Detection of Fcγ Receptor-Mediated Adhesion and Phagocytosis
Author: J.E. Colligan et al, Translator: Xuitao Cao et al, This experiment is from "Compendium Immunology Laboratory Guide".
Operation method
Detection of Fcγ receptor-mediated adhesion and phagocytosis Move Basic scheme FcY receptor-mediated phagocytosis Material Primary macrophages or macrophage cell lines (Elements 6.1 and 8.5) R P M I -5 complete medium (or other medium) Sheep red blood cells (S R B C ), diluted with Alsever's solution I : I (V /V) (Appendix 1) Saline: 0.9 % (m/V) NaCl 200 to 900 Ci/g N a 251CrO4 (30 000 Ci/m m o l , ICN Biomedicals or DuPont N E N ) , saline preparation Polyclonal anti-S R B C antibody (e.g., Diamedix) or anti-FcyRI monoclonal IgG2a type antibody (i.e., conditioner, hybridoma S.S-I, A T C C ) ACK lysate 0.5% (m / V ) SDS solution Stimulants (e.g., mouse IFN-cx/press; see Module 6.4 for other activators) 8-channel pipettes (e.g. Costar Octapette) 9 6-well flat-bottomed cell culture plates (Falcon or Costar) 7 Liquid Flash Meter and 7 Liquid Flash Tubes 15m l and 50m l conical bottom centrifuge tubes IEC Centrifuge (Clinical) Superclearance Collection System (S C S ; Skatron) 1 . Macrophage suspension was prepared and the concentration was adjusted to 2. 5 X IO6 cells/m l . The concentration was adjusted to 2.5 X IO6 cells/m l. The cell suspension was added to each well of a 96-well flat-bottomed culture plate with an 8-channel pipette. Three replicate wells were set up for each experimental group and control group. Place the cells in a cell culture incubator and incubate until the cells are walled (mouse peritoneal macrophages need more than 4 h, other poorly differentiated macrophages may need more time). 2. Add appropriate stimulants to stimulate macrophage Fc y R expression. Type I interferon, such as IFN-a or IFN-p, lOOU/m l, can significantly up-regulate the expression of macrophage FCYR after 48 h. It can be used as a positive control. The group treated with medium alone was used as a negative control. The optimal concentration of different stimulants to regulate the expression of FcYR should be determined according to the pre-test. Additional materials (see basic program for other materials) 2 4-well flat-bottomed cell culture plates (Costar or Falcon) Oscillator, plate type 1 . Prepare a suspension of giant contempt cells and adjust the concentration to 8 X 105 cells/ml. Add 500ul of cell suspension to a 24-well plate. Set up at least 2 duplicate wells for each experimental group and control group. After the cells have attached to the wall in the cell culture incubator, add the stimulant (see basic protocol, steps 1 and 2). 2 . Prepare isotope-labeled and antibody-conditioned SRBC (see basic protocol, steps 4 to 7). Inhibit macrophage phagocytosis by adding 0.I ml of 50 m mol/L iodoacetic acid to 9.9 ml of S RBC suspension. 3 . Add IOOUl of SRBC supernatant to a 7-liquid flash tube containing SCS and read the cp m value (this value is 1/5 of the maximum macrophage adhesion cp m value). 4 . Aspirate the macrophage culture supernatant. Add 500^1 iodoacetic acid-treated SRBC suspension and incubate for I h or for an appropriate period of time (see basic protocol, step 10). 5 . Gently aspirate the unadhered SRBC suspension. Wash the cells by slowly adding 500ul of medium along the wall of the well with an I m l pipette to avoid blowing up macrophages. Repeat the washing 3 times to fully remove the unadhered SRBC. Note: The washing of the second culture plate should be started after the washing of one plate is completely finished. 6. Add 500W of SD S at 0.5% concentration. Add 500W of 0.5 % SD S and shake the plate gently for about 10 min to lyse the macrophages. 7 . Label the 7-fluid flash tubes by number and add to the SDS filter paper. Pipette 400M1 Macrophage Lysate with a micron pipette, carefully add to the appropriate 7-flash tube, and check the cpm value with the 7-flash meter. 8. Calculate the mean value of each sample (see basic protocol, steps 16 to 17). When the results are expressed in terms of SRBC binding, the cp m value of 400 ul of lysate should be converted to the cp m value of 500 ul of total lysate. For more product details, please visit Aladdin Scientific website.
(mouse peritoneal macrophages need more than 4 h, other poorly differentiated macrophages may need a longer time).
3 . The 7 liquid flash tubes were labeled and numbered


150m mol/L iodoacetic acid (I A A; freshly prepared, stored away from light)