MutS/MutL crystal structure reveals that the MutS sliding clamp loads MutL onto DNA

To avoid mutations in the genome, DNA replication is generally followed by DNA mismatch repair (MMR). MMR starts when a MutS homolog recognizes a mismatch and undergoes an ATP-dependent transformation to an elusive sliding clamp state. How this transient state promotes MutL homolog recruitment and activation of repair is unclear. Here we present a crystal structure of the MutS/MutL complex using a site-specifically crosslinked complex and examine how large conformational changes lead to activation of MutL. The structure captures MutS in the sliding clamp conformation, where tilting of the MutS subunits across each other pushes DNA into a new channel, and reorientation of the connector domain creates an interface for MutL with both MutS subunits. Our work explains how the sliding clamp promotes loading of MutL onto DNA, to activate downstream effectors. We thus elucidate a crucial mechanism that ensures that MMR is initiated only after detection of a DNA mismatch.

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Cryo-EM structures reveal how ATP and DNA binding in MutS coordinate the sequential steps of DNA mismatch repair

10.1101/2021.06.03.446775 ◽

2021 ◽

Author(s):

Alessandro Borsellini ◽

Vladislav Kunetsky ◽

Peter Friedhoff ◽

Meindert H. Lamers

Keyword(s):

Dna Binding ◽

Mismatch Repair ◽

Conformational Changes ◽

Atp Hydrolysis ◽

Dna Mismatch Repair ◽

Atp Binding ◽

Dna Mismatch ◽

Sliding Clamp ◽

Adp Release ◽

Atp Binding And Hydrolysis

DNA mismatch repair detects and removes mismatches from DNA reducing the error rate of DNA replication a 100-1000 fold. The MutS protein is one of the key players that scans for mismatches and coordinates the repair cascade. During this, MutS undergoes multiple conformational changes that initiate the subsequent steps, in response to ATP binding, hydrolysis, and release. How ATP induces the different conformations in MutS is not well understood. Here we present four cryo-EM structures of Escherichia coli MutS at sequential stages of the ATP hydrolysis cycle. These structures reveal how ATP binding and hydrolysis induces a closing and opening of the MutS dimer, respectively. Additional biophysical analysis furthermore explains how DNA binding modulates the ATPase cycle by preventing hydrolysis during scanning and mismatch binding, while preventing ADP release in the sliding clamp state. Nucleotide release is achieved when MutS encounters single stranded DNA that is produced during the removal of the daughter strand. This way, the combination of the ATP binding and hydrolysis and its modulation by DNA enable MutS to adopt different conformations needed to coordinate the sequential steps of the mismatch repair cascade.

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Trapping a transient state in DNA mismatch repair: the MutS/MutL sliding clamp loads MutL on DNA

Acta Crystallographica Section A Foundations and Advances ◽

10.1107/s2053273315099830 ◽

2015 ◽

Vol 71 (a1) ◽

pp. s10-s10

Author(s):

Titia K. Sixma

Keyword(s):

Mismatch Repair ◽

Dna Mismatch Repair ◽

Transient State ◽

Dna Mismatch ◽

Sliding Clamp

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Functional Studies on the Candidate ATPase Domains of Saccharomyces cerevisiae MutLα

Molecular and Cellular Biology ◽

10.1128/mcb.20.17.6390-6398.2000 ◽

2000 ◽

Vol 20 (17) ◽

pp. 6390-6398 ◽

Cited By ~ 59

Author(s):

Phuoc T. Tran ◽

R. Michael Liskay

Keyword(s):

Saccharomyces Cerevisiae ◽

Mismatch Repair ◽

Conformational Changes ◽

Atp Hydrolysis ◽

Dna Mismatch Repair ◽

Limited Proteolysis ◽

Atp Binding ◽

Dna Mismatch ◽

Functional Studies

ABSTRACT Saccharomyces cerevisiae MutL homologues Mlh1p and Pms1p form a heterodimer, termed MutLα, that is required for DNA mismatch repair after mismatch binding by MutS homologues. Recent sequence and structural studies have placed the NH2 termini of MutL homologues in a new family of ATPases. To address the functional significance of this putative ATPase activity in MutLα, we mutated conserved motifs for ATP hydrolysis and ATP binding in both Mlh1p and Pms1p and found that these changes disrupted DNA mismatch repair in vivo. Limited proteolysis with purified recombinant MutLα demonstrated that the NH2 terminus of MutLα undergoes conformational changes in the presence of ATP and nonhydrolyzable ATP analogs. Furthermore, two-hybrid analysis suggested that these ATP-binding-induced conformational changes promote an interaction between the NH2 termini of Mlh1p and Pms1p. Surprisingly, analysis of specific mutants suggested differential requirements for the ATPase motifs of Mlh1p and Pms1p during DNA mismatch repair. Taken together, these results suggest that MutLα undergoes ATP-dependent conformational changes that may serve to coordinate downstream events during yeast DNA mismatch repair.

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The properties of Msh2–Msh6 ATP binding mutants suggest a signal amplification mechanism in DNA mismatch repair

Journal of Biological Chemistry ◽

10.1074/jbc.ra118.005439 ◽

2018 ◽

Vol 293 (47) ◽

pp. 18055-18070 ◽

Cited By ~ 5

Author(s):

William J. Graham ◽

Christopher D. Putnam ◽

Richard D. Kolodner

Keyword(s):

Mismatch Repair ◽

Binding Sites ◽

Signal Amplification ◽

Dna Mismatch Repair ◽

Nucleotide Binding ◽

Atp Binding ◽

Dna Mismatch ◽

Nucleotide Binding Sites ◽

Sliding Clamp ◽

Atp Concentration

DNA mismatch repair (MMR) corrects mispaired DNA bases and small insertion/deletion loops generated by DNA replication errors. After binding a mispair, the eukaryotic mispair recognition complex Msh2–Msh6 binds ATP in both of its nucleotide-binding sites, which induces a conformational change resulting in the formation of an Msh2–Msh6 sliding clamp that releases from the mispair and slides freely along the DNA. However, the roles that Msh2–Msh6 sliding clamps play in MMR remain poorly understood. Here, using Saccharomyces cerevisiae, we created Msh2 and Msh6 Walker A nucleotide–binding site mutants that have defects in ATP binding in one or both nucleotide-binding sites of the Msh2–Msh6 heterodimer. We found that these mutations cause a complete MMR defect in vivo. The mutant Msh2–Msh6 complexes exhibited normal mispair recognition and were proficient at recruiting the MMR endonuclease Mlh1–Pms1 to mispaired DNA. At physiological (2.5 mm) ATP concentration, the mutant complexes displayed modest partial defects in supporting MMR in reconstituted Mlh1–Pms1-independent and Mlh1–Pms1-dependent MMR reactions in vitro and in activation of the Mlh1–Pms1 endonuclease and showed a more severe defect at low (0.1 mm) ATP concentration. In contrast, five of the mutants were completely defective and one was mostly defective for sliding clamp formation at high and low ATP concentrations. These findings suggest that mispair-dependent sliding clamp formation triggers binding of additional Msh2–Msh6 complexes and that further recruitment of additional downstream MMR proteins is required for signal amplification of mispair binding during MMR.

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DNA Mismatch Repair System Gets Involved in DNA Replication by Removing Aberrant Structures♦

Journal of Biological Chemistry ◽

10.1074/jbc.p115.660357 ◽

2015 ◽

Vol 290 (40) ◽

pp. 24066-24066

Keyword(s):

Dna Replication ◽

Mismatch Repair ◽

Dna Mismatch Repair ◽

Repair System ◽

Dna Mismatch ◽

Dna Mismatch Repair System ◽

Mismatch Repair System

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Somatic Hypermutation in Muts Homologue (Msh)3-, Msh6-, and Msh3/Msh6-Deficient Mice Reveals a Role for the Msh2–Msh6 Heterodimer in Modulating the Base Substitution Pattern

Journal of Experimental Medicine ◽

10.1084/jem.191.3.579 ◽

2000 ◽

Vol 191 (3) ◽

pp. 579-584 ◽

Cited By ~ 150

Author(s):

Margrit Wiesendanger ◽

Burkhard Kneitz ◽

Winfried Edelmann ◽

Matthew D. Scharff

Keyword(s):

Immune Response ◽

Dna Replication ◽

Mismatch Repair ◽

Dna Mismatch Repair ◽

Somatic Hypermutation ◽

Hot Spot ◽

Base Substitution ◽

Substitution Pattern ◽

Dna Mismatch ◽

Deficient Mice

Although the primary function of the DNA mismatch repair (MMR) system is to identify and correct base mismatches that have been erroneously introduced during DNA replication, recent studies have further implicated several MMR components in somatic hypermutation of immunoglobulin (Ig) genes. We studied the immune response in mice deficient in MutS homologue (MSH)3 and MSH6, two mutually exclusive partners of MSH2 that have not been examined previously for their role in Ig hypermutation. In Msh6−/− and Msh3−/−/Msh6−/− mice, base substitutions are preferentially targeted to G and C nucleotides and to an RGYW hot spot, as has been shown previously in Msh2−/− mice. In contrast, Msh3−/− mice show no differences from their littermate controls. These findings indicate that the MSH2–MSH6 heterodimer, but not the MSH2–MSH3 complex, is responsible for modulating Ig hypermutation.

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The crystal structure of DNA mismatch repair protein MutS binding to a G·T mismatch

Nature ◽

10.1038/35037523 ◽

2000 ◽

Vol 407 (6805) ◽

pp. 711-717 ◽

Cited By ~ 446

Author(s):

Meindert H. Lamers ◽

Anastassis Perrakis ◽

Jacqueline H. Enzlin ◽

Herrie H. K. Winterwerp ◽

Niels de Wind ◽

...

Keyword(s):

Crystal Structure ◽

Mismatch Repair ◽

Dna Mismatch Repair ◽

Dna Mismatch ◽

Repair Protein ◽

Mismatch Repair Protein

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mlh3 separation of function and endonuclease defective mutants display an unexpected effect on meiotic recombination outcomes

10.1101/108498 ◽

2017 ◽

Cited By ~ 2

Author(s):

Najla Al-Sweel ◽

Vandana Raghavan ◽

Abhishek Dutta ◽

V. P. Ajith ◽

Luigi Di Vietro ◽

...

Keyword(s):

Dna Replication ◽

Mismatch Repair ◽

Protein Interactions ◽

Meiotic Recombination ◽

Meiotic Division ◽

Dna Mismatch Repair ◽

Crossing Over ◽

Baker's Yeast ◽

Protein Protein Interactions ◽

Dna Mismatch

AbstractMlh1-Mlh3 is an endonuclease hypothesized to act in meiosis to resolve double Holliday junctions into crossovers. It also plays a minor role in eukaryotic DNA mismatch repair (MMR). To understand how Mlh1-Mlh3 functions in both meiosis and MMR, we analyzed in baker’s yeast 60 new mlh3 alleles. Five alleles specifically disrupted MMR, whereas one (mlh3-32) specifically disrupted meiotic crossing over. Mlh1-mlh3 representatives for each separation of function class were purified and characterized. Both Mlh1-mlh3-32 (MMR+, crossover-) and Mlh1-mlh3-45 (MMR-, crossover+) displayed wild-type endonuclease activities in vitro. Msh2-Msh3, an MSH complex that acts with Mlh1-Mlh3 in MMR, stimulated the endonuclease activity of Mlh1-mlh3-32 but not Mlh1-mlh3-45, suggesting that Mlh1-mlh3-45 is defective in MSH interactions. Whole genome recombination maps were constructed for two mlh3 mutants with opposite separation of function phenotypes, and an endonuclease defective mutant. Unexpectedly, all three showed increases in the number of non-crossover events that were not observed in mlh3Δ. Our observations provide a structure-function map for Mlh3 that reveals the importance of protein-protein interactions in regulating Mlh1-Mlh3’s enzymatic activity. They also illustrate how defective meiotic components can alter the fate of meiotic recombination intermediates, providing new insights for how meiotic recombination pathways are regulated.Author SummaryDuring meiosis, diploid germ cells that become eggs or sperm undergo a single round of DNA replication followed by two consecutive chromosomal divisions. The segregation of chromosomes at the first meiotic division is dependent in most organisms on at least one genetic exchange, or crossover event, between chromosome homologs. Homologs that do not receive a crossover frequently undergo non-disjunction at the first meiotic division, yielding gametes that lack chromosomes or contain additional copies. Such events have been linked to human disease and infertility. Recent studies suggest that the Mlh1-Mlh3 complex is an endonuclease that resolves recombination intermediates into crossovers. Interestingly, this complex also acts as a matchmaker in DNA mismatch repair (MMR) to remove DNA replication errors. How does one complex act in two different processes? We investigated this question by performing a mutational analysis of the baker’s yeast Mlh3 protein. Five mutations were identified that disrupted MMR but not crossing over, and one mutation disrupted crossing over while maintaining MMR. Using a combination of biochemical and genetic analyses to further characterize these mutants we illustrate the importance of protein-protein interactions for Mlh1-Mlh3’s activity. Importantly, we illustrate how defective meiotic components can alter the outcome of meiotic recombination events. They also provide new insights in our understanding of the basis of infertility syndromes.

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