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EcoRi及其他限制性内切酶的反应

The reactions of the EcoRi and other restriction endonucleases.

作者信息

Halford S E, Johnson N P, Grinsted J

出版信息

Biochem J. 1979 May 1;179(2):353-65. doi: 10.1042/bj1790353.

Abstract

The reaction of the EcoRI restriction endonuclease was studied with both the plasmid pMB9 and DNA from bacteriophage lambda as the substrates. With both circular and linear DNA molecules, the only reaction catalysed by the EcoRI restriction endonuclease was the hydrolysis of the phosphodiester bond within one strand of the recognition site on the DNA duplex. The cleavage of both strands of the duplex was achieved only after two independent reactions, each involving a single-strand scission. The reactivity of the enzyme for single-strand scissions was the same for both the first and the second cleavage within its recognition site. No differences were observed between the mechanism of action on supercoiled and linear DNA substrates. Other restriction endonucleases were tested against plasmid pMB9. The HindIII restriction endonuclease cleaved DNA in the same manner as the EcoRI enzyme. However, in contrast with EcoRI, the Sa/I and the BamHI restriction endonucleases appeared to cleave both strands of the DNA duplex almost simultaneously. The function of symmetrical DNA sequences and the conformation of the DNA involved in these DNA--protein interactions are discussed in the light of these observations. The fact that the same reactions were observed on both supercoiled and linear DNA substrates implies that these interactions do not involve the unwinding of the duplex before catalysis.

摘要

以质粒pMB9和噬菌体λ的DNA为底物,研究了EcoRI限制性内切酶的反应。对于环状和线性DNA分子,EcoRI限制性内切酶催化的唯一反应是DNA双链体识别位点一条链内磷酸二酯键的水解。双链体两条链的切割只有在两个独立反应之后才能实现,每个反应都涉及一次单链断裂。该酶对单链断裂的反应性在其识别位点的第一次和第二次切割中是相同的。在超螺旋和线性DNA底物上的作用机制之间未观察到差异。用其他限制性内切酶对质粒pMB9进行了测试。HindIII限制性内切酶与EcoRI酶以相同的方式切割DNA。然而,与EcoRI不同的是,Sa/I和BamHI限制性内切酶似乎几乎同时切割DNA双链体的两条链。根据这些观察结果,讨论了对称DNA序列的功能以及这些DNA-蛋白质相互作用中涉及的DNA构象。在超螺旋和线性DNA底物上观察到相同反应这一事实表明,这些相互作用在催化之前不涉及双链体的解旋。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/db4c/1186633/2602e1c072cb/biochemj00464-0108-a.jpg

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