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Analysis of the subunit assembly of the typeIC restriction-modification enzyme EcoR124I.

机译:TypeIC限制性修饰酶EcoR124I的亚基组装分析。

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Type I restriction-modification (R-M) enzymes are composed of three different subunits, of which HsdS determines DNA specificity, HsdM is responsible for DNA methylation and HsdR is required for restriction. The HsdM and HsdS subunits can also form an independent DNA methyltransferase with a subunit stoichiometry of M2S1. We found that the purified Eco R124I R-M enzyme was a mixture of two species as detected by the presence of two differently migrating specific DNA-protein complexes in a gel retardation assay. An analysis of protein subunits isolated from the complexes indicated that the larger species had a stoichiometry of R2M2S1and the smaller species had a stoichiometry of R1M2S1. In vitro analysis of subunit assembly revealed that while binding of the first HsdR subunit to the M2S1complex was very tight, the second HsdR subunit was bound weakly and it dissociated from the R1M2S1complex with an apparent K d of approximately 2.4 x 10(-7) M. Functional assays have shown that only the R2M2S1complex is capable of DNA cleavage, however, the R1M2S1complex retains ATPase activity. The relevance of this situation is discussed in terms of the regulation of restriction activity in vivo upon conjugative transfer of a plasmid-born R-M system into an unmodified host cell.
机译:I型限制性修饰(R-M)酶由三个不同的亚基组成,其中HsdS决定DNA特异性,HsdM负责DNA甲基化,HsdR要求限制性。 HsdM和HsdS亚基也可以形成化学计量为M2S1的独立DNA甲基转移酶。我们发现,纯化的Eco R124I R-M酶是两种物质的混合物,通过在凝胶延迟测定中存在两种不同迁移的特定DNA-蛋白质复合物来检测。从复合物中分离的蛋白质亚基的分析表明,较大的物种具有R2M2S1的化学计量,较小的物种具有R1M2S1的化学计量。亚基装配体的体外分析表明,尽管第一个HsdR亚基与M2S1复合体的结合非常紧密,但第二个HsdR亚基却被弱结合,并从R1M2S1复合体中解离,表观K d约为2.4 x 10(-7)M功能测定表明,只有R2M2S1复合物能够进行DNA切割,但是,R1M2S1复合物保留了ATP酶活性。关于这种情况的相关性,将在将携带质粒的R-M系统偶联转移到未修饰的宿主细胞中后,在体内限制活性的调节方面进行讨论。

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