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Formation of a covalent complex between methylguanine methyltransferase and DNA via disulfide bond formation between the active site cysteine and a thiol-containing analog of guanine.

机译:通过在活性位点半胱氨酸和鸟嘌呤的含硫醇类似物之间形成二硫键,在甲基鸟嘌呤甲基转移酶和DNA之间形成共价复合物。

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摘要

DNA repair methyltransferases (MTases) remove methyl or other alkyl groups from the O6 position of guanine or the O4 position of thymine by transfering the group to an active site cysteine. In order to trap an MTase-DNA complex via a disulfide bond, 2'-deoxy-6-(cystamine)-2-aminopurine (d6Cys2AP) was synthesized and incorporated into oligonucleotides. d6Cys2AP has a disulfide bond within an alkyl chain linked to the 6 position of 2,6-diaminopurine, which disulfide can be reduced to form a free thiol. Addition of human MTase to reduced oligonucleotide resulted in a protein-DNA complex that was insensitive to denaturation by SDS and high salt, but which readily dissociated in the presence of dithiothreitol. Formation of this complex was prevented by methylation of the active site cysteine. Evidence that the active site cysteine is directly involved in disulfide bond formation was obtained by N-terminal sequencing of peptides that remained associated with DNA after proteolysis of the complex.
机译:DNA修复甲基转移酶(MTase)通过将鸟嘌呤的O6位置或胸腺嘧啶的O4位置转移至活性位点半胱氨酸来去除甲基或其他烷基。为了通过二硫键捕获MTase-DNA复合物,合成了2'-脱氧-6-(胱胺)-2-氨基嘌呤(d6Cys2AP)并将其掺入寡核苷酸中。 d6Cys2AP在连接2,6-二氨基嘌呤6位的烷基链中具有二硫键,该二硫键可被还原形成游离硫醇。将人MTase添加到还原的寡核苷酸中产生了对SDS和高盐变性不敏感的蛋白质-DNA复合物,但是在二硫苏糖醇的存在下容易解离。该复合物的形成通过活性位点半胱氨酸的甲基化来防止。活性位点半胱氨酸直接参与二硫键形成的证据是通过复合物蛋白水解后仍与DNA结合的肽段的N端测序获得的。

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