Properties and functions of human uracil-DNA glycosylase from the UNG gene

DNA糖基化酶 尿嘧啶DNA糖基化酶 生物 尿嘧啶 DNA修复 AP站点 分子生物学 过程性 基底切除修复术 DNA 生物化学 DNA复制
作者
Hans E. Krokan,Marit Otterlei,Hilde Nilsen,Bodil Kavli,Frank Skorpen,Sonja Andersen,Camilla Furu Skjelbred,Mansour Akbari,Per Arne,Geir Slupphaug
出处
期刊:Progress in Nucleic Acid Research and Molecular Biology 卷期号:: 365-386 被引量:81
标识
DOI:10.1016/s0079-6603(01)68112-1
摘要

The human UNG-gene at position 12q24.1 encodes nuclear (UNG2) and mitochondrial (UNG1) forms of uracil-DNA glycosylase using differently regulated promoters, PA and PB, and alternative splicing to produce two proteins with unique N-terminal sorting sequences. PCNA and RPA co-localize with UNG2 in replication foci and interact with N-terminal sequences in UNG2. Mitochondrial UNG1 is processed to shorter forms by mitochondrial processing peptidase (MPP) and an unidentified mitochondrial protease. The common core catalytic domain in UNG1 and UNG2 contains a conserved DNA binding groove and andight-fitting uracil-binding pocket that binds uracil only when the uracil-containing nucleotide is flipped out. Certain single amino acid substitutions in the active site of the enzyme generate DNA glycosylases that remove either thymine or cystosine. These enzymes induce cytotoxic and mutagenic a basic (AP) sites in the E. coli chromosome and were used to examine biological consequences of AP sites. It has been assumed that a major role of the UNG gene product(s) is to repair mutagenic U:G mispairs caused by cytosine deamination. However, one major role of UNG2 is to remove misincorporated dUMP residues. Thus, knockout mice deficient in Ung activity (Ung-1- mice) have only small increases in GC→AT transition mutations, but Ung-1- cells are deficient in removal of misincorporated dUMP and accumulate approximately 2000 uracil residues for cell. We propose that BEr is important both in the prevention of cancer and for preserving the integrity of germ cell DNA during evolution.
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