Crosstalk between CST and RPA regulates RAD51 activity during replication stress

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作者
Kai-Hang Lei
Han-Lin Yang
Hao-Yen Chang
Hsin-Yi Yeh
Dinh Duc Nguyen
Tzu-Yu Lee
Xinxing Lyu
Megan Chastain
Weihang Chai
Hung-Wen Li
Peter Chi
机构
[1] National Taiwan University,Institute of Biochemical Sciences
[2] National Taiwan University,Department of Chemistry
[3] Loyola University Chicago Stritch School of Medicine,Department of Cancer Biology, Cardinal Bernardin Cancer Center
[4] Washington State University,Office of Research
[5] Academia Sinica,Institute of Biological Chemistry
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Replication stress causes replication fork stalling, resulting in an accumulation of single-stranded DNA (ssDNA). Replication protein A (RPA) and CTC1-STN1-TEN1 (CST) complex bind ssDNA and are found at stalled forks, where they regulate RAD51 recruitment and foci formation in vivo. Here, we investigate crosstalk between RPA, CST, and RAD51. We show that CST and RPA localize in close proximity in cells. Although CST stably binds to ssDNA with a high affinity at low ionic strength, the interaction becomes more dynamic and enables facilitated dissociation at high ionic strength. CST can coexist with RPA on the same ssDNA and target RAD51 to RPA-coated ssDNA. Notably, whereas RPA-coated ssDNA inhibits RAD51 activity, RAD51 can assemble a functional filament and exhibit strand-exchange activity on CST-coated ssDNA at high ionic strength. Our findings provide mechanistic insights into how CST targets and tethers RAD51 to RPA-coated ssDNA in response to replication stress.
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