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Department of Microbiology and Immunology, College of Biological Sciences, China Agricultural University, Beijing, 100094, P. R. China

机译:中国农业大学生物科学学院微生物学与免疫学系,北京,100094,P. R.中国

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The interaction of DNA-methyltransferase Ecl18kI (M.Ecl18kI) with a fragment of promoter region of restriction—modification system SsoII was studied. It is shown that dissociation constants of M.Ecl18kI and M.SsoII complexes with DNA ligand carrying a regulatory site previously characterized for M.SsoII have comparable values. A deletion derivative of M.Ecl18kI, Δ(72-379)Ecl18kI, representing the N-terminal protein region responsible for regulation, was obtained. It is shown that such polypeptide fragment has virtually no interaction with the regulatory site. Therefore, the existence of a region responsible for methylation is necessary for maintaining M.Ecl18kI regulatory function. The properties of methyl-transferase NlaX, which is actually a natural deletion derivative of M.Ecl18kI and M.SsoII lacking the first 70 amino acid residues and not being able to regulate gene expression of the SsoII restriction—modification system, were studied. The ability of mutant forms of M.Ecl18kI incorporating single substitutions in regions responsible for regulation and methylation to interact with both sites of DNA recognition was characterized. The data show a correlation between DNA-binding activity of two M.Ecl18kI regions—regulatory and methylating.
机译:研究了DNA-甲基转移酶ECL18KI(M.ECL18KI)与限制性改性系统SSOII启动子区域的片段的相互作用。结果表明,具有预先表征M.SSOII的调节部位的DNA配体的M.ECL18KI和M.SSOII复合物的解离常数具有可比值。得到了代表负责调节的N-末端蛋白区的M.ECL18Ki,δ(72-379)ECL18Ki的缺失衍生物。结果表明,这种多肽片段几乎没有与调节部位相互作用。因此,对维持M.ECL18KI调节功能是必要的存在负责甲基化的区域。研究了甲基转移酶Nlax的性质,其实际上是缺乏前70个氨基酸残基的M.ECL18Ki和M.SSOII的天然缺失衍生物,并且没有能够调节SSOII限制性改性系统的基因表达。特征表征突变形式的M.ECL18KI的突变形式的突变形式掺入负责调节和甲基化的区域中的单一取代。该数据显示两种M.ECL18KI区的DNA结合活性与调节和甲基化之间的相关性。

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