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Human replication protein A can suppress the intrinsic in vitro mutator phenotype of human DNA polymerase λ

机译:人类复制蛋白A可以抑制人类DNA聚合酶λ的固有体外突变体表型

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摘要

DNA polymerase λ (pol λ) is a member of the X family DNA polymerases and is endowed with multiple enzymatic activities. In this work we investigated the in vitro miscoding properties of full-length, human pol λ either in the absence or in the presence of the human auxiliary proteins proliferating cell nuclear antigen (PCNA) and replication protein A (RP-A). Our data suggested that (i) pol λ had an intrinsic ability to create mismatches and to incorporate ribonucleotides at nearly physiological Mn++ and Mg++ concentrations; (ii) the sequence of the template-primer could influence the misincorporation frequency of pol λ; (iii) pol λ preferentially generated G:T and G:G mismatches; (iv) RP-A, but not PCNA, selectively prevented misincorporation of an incorrect nucleotide by pol λ, without affecting correct incorporation and (v) this inhibitory effect required a precise ratio between the concentrations of pol λ and RP-A. Possible physiological implications of these findings for the in vivo fidelity of pol λ are discussed.
机译:DNA聚合酶λ(polλ)是X家族DNA聚合酶的成员,并具有多种酶活性。在这项工作中,我们调查了在不存在或存在人类辅助蛋白的情况下,全长人polλ在体外是否存在误编码特性,这些辅助蛋白会增殖细胞核抗原(PCNA)和复制蛋白A(RP-A)。我们的数据表明:(i)polλ具有产生错配并以接近生理Mn ++ 和Mg ++ 的浓度掺入核糖核苷酸的内在能力; (ii)模板引物的序列可能影响polλ的错误掺入频率; (iii)polλ优先产生G:T和G:G不匹配; (iv)RP-A,而不是PCNA,有选择地防止了polλ误掺入不正确的核苷酸,而又不影响正确的掺入;并且(v)这种抑制作用需要polλ和RP-A的浓度之间具有精确的比例。讨论了这些发现对polλ体内保真度的可能的生理意义。

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