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A high-throughput assay for the comprehensive profiling of DNA ligase fidelity

机译:DNA连接酶保真度综合分析的高通量分析

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摘要

DNA ligases have broad application in molecular biology, from traditional cloning methods to modern synthetic biology and molecular diagnostics protocols. Ligation-based detection of polynucleotide sequences can be achieved by the ligation of probe oligonucleotides when annealed to a complementary target sequence. In order to achieve a high sensitivity and low background, the ligase must efficiently join correctly base-paired substrates, while discriminating against the ligation of substrates containing even one mismatched base pair. In the current study, we report the use of capillary electrophoresis to rapidly generate mismatch fidelity profiles that interrogate all 256 possible base-pair combinations at a ligation junction in a single experiment. Rapid screening of ligase fidelity in a 96-well plate format has allowed the study of ligase fidelity in unprecedented depth. As an example of this new method, herein we report the ligation fidelity of Thermus thermophilus DNA ligase at a range of temperatures, buffer pH and monovalent cation strength. This screen allows the selection of reaction conditions that maximize fidelity without sacrificing activity, while generating a profile of specific mismatches that ligate detectably under each set of conditions.
机译:从传统的克隆方法到现代合成生物学和分子诊断方案,DNA连接酶在分子生物学中有着广泛的应用。当退火至互补靶序列时,可通过探针寡核苷酸的连接来实现多核苷酸序列的基于连接的检测。为了获得高灵敏度和低背景,连接酶必须有效地正确连接碱基配对的底物,同时区分甚至包含一个错配碱基对的底物的连接。在当前的研究中,我们报告了使用毛细管电泳快速生成不匹配的保真度谱图,该图谱在单个实验中在连接结点处询问所有256种可能的碱基对组合。以96孔板的形式快速筛选连接酶保真度使得对连接酶保真度的研究达到了前所未有的深度。作为这种新方法的一个例子,在此我们报道嗜热栖热菌DNA连接酶在一定温度,缓冲液pH和单价阳离子强度范围内的连接保真度。该屏幕允许选择在不牺牲活性的情况下使保真度最大化的反应条件,同时生成可在每组条件下检测到的特定错配图。

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