Arg660Ser mutation in Thermus aquaticus DNA polymerase I suppresses T->C transitions: implication of wobble base pair formation at the nucleotide incorporation step

水热 生物 聚合酶 底漆延伸 DNA聚合酶 碱基对 鸟嘌呤 分子生物学 聚合酶 过程性 核酸外切酶 核苷酸 DNA DNA复制 校对 生物化学 基序列 基因 嗜热菌
作者
Kumi Yoshida
出处
期刊:Nucleic Acids Research [Oxford University Press]
卷期号:29 (20): 4206-4214 被引量:18
标识
DOI:10.1093/nar/29.20.4206
摘要

We examined the replication fidelity of an Arg660Ser (R660S) mutant of Thermus aquaticus DNA polymerase I (Taq pol I). In a forward mutation assay, R660S showed a marked reduction in T→C transitions, one of the most frequent errors made by the wild-type enzyme. Steady-state kinetics showed that R660S discriminates against dGTP incorporation at a template T 13-fold better than the wild-type. R660S was also 3.2-fold less efficient than the wild-type at extending a T:dG mismatch. These results indicate that R660S has enhanced fidelity during incorporation and extension, which reduces its T→C transition frequency. Interestingly, R660S also discriminated correct from incorrect nucleotides at the incorporation step of C:dATP, A:dATP, G:dATP and C:8-OH-dGTP mispairs 28-, 6.0-, 4.1- and 6.8-fold better, respectively, than the wild-type, although it may not always be as accurate as the wild-type at the extension step. A structural model suggests that Arg660 may participate in two interactions that influence fidelity; the guanidinium group of Arg660 might interact with the incoming guanine base at the major groove and it might compete for forming another interaction with the primer terminus. Substituting Arg with Ser may eliminate or alter these interactions and destabilize the closed complex with incorrect substrates. Our data also suggest that T:dGTP and C:dATP base pairs form ‘wobble’ structures at the incorporation step of Taq pol I.

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