Recruitment of DNA repair synthesis machinery to sites of DNA damage/repair in living human cells

被引:41
|
作者
Hashiguchi, Kazunari [1 ]
Matsumoto, Yoshihiro
Yasui, Akira
机构
[1] Tohoku Univ, Inst Dev Aging & Canc, Dept Mol Genet, Sendai, Miyagi 9808575, Japan
[2] Fox Chase Canc Ctr, Div Med Sci, Philadelphia, PA 19111 USA
关键词
D O I
10.1093/nar/gkm115
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
The eukaryotic sliding DNA clamp, proliferating cell nuclear antigen ( PCNA), is essential for DNA replication and repair synthesis. In order to load the ring- shaped, homotrimeric PCNA onto the DNA double helix, the ATPase activity of the replication factor C ( RFC) clamp loader complex is required. Although the recruitment of PCNA by RFC to DNA replication sites has well been documented, our understanding of its recruitment during DNA repair synthesis is limited. In this study, we analyzed the accumulation of endogenous and fluorescent-tagged proteins for DNA repair synthesis at the sites of DNA damage produced locally by UVA- laser micro- irradiation in HeLa cells. Accumulation kinetics and in vitro pull- down assays of the large subunit of RFC ( RFC140) revealed that there are two distinct modes of recruitment of RFC to DNA damage, a simultaneous accumulation of RFC140 and PCNA caused by interaction between PCNA and the extreme N- terminus of RFC140 and a much faster accumulation of RFC140 than PCNA at the damaged site. Furthermore, RFC140 knock- down experiments showed that PCNA can accumulate at DNA damage independently of RFC. These results suggest that immediate accumulation of RFC and PCNA at DNA damage is only partly interdependent.
引用
收藏
页码:2913 / 2923
页数:11
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