Genome Integrity and Structural Biology Laboratory, NIEHS, NIH, Research Triangle Park, NC 27709, USA.
DNA Repair (Amst). 2020 Sep;93:102910. doi: 10.1016/j.dnarep.2020.102910.
DNA polymerase (dpol) β has served as a model for structural, kinetic, and computational characterization of the DNA synthesis reaction. The laboratory directed by Samuel H. Wilson has utilized a multifunctional approach to analyze the function of this enzyme at the biological, chemical, and molecular levels for nearly 50 years. Over this time, it has become evident that correlating static crystallographic structures of dpol β with solution kinetic measurements is a daunting task. However, aided by computational and spectroscopic approaches, novel and unexpected insights have emerged. While dpols generally insert wrong nucleotides with similar poor efficiencies, their capacity to insert the right nucleotide depends on the identity of the dpol. Accordingly, the ability to choose right from wrong depends on the efficiency of right, rather than wrong, nucleotide insertion. Structures of dpol β in various liganded forms published by the Wilson laboratory, and others, have provided molecular insights into the molecular attributes that hasten correct nucleotide insertion and deter incorrect nucleotide insertion. Computational approaches have bridged the gap between structures of intermediate complexes and provided insights into this basic and essential chemical reaction.
DNA 聚合酶 (dpol) β 一直是研究 DNA 合成反应的结构、动力学和计算特征的模型。塞缪尔·H·威尔逊 (Samuel H. Wilson) 领导的实验室近 50 年来一直采用多功能方法在生物学、化学和分子水平上分析该酶的功能。在这段时间里,很明显将 dpol β 的静态晶体结构与溶液动力学测量相关联是一项艰巨的任务。然而,在计算和光谱学方法的帮助下,出现了一些新颖且出人意料的见解。虽然 dpols 通常以相似的低效率插入错误的核苷酸,但它们插入正确核苷酸的能力取决于 dpol 的身份。因此,正确与错误的选择取决于正确核苷酸插入的效率,而不是错误核苷酸插入的效率。威尔逊实验室和其他实验室发表的 dpol β 在各种配体形式下的结构为正确核苷酸插入的加速和错误核苷酸插入的抑制提供了分子见解。计算方法填补了中间复合物结构之间的空白,并为这种基本和必要的化学反应提供了深入了解。
