS. Instrumentation: (1) 48-well flat-ground culture plate. (2) Flow cytometer
Move
The basic process of B cell activation can be divided into the following steps:
(1) Purified B cells, adjust the B cell concentration to 10/ml with RPMI 1640 culture medium containing 10% FCS.
(2) Add 1 ml of B cell suspension to a 48-well flat-bottom plate, i.e. 1x10/well.
(3) Add one of the following stimuli to the B cell suspension and set up 3 replicate wells for each condition:
(1) Anti-IgM antibody, 2~200μg/ml;
2) LPS, 1~100 μg/ml.
3) sCD40L, 0.03~0.1μg/ml.
4) anti-CD40 antibody, 0.2~0.5μg/ml;
(5) negative control without any stimulant.
(4) Place the culture plate in a 37℃, 5% CO2 cell culture incubator for 24-72 hours to obtain activated B cells.
(5) Collect the B cells and surface label the activated B cells with FACS method for the expression of surface molecules, such as MHC class II molecules, CD80 and CD86.
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