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Taq MutS蛋白氨基末端区域与异源双链DNA大沟的光交联作用。

Photocross-linking of the NH2-terminal region of Taq MutS protein to the major groove of a heteroduplex DNA.

作者信息

Malkov V A, Biswas I, Camerini-Otero R D, Hsieh P

机构信息

Genetics and Biochemistry Branch, NIDDK, National Institutes of Health, Bethesda, Maryland 20892-1810, USA.

出版信息

J Biol Chem. 1997 Sep 19;272(38):23811-7. doi: 10.1074/jbc.272.38.23811.

DOI:10.1074/jbc.272.38.23811
PMID:9295328
Abstract

The MutS DNA mismatch repair protein recognizes heteroduplex DNAs containing mispaired or unpaired bases. To identify regions of MutS protein in close proximity to the heteroduplex DNA, we have utilized the photoactivated cross-linking moiety 5-iododeoxyuridine (5-IdUrd). Nucleoprotein complexes of Thermus aquaticus MutS protein bound to monosubstituted 5-IdUrd-containing heteroduplex DNAs were cross-linked with long-wavelength ultraviolet light. Positioning of the 5-IdUrd moiety at one of three positions within the DNA bulge, two nucleotides upstream or three nucleotides downstream of the unpaired base, resulted in an identical subset of cross-linked peptides as determined by proteolytic fingerprinting. The tryptic peptide cross-linked to an unpaired 5-IdUrd residue was determined by peptide sequencing to correspond to a highly conserved region spanning residues 25-49. Cross-linking to the bulge nucleotide occurred at Phe-39, indicating that this residue contacts, or is in close proximity to, the unpaired base of a heteroduplex DNA. Site-directed mutagenesis resulting in the substitution of Ala for Phe-39 reduced the affinity of the mutant protein for heteroduplex DNA by roughly 3 orders of magnitude, but had no apparent effect on its ability to dimerize, its thermostability, or its ATPase activity. These results implicate the region in the vicinity of Phe-39 as being crucial for heteroduplex DNA binding by Taq MutS protein.

摘要

MutS DNA错配修复蛋白可识别含有错配或未配对碱基的异源双链DNA。为了确定MutS蛋白中与异源双链DNA紧密相邻的区域,我们利用了光活化交联部分5-碘脱氧尿苷(5-IdUrd)。嗜热水生菌MutS蛋白与单取代含5-IdUrd的异源双链DNA结合的核蛋白复合物用长波长紫外线进行交联。将5-IdUrd部分定位在DNA凸起内三个位置之一、未配对碱基上游两个核苷酸处或下游三个核苷酸处,通过蛋白水解指纹图谱确定,交联肽的子集相同。通过肽测序确定与未配对的5-IdUrd残基交联的胰蛋白酶肽对应于一个高度保守的区域,该区域跨越第25至49位残基。与凸起核苷酸的交联发生在Phe-39处,表明该残基与异源双链DNA的未配对碱基接触或紧密相邻。定点诱变导致用Ala取代Phe-39,使突变蛋白对异源双链DNA的亲和力降低了约3个数量级,但对其二聚化能力、热稳定性或ATPase活性没有明显影响。这些结果表明,Phe-39附近的区域对于Taq MutS蛋白结合异源双链DNA至关重要。

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Photocross-linking of the NH2-terminal region of Taq MutS protein to the major groove of a heteroduplex DNA.Taq MutS蛋白氨基末端区域与异源双链DNA大沟的光交联作用。
J Biol Chem. 1997 Sep 19;272(38):23811-7. doi: 10.1074/jbc.272.38.23811.
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