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The restriction endonuclease R.NmeDI from Neisseria meningitidis that recognizes a palindromic sequence and cuts the DNA on both sides of the recognition sequence

机译:脑膜炎奈瑟氏球菌的限制性内切酶R.NmeDI识别回文序列并在识别序列的两侧切割DNA

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摘要

The restriction endonuclease Type II R.NmeDI from Neisseria meningitidis 2120 (serogroup C, ST-11 complex) was characterized. The cloned nmeDIR gene was expressed in Escherichia coli cells, and the endonucleolytic and restriction activities of R.NmeDI were then observed in vitro and in vivo. The nmeDIR gene consists of 1056 bp coding 351 aa protein with a calculated molecular weight of M(r) = 39 000 ± 1000 Da. The R.NmeDI enzyme was purified to apparent homogeneity following overexpression, using metal affinity chromatography. This enzyme recognizes a palindrome sequence and cleaves double-stranded DNA upstream and downstream of its recognition sequence (12/7) RCCGGY (7/12) (R = A/G, Y = C/T) cutting out a 25-bp fragment. R.NmeDI cleaves in two steps. The enzyme cleaves the first strand randomly on either side of the recognition sequence generating an intermediate, and the second cleavage occurs more slowly and results in the production of a final reaction product. The R.NmeDI endonuclease requires two recognition sequences for effective cleavage. The tetramer is an active form of the R.NmeDI enzyme.
机译:表征了来自脑膜炎奈瑟氏球菌2120(血清群C,ST-11复合体)的II型限制性核酸内切酶R.NmeDI。克隆的nmeDIR基因在大肠杆菌细胞中表达,并在体内和体外观察到R.NmeDI的内切核酸酶和限制酶活性。 nmeDIR基因由1056 bp编码351 aa蛋白质组成,分子量为M(r)= 39 000±1000 Da。使用金属亲和色谱法,在过度表达后,将R.NmeDI酶纯化至表观均匀性。该酶识别回文序列并在其识别序列的上游和下游切割双链DNA(12/7)RCCGGY(7/12)(R = A / G,Y = C / T)切出25 bp的片段。 R.NmeDI分为两个步骤。该酶在识别序列的任一侧随机切割第一条链,生成中间体,第二次切割发生的速度较慢,并导致最终反应产物的产生。 R.NmeDI核酸内切酶需要两个识别序列才能有效裂解。四聚体是R.NmeDI酶的活性形式。

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