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嗜热古菌嗜热栖热放线菌DNA聚合酶的特性。Vent DNA聚合酶、稳态动力学、热稳定性、持续合成能力、链置换及核酸外切酶活性。

Characterization of a DNA polymerase from the hyperthermophile archaea Thermococcus litoralis. Vent DNA polymerase, steady state kinetics, thermal stability, processivity, strand displacement, and exonuclease activities.

作者信息

Kong H, Kucera R B, Jack W E

机构信息

New England Biolabs, Inc., Beverly, Massachusetts 01915.

出版信息

J Biol Chem. 1993 Jan 25;268(3):1965-75.

PMID:8420970
Abstract

We have isolated, cloned, and characterized a DNA polymerase from the hyperthermophile archaea Thermococcus litoralis, the Tli DNA polymerase (also referred to as Vent DNA polymerase). The enzyme is extremely thermostable, having a half-life of 8 h at 95 degrees C and about 2 h at 100 degrees C. Pseudo-first-order kinetics at 70 degrees C reveal an extremely low Km for a primed M13mp18 substrate (0.1 nM), coupled with a relatively high Km for dNTPs (50 microM). Accompanying extension rates are on the order of 1000 nucleotides/min. Synthesis by the polymerase is largely distributive, adding an average of 7 nucleotides/initiation event. This distributive synthesis can generate products of at least 10,000 bases. Tli DNA polymerase contains a 3'-->5' exonuclease activity that enhances the fidelity of replication by the enzyme (Mattila, P., Korpela, J., Tenkanen, T. and Pitkanen, K. (1991) Nucleic Acids Res. 19, 4967-4973). A 2-amino acid substitution within the conserved exonuclease domain abolishes both double and single strand-dependent exonuclease activity, without altering kinetic parameters for polymerization on a primed single-stranded template. Strand displacement activity by the mutated and unmutated forms increases with increasing temperature and is enhanced in the exonuclease-deficient form of the enzyme.

摘要

我们从嗜热古菌嗜热栖热菌中分离、克隆并鉴定了一种DNA聚合酶,即Tli DNA聚合酶(也称为Vent DNA聚合酶)。该酶具有极高的热稳定性,在95℃下半衰期为8小时,在100℃下约为2小时。70℃下的伪一级动力学表明,对于带引物的M13mp18底物,其Km极低(0.1 nM),而对于dNTPs,Km相对较高(50 μM)。相应的延伸速率约为1000个核苷酸/分钟。该聚合酶的合成主要是分布性的,每次起始事件平均添加7个核苷酸。这种分布性合成可产生至少10000个碱基的产物。Tli DNA聚合酶具有3'→5'核酸外切酶活性,可提高该酶复制的保真度(Mattila, P., Korpela, J., Tenkanen, T.和Pitkanen, K. (1991) Nucleic Acids Res. 19, 4967 - 4973)。保守核酸外切酶结构域内的2个氨基酸替换消除了双链和单链依赖性核酸外切酶活性,而不改变在带引物的单链模板上聚合的动力学参数。突变型和未突变型的链置换活性随温度升高而增加,且在核酸外切酶缺陷型酶中增强。

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