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确定DNA聚合酶核苷酸掺入的稳态动力学。

Determining Steady-State Kinetics of DNA Polymerase Nucleotide Incorporation.

作者信息

Gahlon Hailey L, Sturla Shana J

机构信息

Department of Health Sciences and Technology, ETH Zurich, Zurich, Switzerland.

出版信息

Methods Mol Biol. 2019;1973:299-311. doi: 10.1007/978-1-4939-9216-4_19.

Abstract

Polymerase enzymes catalyze the replication of DNA by incorporating deoxynucleoside monophosphates (dNMPs) into a primer strand in a 5' to 3' direction. Monitoring kinetic aspects of this catalytic process provides mechanistic information regarding polymerase-mediated DNA synthesis and the influences of nucleobase structure. For example, a range of polymerases have different capacities to synthesize DNA depending on the structure of the inserted dNMP (natural or synthetic) and also depending on the templating DNA base (modified vs. unmodified). Under steady-state conditions, relative rates depend on the deoxynucleoside triphosphate (dNTP) residence times in the ternary (polymerase-DNA-dNTP) complex. This chapter describes a method to measure steady-state incorporation efficiencies by which polymerase enzymes insert dNMPs into primer-template (P/T) oligonucleotides. The method described involves the use of a primer oligonucleotide 5' radiolabeled with [γ-P]ATP. Significant established applications of this experiment include studies regarding mechanisms of nucleotide misincorporation as a basis of chemically induced DNA mutation. Further, it can provide information important in various contexts ranging from biophysical to medical-based studies.

摘要

聚合酶通过将脱氧核苷单磷酸(dNMPs)以5'至3'方向掺入引物链来催化DNA复制。监测这一催化过程的动力学方面可提供有关聚合酶介导的DNA合成以及核碱基结构影响的机制信息。例如,一系列聚合酶根据插入的dNMP(天然或合成)的结构以及模板DNA碱基(修饰与未修饰)的不同,具有不同的DNA合成能力。在稳态条件下,相对速率取决于三磷酸脱氧核苷(dNTP)在三元(聚合酶-DNA-dNTP)复合物中的停留时间。本章描述了一种测量稳态掺入效率的方法,通过该方法聚合酶将dNMPs插入引物-模板(P/T)寡核苷酸中。所描述的方法涉及使用用[γ-P]ATP进行5'放射性标记的引物寡核苷酸。该实验的重要既定应用包括关于核苷酸错掺入机制的研究,作为化学诱导DNA突变的基础。此外,它可以在从生物物理到医学研究等各种背景下提供重要信息。

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