Structural basis for removal of adenine mispaired with 8-oxoguanine by MutY adenine DNA glycosylase

Fromme, J. Christopher; Banerjee, Anirban; Huang, Susan; Verdine, Gregory L.

doi:10.1038/nature02306

Cited by 304 publications

(489 citation statements)

References 24 publications

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“…In E. coli MutY, the corresponding mutations (Y82C and G253D) lead to modest decreases in substrate binding affinity and rate of excision [77]. In addition, structural studies show that Y82 and G253 interact with the DNA near the 8-oxoguanine lesion site [39][40]. It is likely that Y82 and G253 are involved in substrate recognition, but it is still not completely understood how all of the mutations implicated in MAP give rise to cancer.…”

Section: Discussionmentioning

confidence: 99%

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DNA repair glycosylases with a [4Fe–4S] cluster: A redox cofactor for DNA-mediated charge transport?

Boal

Yavin

Barton

2007

Journal of Inorganic Biochemistry

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The [4Fe-4S] cluster is ubiquitous to a class of base excision repair enzymes, in organisms ranging from bacteria to man, and was first considered as a structural element, owing to its redox stability under physiological conditions. When studied bound to DNA, two of these repair proteins (MutY and Endonuclease III from Escherichia coli) display DNA-dependent reversible electron transfer with characteristics typical of high potential iron proteins. These results have inspired a reexamination of the role of the [4Fe-4S] cluster in this class of enzymes. Might the [4Fe-4S] cluster be used as a redox cofactor to search for damaged sites using DNA-mediated charge transport, a process well known to be highly sensitive to lesions and mismatched bases? Described here are experiments demonstrating the utility of DNA-mediated charge transport in characterizing these DNA-binding metalloproteins, as well as efforts to elucidate this new function for DNA as an electronic signaling medium among the proteins.

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Section: Discussionmentioning

confidence: 99%

“…Crystal structures are available for MutY and Endo III both free and bound to DNA [18][19][20][39][40]. These provide many clues about the environment of the cluster in both states.…”

Section: Introductionmentioning

confidence: 99%

DNA repair glycosylases with a [4Fe–4S] cluster: A redox cofactor for DNA-mediated charge transport?

Boal

Yavin

Barton

2007

Journal of Inorganic Biochemistry

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“…Such configurations are relatively common, as, for example, in structures of the conserved motif IVof the 4.5 S RNA alone, 46 the SRP RNA complex with Ffh M domain, 47 the RNA complexes of the SRP Alu domain, 48 and DNA-editing complexes involved in repair and excision of 8-oxoguanine:adenine mispairs. 49,50 Previously, mutations of residues associated with the activation region, in particular Arg195, have been assayed in the context of the assembled SRP: FtsY complex 15 and found to exhibit deficiencies in GTPase activation. It is possible that these defects, rather than reflecting a contribution to the chemistry of GTP hydrolysis per se (as in an arginine finger mechanism 51 ), reflect instead interactions of the activation region with the 4.5 S RNA of the SRP.…”

Section: Discussionmentioning

confidence: 99%

Structure of a GDP:AlF4 Complex of the SRP GTPases Ffh and FtsY, and Identification of a Peripheral Nucleotide Interaction Site

Focia

Gawronski-Salerno

Coon

et al. 2006

Journal of Molecular Biology

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The signal recognition particle (SRP) GTPases Ffh and FtsY play a central role in co-translational targeting of proteins, assembling in a GTP-dependent manner to generate the SRP targeting complex at the membrane. A suite of residues in FtsY have been identified that are essential for the hydrolysis of GTP that accompanies disengagement. We have argued previously on structural grounds that this region mediates interactions that serve to activate the complex for disengagement and term it the activation region. We report here the structure of a complex of the SRP GTPases formed in the presence of GDP:AlF 4 . This complex accommodates the putative transition-state analog without undergoing significant change from the structure of the ground-state complex formed in the presence of the GTP analog GMPPCP. However, small shifts that do occur within the shared catalytic chamber may be functionally important. Remarkably, an external nucleotide interaction site was identified at the activation region, revealed by an unexpected contaminating GMP molecule bound adjacent to the catalytic chamber. This site exhibits conserved sequence and structural features that suggest a direct interaction with RNA plays a role in regulating the activity of the SRP targeting complex.

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“…1). 24 In addition, the removal of N3 is unlikely to affect base pairing with OG, and therefore should not globally alter the recognition features of the mismatched base pair or the ease with which MutY mediates base pair disruption. Thus, the reduced ability of MutY to remove Z3 relative to A is likely due to alterations of the electronic properties of the base.…”

mentioning

confidence: 99%

“…DNA bending and distortion that is associated with forming the catalytically competent DNA-MutY intermediate is expected to be facilitated by electrostatic and hydrogenbonding interactions of DNA backbone phosphates with amino acid side chains and backbone amides. 24 In the case of G:A substrates, accessing the catalytically competent intermediate must rely heavily on nonspecific electrostatic interactions to explain the sensitivity to the increased salt concentration. 36,37 In contrast, with OG:A substrates, nonspecific electrostatic interactions are not as critical for efficient adenine removal.…”

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confidence: 99%

Unnatural substrates reveal the importance of 8-oxoguanine for in vivo mismatch repair by MutY

et al. 2007

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Escherchia coli MutY plays an important role in preventing mutations associated with the oxidative lesion 7,8-dihydro-8-oxo-2′-deoxyguanosine (OG) in DNA by excising adenines from OG:A mismatches as the first step of base excision repair. To determine the importance of specific steps in the base pair recognition and base removal process of MutY, we have evaluated the effects of modifications of the OG:A substrate on the kinetics of base removal, mismatch affinity and repair to G:C in an Escherchia coli-based assay. Surprisingly, adenine modification was tolerated in the cellular assay, while modification of OG results in minimal cellular repair. High affinity for the mismatch and efficient base removal require the presence of OG. Taken together, these results suggest that the presence of OG is a critical feature for MutY to locate OG:A mismatches and select the appropriate adenines for excision to initiate repair in vivo prior to replication.The mismatch repair (MMR) pathway in E. coli relies on methylation at a GATC sequence to direct the repair machinery to remove the mismatched base on the newly synthesized strand. 1 However, almost two decades ago, an activity was detected in E. coli cell extracts that restored G:A mismatches to G:C matches and was insensitive to the methylation state of the template strand. [2][3][4] Concurrently, a mutator locus in E. coli (mutY) was identified that generated G:C → T:A transversion mutations. 5 It was later determined that the mutY gene product is an adenine glycosylase capable of removing adenines from G:A mismatches as the first step in base excision repair (BER). [6][7][8][9][10] The subsequent activity of downstream BER pathway enzymes, e.g. the AP endonuclease, deoxyribophosphate lyase, polymerase and ligase, restores the G:C base pair in a methylation-independent fashion. 11 MutY was also found to participate in the prevention of mutations caused by 7,8-dihydro-8-oxo-2′-deoxyguanosine (OG, 1) by removal of adenine from OG:A mismatches. 10,12,13,14 Polymerase misinsertion of dAMP opposite OG creates OG:A mismatches that can lead to formation of T:A base pairs upon a second round of replication. 12 Recently, MutY has been in the spotlight due to the correlation between inherited biallelic mutations in the gene encoding the human homologue of MutY (MUTYH) and colorectal cancer. 10,15,16 *Author to whom correspondence should be addressed. Email: david@chem.ucdavis.edu,. # These authors contributed equally to this manuscript. We have previously examined the features of mismatched substrates that are required for efficient lesion recognition and adenine excision by MutY using pre-steady state and singleturnover kinetics. [17][18][19] Pre-steady state experiments revealed that MutY has a high affinity for the product such that release of the DNA product is rate-limiting. 17,19,20 Moreover, the identity of the base opposite A greatly affects both the rate of product release as well as the intrinsic rate of adenine removal determined under single-turnover conditions....

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Structural basis for removal of adenine mispaired with 8-oxoguanine by MutY adenine DNA glycosylase

Cited by 304 publications

References 24 publications

DNA repair glycosylases with a [4Fe–4S] cluster: A redox cofactor for DNA-mediated charge transport?

DNA repair glycosylases with a [4Fe–4S] cluster: A redox cofactor for DNA-mediated charge transport?

Structure of a GDP:AlF4 Complex of the SRP GTPases Ffh and FtsY, and Identification of a Peripheral Nucleotide Interaction Site

Unnatural substrates reveal the importance of 8-oxoguanine for in vivo mismatch repair by MutY

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