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Cited 104 time in webofscience Cited 105 time in scopus
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MutS switches between two fundamentally distinct clamps during mismatch repair SCIE SCOPUS

Title
MutS switches between two fundamentally distinct clamps during mismatch repair
Authors
Jeong, CCho, WKSong, KMCook, CYoon, TYBan, CFishel, RLee, JB
Date Issued
2011-03
Publisher
NATURE PUBLISHING GROUP
Abstract
Single-molecule trajectory analysis has suggested DNA repair proteins may carry out a one-dimensional (1D) search on naked DNA encompassing > 10,000 nucleotides. Organized cellular DNA (chromatin) presents substantial barriers to such lengthy searches. Using dynamic single-molecule fluorescence resonance energy transfer, we determined that the mismatch repair (MMR) initiation protein MutS forms a transient clamp that scans duplex DNA for mismatched nucleotides by 1D diffusion for 1 s (similar to 700 base pairs) while in continuous rotational contact with the DNA. Mismatch identification provokes ATP binding (3 s) that induces distinctly different MutS sliding clamps with unusual stability on DNA (similar to 600 s), which may be released by adjacent single-stranded DNA (ssDNA). These observations suggest that ATP transforms short-lived MutS lesion scanning clamps into highly stable MMR signaling clamps that are capable of competing with chromatin and recruiting MMR machinery, yet are recycled by ssDNA excision tracts.
Keywords
ESCHERICHIA-COLI MUTS; NONPOLYPOSIS COLORECTAL-CANCER; DNA MISMATCH; SINGLE-MOLECULE; FLUORESCENCE SPECTROSCOPY; RECOGNITION COMPLEX; HETERODUPLEX DNA; SLIDING CLAMP; PROTEIN MUTS; HMSH2-HMSH6
URI
https://oasis.postech.ac.kr/handle/2014.oak/24958
DOI
10.1038/NSMB.2009
ISSN
1545-9985
Article Type
Article
Citation
NATURE STRUCTURAL & MOLECULAR BIOLOGY, vol. 18, no. 3, page. 379 - U174, 2011-03
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