Structure of the MutL C-terminal domain: a model of intact MutL and its roles in mismatch repair

Guarné, Alba; Ramón‐Maiques, Santiago; Wolff, Erika M.; Ghirlando, Rodolfo; Hu, Xiaojian; Miller, Jeffrey H; Yang, Wei

doi:10.1038/sj.emboj.7600412

Cited by 166 publications

(296 citation statements)

References 58 publications

(77 reference statements)

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“…In contrast to E. coli MutL, the N-terminal fragment of hPMS2 remains a monomer in the crystal structure, even in the presence of ATP, and the monomeric fragment is capable of ATP hydrolysis (Guarne et al, 2001). A crystal structure of a C-terminal dimerization domain of E. coli MutL reveals a V-shaped dimer that plays critical roles in the activation of UvrD by MutL and in DNA binding by MutL (Guarne et al, 2004). The DNA binding activity of MutL has been shown to be essential for methyl-directed MMR in E. coli (Robertson et al, 2006a).…”

Section: Mutation Avoidance and Post-replication Repairmentioning

confidence: 98%

DNA mismatch repair: Molecular mechanism, cancer, and ageing

Hsieh

Yamane

2008

Mechanisms of Ageing and Development

376

359

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DNA mismatch repair (MMR) proteins are ubiquitous players in a diverse array of important cellular functions. In its role in post-replication repair, MMR safeguards the genome correcting base mispairs arising as a result of replication errors. Loss of MMR results in greatly increased rates of spontaneous mutation in organisms ranging from bacteria to humans. Mutations in MMR genes cause hereditary nonpolyposis colorectal cancer, and loss of MMR is associated with a significant fraction of sporadic cancers. Given its prominence in mutation avoidance and its ability to target a range of DNA lesions, MMR has been under investigation in studies of ageing mechanisms. This review summarizes what is known about the molecular details of the MMR pathway and the role of MMR proteins in cancer susceptibility and ageing.

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Section: Mutation Avoidance and Post-replication Repairmentioning

confidence: 98%

DNA mismatch repair: Molecular mechanism, cancer, and ageing

Hsieh

Yamane

2008

Mechanisms of Ageing and Development

376

359

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“…Interestingly, the substitution within the DQHA(X) 2 E(X) 4 E motif of E. coli MutL includes two Arg residues, and these Arg sidechains were shown to be important for DNA binding (Fig. 2B) [8]. In the modeled PMS2 structure, the DQHA(X) 2 E(X) 4 E motif is juxtaposed to another sequence motif, CXHGRP, conserved among hPMS2-like MutL homologs ( Fig.…”

mentioning

confidence: 97%

“…This conserved motif is mapped onto an exposed surface of the C-terminal domain based on the crystal structure of the E. coli protein ( Fig. 2A) since all MutL homologs are predicted to have a conserved tertiary fold [8,9]. Interestingly, the substitution within the DQHA(X) 2 E(X) 4 E motif of E. coli MutL includes two Arg residues, and these Arg sidechains were shown to be important for DNA binding (Fig.…”

mentioning

confidence: 99%

“…In the modeled PMS2 structure, the DQHA(X) 2 E(X) 4 E motif is juxtaposed to another sequence motif, CXHGRP, conserved among hPMS2-like MutL homologs ( Fig. 2A) [8,9]. Although the overall structure and arrangement of the conserved residues in hPMSs do not immediately resemble any known nucleases, conserved Cys, His, Asp and Glu residues in this region can readily form a metal ion-binding site.…”

mentioning

confidence: 99%

“…To avoid non-mismatch-dependent activation, the MutH endonuclease activity needs to be negatively regulated. Both SeqA and the Dam methylase in E. coli bind and compete for hemimethylated GATC with much lower K d 's (nM) than that of MutH (μM) [8,[18][19][20][21]. They likely prevent MutH from accessing the newly synthesized daughter strand in the absence of a mismatch.…”

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Human MutLα: The jack of all trades in MMR is also an endonuclease

Yang

2007

DNA Repair

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SummaryRecently, Paul Modrich's group reported the discovery of an intrinsic endonuclease activity for human MutLα. This breakthrough provides a satisfactory answer to the longstanding puzzle of a missing nuclease activity in human mismatch repair and will undoubtedly lead to new investigations of DNA repair and replication. Here, the implications of this exciting new finding are discussed in the context of mismatch repair in E. coli and humans.Correction of replication errors by mismatch repair (MMR) has long been recognized as critical for genomic stability. Inactivation of MMR in humans has been implicated in > 90% of hereditary nonpolyposis colorectal cancers [1]. Like every DNA repair process, the success of MMR depends on two essential steps: lesion detection and removal. MMR is unique in two aspects. The targets of repair are normal rather than damaged nucleotides, and nucleotide removal has to be specific to the newly synthesized daughter strand and not the template. E. coli MMR is the best understood and has been fully reconstituted in vitro using a dozen or so purified proteins [2,3]. Recognition of a normal nucleotide that fails to make a Watson-Crick base pair in a DNA duplex is accomplished by the MutS protein. The strand specificity of MMR in E. coli is conferred by a sequence and methylation specific endonuclease MutH, which makes an incision (nick) 5′ to a GATC sequence in the unmethylated daughter strand. The GATC sequence may be several hundred base pairs from the mismatch on either the 5′ or 3′ side (Fig. 1A). The direction of daughter strand removal is strongly biased towards the shorter track between the nick and mismatch in a circular genome. The degradation of hundreds to a thousand nucleotides is carried out by one of several exonucleases with 5′ → 3′ or 3′-gt; 5′ polarity in the presence of the UvrD helicase and the single strand binding protein SSB. An additional central player in MMR is MutL, a molecular matchmaker that mediates proteinprotein interactions and coordinates mismatch recognition with strand incision and degradation (Fig. 1A).The MMR pathway is conserved from E. coli to humans [3]. The essential proteins known to specialize in human MMR are so far limited to MutS and MutL homologs and a 5′ → 3′ exonuclease, ExoI. Eukaryotic MutS and MutL are heterodimers of homologous subunits as opposed to homodimers in bacteria. Human MutSα consists of MSH2 and MSH6, and MutLα consists of MLH1 and PMS2. A strand-specific endonuclease that nicks the daughter strand, like MutH in E. coli, is missing in all eukaryotes and in many bacteria. It is thusCorrespondence and request for material should be addressed to W.Y. e-mail: Wei.Yang@nih.gov phone: (301), 402-4645, fax: (301) 496-0201. Publisher's Disclaimer: This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its...

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MutL: conducting the cell's response to mismatched and misaligned DNA

Polosina

Cupples

2009

BioEssays

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Base pair mismatches in DNA arise from errors in DNA replication, recombination, and biochemical modification of bases. Mismatches are inherently transient. They are resolved passively by DNA replication, or actively by enzymatic removal and resynthesis of one of the bases. The first step in removal is recognition of strand discontinuity by one of the MutS proteins. Mismatches arising from errors in DNA replication are repaired in favor of the base on the template strand, but other mismatches trigger base excision or nucleotide excision repair (NER), or non-repair pathways such as hypermutation, cell cycle arrest, or apoptosis. We argue that MutL homologues play a key role in determining biologic outcome by recruiting and/or activating effector proteins in response to lesion recognition by MutS. We suggest that the process is regulated by conformational changes in MutL caused by cycles of ATP binding and hydrolysis, and by physiologic changes which influence effector availability.

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Structure of the MutL C-terminal domain: a model of intact MutL and its roles in mismatch repair

Cited by 166 publications

References 58 publications

DNA mismatch repair: Molecular mechanism, cancer, and ageing

DNA mismatch repair: Molecular mechanism, cancer, and ageing

Human MutLα: The jack of all trades in MMR is also an endonuclease

MutL: conducting the cell's response to mismatched and misaligned DNA

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