After electrophor etic transfer to nitrocellulose, reactive proteins were detected using antisera specific for actin, HtrA2 Omi, UCH L1, HA, PARP 1 and the ECL detection kit. Equal loading as well as efficiency of transfer was routinely verified for all Western blots by Ponceau S staining, and by reprobing the membranes for actin. Generation of monoclonal UCH L1 antibodies Wistar rats were initially immunized intraperitoneally with 100 ug of purified UCH L1 in 60 ul phosphate buffer saline emulsified with 40 ul of Gerbu adjuvant MM. The rats were boosted i. p. on days 14 and 21 with 50 ug of purified protein emulsified with 20% v v of the adjuvant. The last two doses were administered on days 28 and 29 without adjuvant, while the fusion was done on day 30.
Spleen cells from immunized animals were collected and fused with Ag8. 653 myeloma cells using polyethylene glycol 1500. The fused cells were cultured in selection medium for 10 days and screened by ELISA for anti UCH L1 antibodies. Hybridoma clones producing anti UCH L1 monoclonal antibodies were then cultivated in serum free medium and the mAbs were purified using protein G affinity chromato graphy. The isotype of the anti UCH L clone was determined by using ELISA rat mAb isotyping kit. Immunoprecipitations Cellular lysates were precleared with GammaBind G sepharose and immunoprecipitation was performed over night on ice using anti ubiquitin IgG1 monoclonal antibody. After collection of the immunecomple es with GammaBind G sepharose and three washing steps in lysis buffer, the immunoprecipitated proteins were analyzed by SDS PAGE and Western blot.
Generation of stably transfected podocytes with inducible overe pression or downregulation of UCH L1 For inducible overe pression of UCH L1, the Retro Tet On Advanced Inducible E pression System was used according to the manufacturers instructions. Briefly, wildtype murine UCH L1 was amplified by polymerase chain reaction from murine podocytes and subse quently cloned into the multiple cloning site of the pRetro Tight Pur vector using NotI and MluI. The sequence of UCH L1 was verified by sequen cing. For virus production, phoeni ecotropic packaging cells were transfected using DNA CaCl2 precipitation with the pRetro Tet On Advanced vector, with the pRetro Tight Pur UCH L1 vector or the pRetro TightPur empty vector as a control, respectively.
The virus containing supernatant of the pRetro Tet On transfected phoeni cells was transferred Drug_discovery to a 10 cm plate containing podocyte target cells at around 50% to 60% confluence. the infection steps were repeated twice. Selection for integration of the pRetro Tet On Advanced e pression plasmid was per formed with G418 for 7 days. Afterwards, the virus containing supernatant of the pRetro Tight Pur UCH L1 transfected phoeni cells was transferred to the pRetro Tet On Advanced transduced podocyte target cells.
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