A Highly Conserved Lysine Residue in phi29 DNA Polymerase is Important for Correct Binding of the Templating Nucleotide during Initiation of phi29 DNA Replication.

Truniger V; Lazaro JM; Blanco L; Salas M

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A Highly Conserved Lysine Residue in phi29 DNA Polymerase is Important for Correct Binding of the Templating Nucleotide during Initiation of phi29 DNA Replication.

机译：phi29 DNA聚合酶中高度保守的赖氨酸残基对于phi29 DNA复制启动过程中模板核苷酸的正确结合非常重要。

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DNA polymerases that initiate replication by protein-priming are able to catalyze terminal protein (TP)-primed initiation, the following transition steps and finally DNA-primed elongation. Therefore, their structures must be able to position sequentially both primers, TP and DNA, at a common binding site. For DNA-templated initiation, these DNA polymerases have to bind the origin of replication as template and TP as primer. It is likely that very precise interactions are required to position both TP and templating nucleotide at the polymerization active site. Such a specificity during TP-priming must rely on specific amino acids that must be evolutionarily conserved in this subfamily of DNA polymerases. By site-directed mutagenesis, we have analyzed the functional significance of Lys392 of phi29 DNA polymerase, immediately adjacent to the Kx(3)NSxYG motif, and specifically conserved among protein-primed DNA polymerases. During TP-primed initiation, mutations in this residue did not affect untemplated TP-dAMP formation, indicating that the interaction with the initiating nucleotide and TP were not affected, whereas the template-directed initiation activity was severely inhibited. Both mutant DNA polymerases had a wild-type-like (overall) DNA binding activity. We thus infer that residue Lys392 of phi29 DNA polymerase is important for the correct positioning of the templating nucleotide at the polymerization active site, a critical requirement during template-directed TP-priming at phi29 DNA origins. Consequently, mutation of this residue compromised the fidelity of the initiation reaction, not controlled by the 3'-5' exonuclease activity. During DNA-primed polymerization, the mutant polymerases showed a defect in translocation of the template strand. This translocation problem could be the consequence of a more general defect in the stabilization and positioning of a next templating nucleotide at the polymerization active site, during DNA-primed DNA synthesis. (c) 2002 Elsevier Science Ltd.

机译：通过蛋白质引发引发复制的DNA聚合酶能够催化末端蛋白质（TP）引发的引发，随后的过渡步骤以及最终DNA引发的延伸。因此，它们的结构必须能够将引物TP和DNA顺序放置在一个共同的结合位点。对于DNA模板起始，这些DNA聚合酶必须结合复制起点作为模板，并结合TP作为引物。可能需要非常精确的相互作用才能在聚合活性位点同时定位TP和模板化核苷酸。 TP引发过程中的这种特异性必须依赖于在DNA聚合酶亚家族中必须进化保守的特定氨基酸。通过定点诱变，我们已经分析了phi29 DNA聚合酶的Lys392的功能意义，它紧邻Kx（3）NSxYG基序，并且在蛋白质引发的DNA聚合酶中特别保守。在TP引发的启动过程中，此残基中的突变不影响未模板化TP-dAMP的形成，表明与起始核苷酸和TP的相互作用不受影响，而模板指导的启动活性受到严重抑制。两种突变型DNA聚合酶均具有野生型（整体）DNA结合活性。因此，我们推断，phi29 DNA聚合酶的Lys392残基对于模板核苷酸在聚合活性位点的正确定位很重要，这是在phi29 DNA起源的模板定向TP引发过程中的关键要求。因此，该残基的突变损害了起始反应的保真度，不受3'-5'核酸外切酶活性的控制。在DNA引发的聚合过程中，突变型聚合酶显示模板链易位缺陷。此易位问题可能是在DNA引发的DNA合成过程中，下一个模板核苷酸在聚合活性位点的稳定性和定位中存在更普遍缺陷的结果。（c）2002爱思唯尔科学有限公司。

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《Journal of Molecular Biology》 |2002年第1期|共14页
作者
Truniger V; Lazaro JM; Blanco L; Salas M;
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正文语种 eng
中图分类分子生物学;
关键词
tissue polypeptide specific antigen; DNA; DNA-Directed DNA Polymerase; Nucleotides; 核苷酸类;

机译：tissue polypeptide specific antigen;DNA;DNA-Directed DNA Polymerase;Nucleotides;核苷酸类;

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专利

1. A Highly Conserved Lysine Residue in phi29 DNA Polymerase is Important for Correct Binding of the Templating Nucleotide during Initiation of phi29 DNA Replication. [J] . Truniger V, Lazaro JM, Blanco L, Journal of Molecular Biology . 2002,第1期

机译：phi29 DNA聚合酶中高度保守的赖氨酸残基对于phi29 DNA复制启动过程中模板核苷酸的正确结合非常重要。
2. Two Positively Charged Residues of phi29 DNA Polymerase, Conserved in Protein-primed DNA Polymerases, are Involved in Stabilisation of the Incoming Nucleotide. [J] . Truniger V, Lazaro JM, Salas M Journal of Molecular Biology . 2004,第2期

机译：在蛋白质引发的DNA聚合酶中保守的phi29 DNA聚合酶的两个带正电荷的残基涉及稳定传入的核苷酸。
3. phi29 DNA Polymerase-Terminal Protein Interaction. Involvement of Residues Specifically Conserved Among Protein-primed DNA Polymerases. [J] . Rodriguez I, Lazaro JM, Salas M, Journal of Molecular Biology . 2004,第4期

机译：phi29 DNA聚合酶-末端蛋白相互作用。在蛋白质引发的DNA聚合酶中特别保守的残基的参与。
4. Towards an understanding of protein-protein interaction network hierarchies. Analysis of DnaN (β)-binding peptide motifs in members of protein families interacting with the eubacterial processivity clamp, the β subunit of DNA Polymerase III [C] . Brian P. Dalrymple, Gene Wijffels, Kritaya Kongsuwan, Asia-Pacific Bioinformatics Conference(APBC 2003); 200302; Adelaide(AU) . 2003

机译：对蛋白质-蛋白质相互作用网络层次结构的理解。蛋白质家族成员与DNA聚合酶III的优生过程性钳位相互作用的DnaN（β）结合肽基序分析
5. Single Molecule Studies of Genome Packaging in Bacteriophage Phi29 Reveal Nonequilibrium DNA Dynamics and Continuous Allosteric Regulation of the Packaging Motor Complex [D] . Berndsen, Zachary T. 2015

机译：噬菌体Phi29基因组包装的单分子研究揭示了包装运动复合体的非平衡DNA动力学和连续变构调节。
6. Primer-terminus stabilization at the 3-5 exonuclease active site of phi29 DNA polymerase. Involvement of two amino acid residues highly conserved in proofreading DNA polymerases. [O] . M de Vega, J M Lazaro, M Salas, 1996

机译：phi29 DNA聚合酶3-5核酸外切酶活性位点的引物末端稳定。在校对DNA聚合酶中高度保守的两个氨基酸残基的参与。
7. A positively charged residue of phi 29 DNA polymerase, highly conserved in DNA polymerases from families A and B, is involved in binding the incoming nucleotide [O] . Truniger, Verónica, Lázaro, José M., Esteban, Francisco J., 2002

机译：phi 29 DNA聚合酶的带正电荷的残基在A和B族的DNA聚合酶中高度保守，参与结合进入的核苷酸

A Highly Conserved Lysine Residue in phi29 DNA Polymerase is Important for Correct Binding of the Templating Nucleotide during Initiation of phi29 DNA Replication.

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