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Eukaryotic RNases H1 act processively by interactions through the duplex RNA-binding domain

机译:真核细胞核糖核酸酶H1通过双链体RNA结合域的相互作用进行性作用

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摘要

Ribonucleases H have mostly been implicated in eliminating short RNA primers used for initiation of lagging strand DNA synthesis. Escherichia coli RNase HI cleaves these RNA-DNA hybrids in a distributive manner. We report here that eukaryotic RNases H1 have evolved to be processive enzymes by attaching a duplex RNA-binding domain to the RNase H region. Highly conserved amino acids of the duplex RNA-binding domain are required for processivity and nucleic acid binding, which leads to dimerization of the protein. The need for a processive enzyme underscores the importance in eukaryotic cells of processing long hybrids, most of which remain to be identified. However, long RNA-DNA hybrids formed during immunoglobulin class-switch recombination are potential targets for RNase H1 in the nucleus. In mitochondria, where RNase H1 is essential for DNA formation during embryogenesis, long hybrids may be involved in DNA replication.
机译:核糖核酸H主要与消除用于落后链DNA合成的短RNA引物有关。大肠杆菌RNase HI以分布方式切割这些RNA-DNA杂种。我们在这里报告说,通过将双链体RNA结合结构域附加到RNase H区域,真核RNases H1已经进化为过程性酶。双链RNA结合结构域的高度保守的氨基酸是持续性和核酸结合所必需的,这导致蛋白质的二聚化。对加工酶的需要强调了在加工长杂种的真核细胞中的重要性,其中大多数尚待确定。然而,在免疫球蛋白类别转换重组过程中形成的长RNA-DNA杂种是细胞核中RNase H1的潜在靶标。在线粒体中,RNase H1对于胚胎发生过程中的DNA形成至关重要,而长杂交体可能参与DNA复制。

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