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底物与大肠杆菌核糖核酸酶P催化性RNA亚基的多种结合模式。

Multiple binding modes of substrate to the catalytic RNA subunit of RNase P from Escherichia coli.

作者信息

Pomeranz Krummel D A, Altman S

机构信息

Department of Molecular, Cellular, and Developmental Biology, Yale University, New Haven, Connecticut 06511, USA.

出版信息

RNA. 1999 Aug;5(8):1021-33. doi: 10.1017/s1355838299990416.

Abstract

M1 RNA that contained 4'-thiouridine was photochemically cross-linked to different substrates and to a product of the reaction it governs. The locations of the cross-links in these photochemically induced complexes were identified. The cross-links indicated that different substrates share some contacts but have distinct binding modes to M1 RNA. The binding of some substrates also results in a substrate-dependent conformational change in the enzymatic RNA, as evidenced by the appearance of an M1 RNA intramolecular cross-link. The identification of the cross-links between M1 RNA and product indicate that they are shared with only one of the three cross-linked E-S complexes that were identified, an indication of noncompetitive inhibition by the product. We also examined whether the cross-linked complexes between M1 RNA and substrate(s) or product are altered in the presence of the enzyme's protein cofactor (C5 protein) and in the presence of different concentrations of divalent metal ions. C5 protein enhanced the yield of certain M1 RNA-substrate cross-linked complexes for both wild-type M1 RNA and a deletion mutant of M1 RNA (delta[273-281]), but not for the M1 RNA-product complex. High concentrations of Mg2+ increased the yield of all M1 RNA-substrate complexes but not the M1 RNA-product complex.

摘要

含有4'-硫代尿苷的M1 RNA通过光化学方法与不同底物以及它所催化反应的产物交联。确定了这些光化学诱导复合物中交联的位置。交联结果表明,不同底物有一些共同的接触点,但与M1 RNA的结合模式不同。一些底物的结合还导致酶RNA发生底物依赖性构象变化,M1 RNA分子内交联的出现证明了这一点。M1 RNA与产物之间交联的确定表明,它们仅与所鉴定的三种交联E-S复合物之一共享,这表明产物存在非竞争性抑制。我们还研究了在酶的蛋白质辅因子(C5蛋白)存在以及不同浓度二价金属离子存在的情况下,M1 RNA与底物或产物之间的交联复合物是否会发生改变。C5蛋白提高了野生型M1 RNA和M1 RNA缺失突变体(delta[273-281])某些M1 RNA-底物交联复合物的产量,但对M1 RNA-产物复合物没有作用。高浓度的Mg2+提高了所有M1 RNA-底物复合物的产量,但对M1 RNA-产物复合物没有作用。

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