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MBC in Press, published online ahead of print March 2, 2005
Mol. Biol. Cell 10.1091/mbc.E04-11-1006

A more recent version of this article appeared on May 1, 2005
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Submitted on November 17, 2004
Revised on February 1, 2005
Accepted on February 19, 2005

ATRIP Binding to RPA-ssDNA Promotes ATR-ATRIP Localization but Is Dispensable for Chk1 Phosphorylation

Heather L. Ball, Jeremy S. Myers, and David Cortez

Department of Biochemistry, Vanderbilt University, Nashville, TN 37232

Monitoring Editor: John Cleveland

ATR associates with the regulatory protein ATRIP which has been proposed to localize ATR to sites of DNA damage through an interaction with single-stranded DNA (ssDNA) coated with replication protein A (RPA). We tested this hypothesis and found that ATRIP is required for ATR accumulation at intranuclear foci induced by DNA damage. A domain at the N-terminus of ATRIP is necessary and sufficient for interaction with RPA-ssDNA. Deletion of the ssDNA-RPA interaction domain of ATRIP greatly diminished accumulation of ATRIP into foci. However, the ATRIP-RPA-ssDNA interaction is not sufficient for ATRIP recognition of DNA damage. A splice variant of ATRIP that cannot bind to ATR revealed that ATR association is also essential for proper ATRIP localization. Furthermore, the ATRIP-RPA-ssDNA interaction is not absolutely essential for ATR activation since ATR phosphorylates Chk1 in cells expressing only a mutant of ATRIP that does not bind to RPA-ssDNA. These data suggest that binding to RPA-ssDNA is not the essential function of ATRIP in ATR-dependent checkpoint signaling and ATR has an important function in properly localizing the ATR-ATRIP complex.


Address correspondence to: David Cortez (david.cortez{at}vanderbilt.edu)




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