细菌 RNase HII 和 HIII 的底物特异性受金属可用性的影响。
Substrate Specificity for Bacterial RNases HII and HIII Is Influenced by Metal Availability.
机构信息
Department of Molecular, Cellular, and Developmental Biology, University of Michigan, Ann Arbor, Michigan, USA.
Department of Molecular, Cellular, and Developmental Biology, University of Michigan, Ann Arbor, Michigan, USA
出版信息
J Bacteriol. 2018 Jan 24;200(4). doi: 10.1128/JB.00401-17. Print 2018 Feb 15.
We tested the activities of four predicated RNase H enzymes, including two RNase HI-type enzymes, in addition to RNase HII (RnhB) and RNase HIII (RnhC), on several RNA-DNA hybrid substrates with different divalent metal cations. We found that the two RNase HI-type enzymes, YpdQ and YpeP, failed to show activity on the three substrates tested. RNase HII and RNase HIII cleaved all the substrates tested, although the activity was dependent on the metal made available. We show that RNase HII and RNase HIII are both able to incise 5' to a single ribonucleoside monophosphate (rNMP). We show that RNase HIII incision at a single rNMP occurs most efficiently with Mn, an activity we found to be conserved among other Gram-positive RNase HIII enzymes. Characterization of RNases HII and HIII with metal concentrations in the physiological range showed that RNase HII can cleave at single rNMPs embedded in DNA while RNase HIII is far less effective. Further, using metal concentrations within the physiological range, RNase HIII efficiently cleaved longer RNA-DNA hybrids lacking an RNA-DNA junction, while RNase HII was much less effective. Phenotypic analysis showed that cells with an deletion were sensitive to hydroxyurea (HU). In contrast, cells with an deletion showed wild-type growth in the presence of HU, supporting the hypothesis that RNases HII and HIII have distinct substrate specificities This work demonstrates how metal availability influences the substrate recognition and activity of RNases HII and HIII, providing insight into their functions RNase H represents a class of proteins that cleave RNA-DNA hybrids, helping resolve R-loops and Okazaki fragments, as well as initiating the process of ribonucleotide excision repair (RER). We investigated the activities of four RNase H enzymes and found that only RNases HII and HIII have activity and that their substrate preference is dependent on metal availability. To understand the factors that contribute to RNase HII and RNase HIII substrate preference, we show that in the presence of metal concentrations within the physiological range, RNases HII and HIII have distinct activities on different RNA-DNA hybrids. This work provides insight into how RNases HII and HIII repair the broad range of RNA-DNA hybrids that form in Gram-positive bacteria.
我们测试了四种预测的 RNase H 酶的活性,包括两种 RNase HI 型酶,以及 RNase HII(RnhB)和 RNase HIII(RnhC),在几种不同二价金属阳离子存在的情况下,用几种 RNA-DNA 杂交底物进行测试。我们发现,两种 RNase HI 型酶 YpdQ 和 YpeP 未能在三种测试的底物上显示活性。RNase HII 和 RNase HIII 均能切割所有测试的底物,尽管活性取决于提供的金属。我们表明,RNase HII 和 RNase HIII 都能够在单个核糖核苷酸单磷酸(rNMP)的 5' 处切割。我们表明,在单个 rNMP 处的 RNase HIII 切割最有效地发生在 Mn 中,我们发现这种活性在其他革兰氏阳性 RNase HIII 酶中是保守的。用生理范围内的金属浓度对 RNase HII 和 HIII 进行表征表明,RNase HII 可以切割嵌入 DNA 中的单个 rNMP,而 RNase HIII 的效率则要低得多。此外,在生理范围内的金属浓度下,RNase HIII 有效地切割缺少 RNA-DNA 连接的较长 RNA-DNA 杂交物,而 RNase HII 的效果则差得多。表型分析表明, 缺失的细胞对羟基脲(HU)敏感。相比之下, 缺失的细胞在 HU 存在的情况下表现出野生型生长,这支持了 RNase HII 和 HIII 具有不同的底物特异性的假设。这项工作表明了金属可用性如何影响 RNase HII 和 HIII 的底物识别和活性,为它们的功能提供了深入了解。RNase H 是一类能切割 RNA-DNA 杂交体的蛋白质,有助于解决 R 环和 Okazaki 片段,以及启动核糖核苷酸切除修复(RER)过程。我们研究了四种 RNase H 酶的活性,发现只有 RNase HII 和 HIII 具有活性,并且它们的底物偏好取决于金属可用性。为了了解导致 RNase HII 和 HIII 底物偏好的因素,我们表明,在生理范围内的金属浓度存在下,RNase HII 和 HIII 在不同的 RNA-DNA 杂交物上具有不同的活性。这项工作深入了解了 RNase HII 和 HIII 如何修复革兰氏阳性菌中形成的广泛的 RNA-DNA 杂交物。
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