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M1.MboII和M2.MboII型IIS甲基转移酶:特异性不同,作用靶点相同。

M1.MboII and M2.MboII type IIS methyltransferases: different specificities, the same target.

作者信息

Furmanek-Blaszk Beata, Boratynski Robert, Zolcinska Natalia, Sektas Marian

机构信息

Department of Microbiology, University of Gdansk, 80-822 Gdansk, Kladki 24, Poland.

出版信息

Microbiology (Reading). 2009 Apr;155(Pt 4):1111-1121. doi: 10.1099/mic.0.025023-0.

Abstract

Methylation of a base in a specific DNA sequence protects the DNA from nucleolytic cleavage by restriction enzymes recognizing the same sequence. The MboII restriction-modification (R-M) system of Moraxella bovis ATCC 10900 consists of a restriction endonuclease gene and two methyltransferase genes. The enzymes encoded by this system recognize an asymmetrical sequence 5'-GAAGA-3'/3'-CTTCT-5'. M1.MboII modifies the last adenine in the recognition sequence 5'-GAAGA-3' to N(6)-methyladenine. A second methylase, M2.MboII, was cloned and purified to electrophoretic homogeneity using a four-step chromatographic procedure. It was demonstrated that M2.MboII modifies the internal cytosine in the recognition sequence 3'-CTTCT-5', yielding N(4)-methylcytosine, and moreover is able to methylate single-stranded DNA. The protein exists in solution as a monomer of molecular mass 30 000+/-1000 Da under denaturing conditions. Divalent cations (Ca(2+), Mg(2+), Mn(2+) and Zn(2+)) inhibit M2.MboII methylation activity. It was found that the isomethylomer M2.NcuI from Neisseria cuniculi ATCC 14688 behaves in the same manner. Functional analysis showed that the complete MboII R-M system, consisting of two methyltransferases genes and the mboIIR gene, is the most stable and the least harmful to bacterial cells.

摘要

特定DNA序列中碱基的甲基化可保护DNA免受识别相同序列的限制性内切酶的核酸酶切割。牛莫拉菌ATCC 10900的MboII限制修饰(R-M)系统由一个限制性内切酶基因和两个甲基转移酶基因组成。该系统编码的酶识别不对称序列5'-GAAGA-3'/3'-CTTCT-5'。M1.MboII将识别序列5'-GAAGA-3'中的最后一个腺嘌呤修饰为N(6)-甲基腺嘌呤。通过四步色谱法克隆并纯化了第二种甲基化酶M2.MboII,使其达到电泳纯。结果表明,M2.MboII修饰识别序列3'-CTTCT-5'中的内部胞嘧啶,生成N(4)-甲基胞嘧啶,而且能够甲基化单链DNA。在变性条件下,该蛋白以分子量为30 000±1000 Da的单体形式存在于溶液中。二价阳离子(Ca(2+)、Mg(2+)、Mn(2+)和Zn(2+))抑制M2.MboII的甲基化活性。发现来自兔源奈瑟菌ATCC 14688的同甲基化异构体M2.NcuI表现出相同的行为。功能分析表明,由两个甲基转移酶基因和mboIIR基因组成的完整MboII R-M系统最稳定,对细菌细胞的危害最小。

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