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The non-specific adenine DNA methyltransferase M. EcoGII

机译:非特异性腺嘌呤DNA甲基转移酶M. Ecogii

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We describe the cloning, expression and characterization of the first truly non-specific adenine DNA methyltransferase, M.EcoGII. It is encoded in the genome of the pathogenic strain Escherichia coli O104: H4 C227-11, where it appears to reside on a cryptic prophage, but is not expressed. However, when the gene encoding M. EcoGII is expressed in vivo - using a high copy pRRS plasmid vector and a methylation-deficient E. coli host-extensive in vivo adenine methylation activity is revealed. M. EcoGII methylates adenine residues in any DNA sequence context and this activity extends to dA and rA bases in either strand of a DNA: RNA-hybrid oligonucleotide duplex and to rA bases in RNAs prepared by in vitro transcription. Using oligonucleotide and bacteriophage M13mp18 virion DNA substrates, we find that M. EcoGII also methylates single-stranded DNA in vitro and that this activity is only slightly less robust than that observed using equivalent double-stranded DNAs. In vitro assays, using purified recombinant M. EcoGII enzyme, demonstrate that up to 99% of dA bases in duplex DNA substrates can be methylated thereby rendering them insensitive to cleavage by multiple restriction endonucleases. These properties suggest that the enzyme could also be used for high resolution mapping of protein binding sites in DNA and RNA substrates.
机译:我们描述了第一个真正非特异性腺嘌呤DNA甲基转移酶M.ecogii的克隆,表达和表征。它在致病菌株大肠杆菌O104:H4 C227-11的基因组中编码,在那里它似乎存在于隐蔽的预兆上,但未表达。然而,当编码M. Ecogii的基因在体内表达时 - 使用高拷贝PRRS质粒载体和甲基化缺陷的大肠杆菌宿主在体内腺嘌呤甲基化活性中进行。 M. Ecogii在任何DNA序列上下文中的腺嘌呤残基,该活性延伸到DNA的任一链中的DA和Ra碱:RNA杂化寡核苷酸双链链和通过体外转录制备的RNA中的Ra碱基。使用寡核苷酸和噬菌体M13MP18 Viorion DNA基质,我们发现M. Ecogii在体外也甲基化单链DNA,并且该活性仅比使用当量的双链DNA观察到的稳定性略低。在体外测定中,使用纯化的重组M. eCogii酶,证明高达99%的双相DNA基材中的DA碱可以甲基化,从而使它们不敏感以通过多种限制内切核酸核酸核酸裂解不敏感。这些性质表明酶也可用于DNA和RNA基材中的蛋白质结合位点的高分辨率映射。

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