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The location of protein S8 and surrounding elements of 16S rRNA in the 70S ribosome from combined use of directed hydroxyl radical probing and X-ray crystallography.

机译:结合使用定向羟基自由基探测和X射线晶体学分析技术,可以确定70S核糖体中蛋白质S8和16S rRNA周围元件的位置。

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摘要

Ribosomal protein S8, which is essential for the assembly of the central domain of 16S rRNA, is one of the most thoroughly studied RNA-binding proteins. To map its surrounding RNA in the ribosome, we carried out directed hydroxyl radical probing of 16S rRNA using Fe(II) tethered to nine different positions on the surface of protein S8 in 70S ribosomes. Hydroxyl radical-induced cleavage was observed near the classical S8-binding site in the 620 stem, and flanking the other S8-footprinted regions of the central domain at the three-helix junction near position 650 and the 825 and 860 stems. In addition, cleavage near the 5' terminus of 16S rRNA, in the 300 region of its 5' domain, and in the 1070 region of its 3'-major domain provide information about the proximity to S8 of RNA elements not directly involved in its binding. These data, along with previous footprinting and crosslinking results, allowed positioning of protein S8 and its surrounding RNA elements in a 7.8-A map of the Thermus thermophilus 70S ribosome. The resulting model is in close agreement with the extensive body of data from previous studies using protein-protein and protein-RNA crosslinking, chemical and enzymatic footprinting, and genetics.
机译:核糖体蛋白S8是16S rRNA中央结构域组装所必需的,是最深入研究的RNA结合蛋白之一。为了在核糖体中定位其周围的RNA,我们使用Fe(II)拴系到70S核糖体中蛋白质S8表面上的9个不同位置,对16S rRNA进行了定向羟基自由基探测。在620茎的经典S8结合位点附近观察到羟基自由基诱导的裂解,并在650茎和825和860茎附近的三螺旋连接处侧接中央结构域的其他S8足迹区域。此外,在其5'结构域的300区域和其3'主要结构域的1070区域中16S rRNA的5'末端附近的切割可提供有关与S8无关的RNA元件的直接相关信息。捆绑。这些数据,以及以前的足迹和交联结果,使得蛋白质S8及其周围的RNA元件可以定位在嗜热菌70S核糖体的7.8-A图中。所得模型与以前使用蛋白质-蛋白质和蛋白质-RNA交联,化学和酶促足迹法以及遗传学进行的研究得出的大量数据非常吻合。

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