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编码Eco RI核酸内切酶和甲基化酶的DNA序列分析。

Sequence analysis of the DNA encoding the Eco RI endonuclease and methylase.

作者信息

Greene P J, Gupta M, Boyer H W, Brown W E, Rosenberg J M

出版信息

J Biol Chem. 1981 Mar 10;256(5):2143-53.

PMID:6257703
Abstract

The Eco RI endonuclease and methylase recognize the same hexanucleotide substrate sequence. We have determined the sequence of a fragment of DNA which encodes these enzymes using the chain-termination method of Sanger (Sanger, F., Nicklen, S., and Coulson, A. R. (1977) Proc. Natl. Acad. Sci. U. S. A. 74, 5463-5467). The amino acid sequences of both enzymes were derived from the DNA sequence. The coding regions selected include the only open translational frames of sufficient length to accommodate the enzymes. They coincide with previously established gene boundaries and orientation. The predicted amino acid sequences correlate well with analyses of the purified protein. Comparison of the nucleotide and protein sequences reveals no homology between the endonuclease and methylase which might provide insight into the origin of the restriction-modification system or the mechanism of common substrate recognition. Based on secondary structure predictions, the two enzymes also have grossly different molecular architecture. The base composition of the sequence is 65% A + T, and the codon usage is significantly different from that observed in several Escherichia coli chromosomal genes. In some cases, frequently selected codons are recognized by minor tRNA species. A spontaneous mutation in the endonuclease gene was isolated. Serine replaces arginine at residue 187. In crude extracts, Eco RI specific cleavage is approximately 0.3% wild type.

摘要

Eco RI核酸内切酶和甲基化酶识别相同的六核苷酸底物序列。我们使用桑格的链终止法(桑格,F.,尼克伦,S.,和库尔森,A. R.(1977年)《美国国家科学院院刊》74,5463 - 5467)确定了编码这些酶的一段DNA片段的序列。两种酶的氨基酸序列均由该DNA序列推导得出。所选的编码区域包括唯一足够长以容纳这些酶的开放阅读框。它们与先前确定的基因边界和方向一致。预测的氨基酸序列与纯化蛋白质的分析结果高度相关。核苷酸和蛋白质序列的比较表明,核酸内切酶和甲基化酶之间没有同源性,这可能为限制 - 修饰系统的起源或共同底物识别机制提供见解。基于二级结构预测,这两种酶的分子结构也有很大差异。该序列的碱基组成为65%的A + T,密码子使用情况与在几个大肠杆菌染色体基因中观察到的情况有显著差异。在某些情况下,常用密码子由次要tRNA种类识别。分离出了核酸内切酶基因中的一个自发突变。在第187位残基处,丝氨酸取代了精氨酸。在粗提物中,Eco RI特异性切割约为野生型的0.3%。

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