A kinase-independent function of c-Abl in promoting proteolytic destruction of damaged DNA binding proteins.

TitleA kinase-independent function of c-Abl in promoting proteolytic destruction of damaged DNA binding proteins.
Publication TypeJournal Article
Year of Publication2006
AuthorsChen X, Zhang J, Lee J, Lin PS, Ford JM, Zheng N, Zhou P
JournalMol Cell
Volume22
Issue4
Pagination489-99
Date Published2006 May 19
ISSN1097-2765
KeywordsAnimals, Cells, Cultured, Cullin Proteins, DNA Damage, DNA Repair, DNA-Binding Proteins, Gene Silencing, Mice, Proto-Oncogene Proteins c-abl, RNA, Small Interfering, Transcription Factors, Ubiquitin, Ultraviolet Rays
Abstract

Damaged DNA binding proteins (DDBs) play a critical role in the initial recognition of UV-damaged DNA and mediate recruitment of nucleotide excision repair factors. Previous studies identified DDB2 as a target of the CUL-4A ubiquitin ligase. However, the biochemical mechanism governing DDB proteolysis and its underlying physiological function in the removal of UV-induced DNA damage are largely unknown. Here, we report that the c-Abl nonreceptor tyrosine kinase negatively regulates the repair of UV-induced photolesions on genomic DNA. Biochemical studies revealed that c-Abl promotes CUL-4A-mediated DDB ubiquitination and degradation in a manner that does not require its tyrosine kinase activity both under normal growth conditions and following UV irradiation. Moreover, c-Abl activates DDB degradation in part by alleviating the inhibitory effect of CAND1/TIP120A on CUL-4A. These results revealed a kinase-independent function of c-Abl in a ubiquitin-proteolytic pathway that regulates the damage recognition step of nucleotide excision repair.

DOI10.1016/j.molcel.2006.04.021
Alternate JournalMol Cell
PubMed ID16713579
Grant List5R01-CA098210 / CA / NCI NIH HHS / United States
5R01-CA108794 / CA / NCI NIH HHS / United States
T32-GM08539-10 / GM / NIGMS NIH HHS / United States
Related Lab: 
Related Faculty: 
Pengbo Zhou, Ph.D.

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