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Detecting protein-induced folding of the U4 snRNA kink-turn by single-molecule multiparameter FRET measurements

机译:通过单分子多参数FRET测量检测蛋白诱导的U4 snRNA拐弯折叠

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摘要

The kink-turn (k-turn), a new RNA structural motif found in the spliceosome and the ribosome, serves as a specific protein recognition element and as a structural building block. While the structure of the spliceosomal U4 snRNA k-turn/15.5K complex is known from a crystal structure, it is unclear whether the k-turn also exists in this folded conformation in the free U4 snRNA. Thus, we investigated the U4 snRNA k-turn by single-molecule FRET measurements in the absence and presence of the 15.5K protein and its dependence on the Na+ and Mg2+ ion concentration. We show that the unfolded U4 snRNA k-turn introduces a kink of 85 degrees +/- 15 degrees in an RNA double helix. While Na+ and Mg2+ ions induce this more open conformation of the k-turn, binding of the 15.5K protein was found to induce the tightly kinked conformation in the RNA that increases the kink to 52 degrees +/- 15 degrees. By comparison of the measured FRET distances with a computer-modeled structure, we show that this strong kink is due to the k-turn motif adopting its folded conformation. Thus, in the free U4 snRNA, the k-turn exists only in an unfolded conformation, and its folding is induced by binding of the 15.5K protein.
机译:扭折(k-turn)是在剪接体和核糖体中发现的一种新的RNA结构基序,它是一种特定的蛋白质识别元件,也是一种结构构件。虽然从晶体结构已知剪接U4 snRNA k-turn / 15.5K复合物的结构,但尚不清楚k-turn是否也存在于游离U4 snRNA的这种折叠构象中。因此,我们在不存在和存在15.5K蛋白及其对Na +和Mg2 +离子浓度的依赖性的情况下,通过单分子FRET测量研究了U4 snRNA的转角。我们显示,未折叠的U4 snRNA旋转角度会在RNA双螺旋中引入85度+/- 15度的扭结。尽管Na +和Mg2 +离子诱导k转的这种更开放的构象,但发现15.5K蛋白的结合会诱导RNA中的紧密扭结构象,从而使扭结增加至52度+/- 15度。通过将测得的FRET距离与计算机模型结构进行比较,我们显示出这种强烈的扭结是由于k圈主题采用了其折叠构型。因此,在游离的U4 snRNA中,k-turn仅以未折叠的构象存在,并且其折叠是通过15.5K蛋白的结合诱导的。

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