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与大肠杆菌单链DNA结合蛋白交联的ATP可被引发酶的催化中心用作在噬菌体G4oric模板上合成引物RNA的起始核苷酸。

ATP cross-linked to Escherichia coli single-strand DNA-binding protein can be utilized by the catalytic center of primase as initiating nucleotide for primer RNA synthesis on phage G4oric template.

作者信息

Godson G N, Mustaev A A, Sun W

机构信息

Biochemistry Department, New York University Medical Center 10016, USA.

出版信息

Biochemistry. 1998 Mar 17;37(11):3810-7. doi: 10.1021/bi972455f.

Abstract

We report a new observation of the role of Escherichia coli single-strand DNA binding protein (SSB) in synthesis of primer RNA (pRNA) catalyzed by.E.coli primase on the SSB-coated phage G4oric template. Using a set of ATP priming substrates with reactive groups attached to the 5' gamma-phosphate on different length "arms", we have demonstrated that, in the primase/SSB/G4oric pRNA synthesis complex, ATP cross-linked to both primase and SSB could be equally utilized as initiating nucleotide for pRNA synthesis. The distance between SSB surface and alpha-phosphorus of the priming substrate was estimated to be less than 7 A. ATP cross-linked to primase and SSB can be further elongated in the presence of other NTPs, giving almost identical patterns of covalently attached pRNAs of up to 12 nucleotides in length. The regions of primase and SSB with cross-linked ATP that can be used for pRNA synthesis are, therefore, arranged in a similar way relative to the active center of pRNA synthesis. The pRNA covalently linked to SSB was localized, mapping between Met48 and Trp88. This observation raises the possibility that SSB may play an active role in the initiation of pRNA synthesis in this system.

摘要

我们报道了一项关于大肠杆菌单链DNA结合蛋白(SSB)在大肠杆菌引发酶催化的引物RNA(pRNA)合成中作用的新观察结果,该合成反应发生在包被有SSB的噬菌体G4oric模板上。使用一组在不同长度“臂”的5'γ-磷酸上连接有反应基团的ATP引发底物,我们证明,在引发酶/SSB/G4oric pRNA合成复合物中,与引发酶和SSB都交联的ATP可同样用作pRNA合成的起始核苷酸。据估计,SSB表面与引发底物α-磷之间的距离小于7埃。在其他NTP存在的情况下,与引发酶和SSB交联的ATP可进一步延长,产生长度达12个核苷酸的共价连接pRNA的几乎相同模式。因此,与可用于pRNA合成的交联ATP的引发酶和SSB区域相对于pRNA合成活性中心以相似方式排列。与SSB共价连接的pRNA被定位,位于Met48和Trp88之间。这一观察结果增加了SSB可能在该系统中pRNA合成起始中发挥积极作用的可能性。

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