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φ29 DNA 聚合酶 Lys529 在稳定 DNA 引发末端和聚合部位末端蛋白引发残基中的双重作用。

Dual role of φ29 DNA polymerase Lys529 in stabilisation of the DNA priming-terminus and the terminal protein-priming residue at the polymerisation site.

机构信息

Instituto de Biología Molecular "Eladio Viñuela" (CSIC), Centro de Biología Molecular "Severo Ochoa" (CSIC-UAM), Universidad Autónoma, Cantoblanco, Madrid, Spain.

出版信息

PLoS One. 2013 Sep 4;8(9):e72765. doi: 10.1371/journal.pone.0072765. eCollection 2013.

Abstract

Resolution of the crystallographic structure of φ29 DNA polymerase binary and ternary complexes showed that residue Lys529, located at the C-terminus of the palm subdomain, establishes contacts with the 3' terminal phosphodiester bond. In this paper, site-directed mutants at this Lys residue were used to analyse its functional importance for the synthetic activities of φ29 DNA polymerase, an enzyme that starts linear φ29 DNA replication using a terminal protein (TP) as primer. Our results show that single replacement of φ29 DNA polymerase residue Lys529 by Ala or Glu decreases the stabilisation of the primer-terminus at the polymerisation active site, impairing both the insertion of the incoming nucleotide when DNA and TP are used as primers and the translocation step required for the next incoming nucleotide incorporation. In addition, combination of the DNA polymerase mutants with a TP derivative at residue Glu233, neighbour to the priming residue Ser232, leads us to infer a direct contact between Lys529 and Glu233 for initiation of TP-DNA replication. Altogether, the results are compatible with a sequential binding of φ29 DNA polymerase residue Lys529 with TP and DNA during replication of TP-DNA.

摘要

φ29 DNA 聚合酶二元和三元复合物的晶体结构解析表明,位于手掌亚结构末端的残基赖氨酸 529 与 3'末端磷酸二酯键建立了联系。在本文中,该赖氨酸残基的定点突变用于分析其对 φ29 DNA 聚合酶合成活性的功能重要性,该酶使用末端蛋白 (TP) 作为引物开始线性 φ29 DNA 复制。我们的结果表明,φ29 DNA 聚合酶残基赖氨酸 529 被丙氨酸或谷氨酸单取代会降低聚合活性位点处引物末端的稳定性,从而损害当 DNA 和 TP 用作引物时进入核苷酸的插入以及下一进入核苷酸掺入所需的易位步骤。此外,将 DNA 聚合酶突变体与突变到 Glu233 残基的 TP 衍生物(紧邻引发残基 Ser232)组合使用,使我们推断 Lys529 与 Glu233 之间存在直接接触,以启动 TP-DNA 复制。总的来说,这些结果与 φ29 DNA 聚合酶残基 Lys529 在复制 TP-DNA 期间与 TP 和 DNA 的顺序结合是一致的。

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