首页> 外文期刊>Nucleic Acids Research >The HsdR subunit of R.EcoR124II: cloning and over-expression of the gene and unexpected properties of the subunit.
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The HsdR subunit of R.EcoR124II: cloning and over-expression of the gene and unexpected properties of the subunit.

机译:R.EcoR124II的HsdR亚基:基因的克隆和过表达以及该亚基的意外特性。

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摘要

Type I restriction endonucleases are composed of three subunits, HsdR, HsdM and HsdS. The HsdR subunit is absolutely required for restriction activity; while an independent methylase is composed of HsdM and HsdS subunits. DNA cleavage is associated with a powerful ATPase activity during which DNA is translocated by the enzyme prior to cleavage. The presence of a Walker type I ATP-binding site within the HsdR subunit suggested that the subunit may be capable of independent enzymatic activity. Therefore, we have, for the first time, cloned and over-expressed the hsdRgene of the type IC restriction endonuclease EcoR124II. The purified HsdR subunit was found to be a soluble monomeric protein capable of DNA- and Mg2+-dependent ATP hydrolysis. The subunit was found to have a weak nuclease activity both in vivo and in vitro, and to bind plasmid DNA; although was not capable of binding a DNA oligoduplex. We were also able to reconstitute the fully active endonuclease from purified M. EcoR124I and HsdR. This isthe first clear demonstration that the HsdR subunit of a type I restriction endonuclease is capable of independent enzyme activity, and suggests a mechanism for the evolution of the endonuclease from the independent methylase.
机译:I型限制性核酸内切酶由三个亚基组成:HsdR,HsdM和HsdS。 HsdR亚基是限制活性的绝对必需。而独立的甲基化酶则由HsdM和HsdS亚基组成。 DNA切割与强大的ATPase活性相关,在此期间,DNA在切割前被酶转移。 HsdR亚基中存在Walker I型ATP结合位点提示该亚基可能具有独立的酶促活性。因此,我们首次克隆并过表达了IC型限制性核酸内切酶EcoR124II的hsdR基因。发现纯化的HsdR亚基是能够进行DNA和Mg2 +依赖性ATP水解的可溶性单体蛋白。发现该亚基在体内和体外均具有弱的核酸酶活性,并能结合质粒DNA。尽管不能结合DNA寡聚体。我们还能够从纯化的M. EcoR124I和HsdR重构完全活性的核酸内切酶。这是第一个明确的证明,I型限制性核酸内切酶的HsdR亚基具有独立的酶活性,并暗示了核酸内切酶从独立的甲基化酶进化的机制。

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