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[大鼠肝脏的3'→5'核酸外切酶与复制错误的校正]

[3'-->5'-exonucleases of the rat liver and the correction of replication errors].

作者信息

Beliakova N V, Kleĭner N E, Kravetskaia T P, Legina O K, Naryzhnyĭ S N, Perrino F V, Shevelev I V, Krutiakov V M

出版信息

Izv Akad Nauk SSSR Biol. 1992 Sep-Oct(5):744-52.

PMID:1332991
Abstract

Mammalian nuclear DNA polymerases alpha and beta are lack of the proofreading 3'-->5' exonucleolytic activity. 40 and 50 kDa 3'-->5' exonucleases were isolated from rat liver. The exonucleases were shown to excise mismatched nucleotides from poly[d(A--T)] template 10 and 2 fold faster than matched ones. The addition of either exonuclease to DNA polymerase alpha from rat liver or calf thymus 5-10 times increased the accuracy of reproduction of primed DNA from bacteriophage phi X174 amber 3, values of exonuclease and DNA polymerase activities being approximately equal. The exonuclease activity surpasses the DNA polymerase one by an order of magnitude in chromatin and nuclear membrane. These data, taken together, are indicative of potent proofreading into hepatocytes.

摘要

哺乳动物的核DNA聚合酶α和β缺乏3'→5'核酸外切酶校对活性。从大鼠肝脏中分离出40 kDa和50 kDa的3'→5'核酸外切酶。这些核酸外切酶从聚[d(A-T)]模板中切除错配核苷酸的速度比匹配核苷酸快10倍和2倍。将任何一种核酸外切酶添加到来自大鼠肝脏或小牛胸腺的DNA聚合酶α中,可使噬菌体φX174琥珀3引发的DNA复制准确性提高5-10倍,核酸外切酶和DNA聚合酶活性的值大致相等。在染色质和核膜中,核酸外切酶活性比DNA聚合酶活性高一个数量级。综合这些数据表明,肝细胞中存在强大的校对功能。

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