Fusion is an important procedure to produce monoclonal antibodies (MoAb
网站地图本站论坛
高级搜索收藏本站
热门关键字: 细胞培养  pcr  琼脂糖凝胶电泳  质粒DNA的提取  凝胶加样缓冲液  PCR inventor
 
 当前位置:试验方案>蛋白试验>免疫学> 正文

Fusion is an important procedure to produce monoclonal antibodies (MoAb

点击:   作者:   来源:  时间: 2007-04-10  本站论坛
Fusion is an important procedure to produce monoclonal antibodies (MoAb).

PROTOCOL
  1. prepare the culture of myeloma cells and maintain the concentration of the cells at the level of less than 10^6 cells/ml (IMDM 10% FCS/FBS). Just before the fusion wash 3 times in IMDM (serum free!), 1200 rpm, 5min, 37ѓC. Count cells.
  2. sacrifice the mouse and dissect the spleen.
  3. tease the spleen in ice-cold IMDM (serum free!); pass through the nylon filter; wash 3 times in IMDM (serum free!), 1200 rpm, 5min, 37ѓC. Count cells.
  4. mix 10^8 spleen cells (in 25 ml of IMDM [serum free]) with 2x10^7 myeloma cells (in 25 ml of IMDM [serum free]) in Falcon-50 ml conical tube.
  5. centrifuge at 1200 rpm, 5 min, 37ѓC.
  6. aspirate the supernatant (SN) with a Pasteur pipette (all till the last drop!!!)
  7. gently break the pellet by tapping of the bottom of the tube.
  8. place the tube on 37ѓC water bath; add slowly, dop by drop 1 ml of pre-warmed (37ѓC) 50% PEG 1500 (polyethylene glycol, Roche, Germany) continously stirring the cells with the pipette tip (this procedure lasts for a period over 1 min)
  9. add 1 ml of pre-warmed to 37ѓC IMDM continously stirring the mixture (this procedure lasts for a period over 1 min).
  10. add 3 ml of pre-warmed to 37ѓC IMDM continously stirring the mixture (this procedure lasts for a period over 3 min).
  11. add 10 ml of pre-warmed to 37ѓC IMDM continously stirring the mixture (this procedure lasts for a period over 1-2 min).
  12. let to stay for 5 min on the 37ѓC water bath.
  13. centrifuge at 1200 rpm, 5 min, 37ѓC; aspirate the SN.
  14. resuspend the cells in IMDM-FCS(10%v/v) - HTx100 (1%v/v) - AJ(5%v/v) - IL-6, 0.5x10^6 cells/ml (calculation figured out from the number of spleen cells the fusion was started from); let to stay in incubator, 37ѓC, pCO2 7% for 2 hours in a big flasc.
  15. add aminopterin; distribute on 96-wells cell culture plates (Nunc) (200µl/well); place in incubator (37ѓC, pCO2 7%) enveloped in aluminium paper.
  16. check the cultures 1-2-7 days after the fusion.
  17. on day 7-10 change the culture medium.
  18. test clones when thay occupy 25% of the bottom surface of the well.
SOLUTIONS
  1. IMDM (Iscove's Modified Dulbecco's Medium with 25 mM Hepes/with L-Glutamine) BioWhittaker Europe Cat.: BE12-722F
  2. IMDM-FCS(10%v/v)-HTx100(1%v/v)-AJ(5%v/v)-IL-6 (100 U/ml)
  3. IMDM - FCS(10%v/v) - HTx100(1%v/v) - AJ(5%v/v) - IL 6 (100 U/ml) - aminopterine x100 (1% v/v)
  4. HT (hypoxantine-thymidine)x100, 0.22 (or 0.45) µm-filtered, store at -20ѓC = hypoxantine solution, 50 ml thymidine solution, 50 ml ddH2O up to 250 ml
  5. hypoxantine solution = hypoxantine, 340 mg ddH2O up to 50 ml NaOH 1 N, 3 ml -> heat to 37ѓC
  6. thymidine solution = thymidine (2'-desoxy-thymidine), 96 mg ddH2O up to 50 ml
  7. AJ (from "ajouter" , to add, local slang), 3 L, 0.22 (or 0.45) µm-filtered, store at -20ѓC = Asp-Arg x100, 1 L Gluta x 50, 2 L mercaptoethanol, 350 µl
  8. Asp-Arg x100, 1 L, pH 6.0 = L-Asparagine, 3.6 g (0.24 mM) L-Arginine (0.55 mM), 11.6 g HCl, 0.5N, 100 ml -> heat to 37ѓC, add ddH2O up to 1 L
  9. Gluta x50, 1 L, pH 6.0 = glutamine, 10.8 g (1.48 mM) HCl, 0.5N, 100 ml -> heat to 37ѓC, add ddH2O up to 1 L
  10. aminopterine x100, 0.22-0.45 µm-filtered, store at -20ѓC = aminopterine, 4.4 mg (3.8µM) ddH2O, 50 ml NaOH, 1N, 100 µl-> heat to 37ѓC, add ddH2O up to 250 ml
    fusion

上一篇:Tips and hints for the storage of antibodies   下一篇:Protocol for Cell Fusion

 
推荐文章
 
相关文章
推荐专题
 


↑返回顶部   打印本页   关闭窗口↓  
 本站申明 联系我们 网站地图
Copyright© 试验方案

Powered by DedeCms email:htmyth#yahoo.com.cn

Optimized to 1024x768 to Firefox,Opera and MS-IE6