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The signal recognition particle binds to protein L23 at the peptide exit of the Escherichia coli ribosome.

机译:信号识别颗粒在大肠杆菌核糖体的肽出口处与蛋白L23结合。

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The signal recognition particle (SRP) from Escherichia coli, composed of Ffh protein and 4.5S RNA, mediates membrane targeting of translating ribosomes displaying a signal or signal-anchor sequence. SRP binds at the peptide exit of the large ribosomal subunit. Structural details of the interaction are not known. Here, the position of Ffh or SRP on the ribosome was probed by using site-specific UV-induced crosslinking by p-azidophenacyl bromide (AzP) attached to a number of cysteine residues engineered into surface positions of Ffh. Efficient crosslinking to vacant ribosomes took place from two positions (AzP17 and AzP25) in the N domain of Ffh, both with Ffh and SRP. Both AzP17 and AzP25 were predominantly crosslinked to ribosomal protein L23 that is located at the peptide exit of the 50S subunit. The SRP receptor, FtsY, did not change the crosslink pattern, whereas the presence of a nascent signal peptide on the ribosome resulted in a second crosslink between Ffh(AzP17) and protein L23, indicating that binding to the nascent signal peptide induced a slightly different arrangement of SRP on the ribosome. These results indicate a model of the topographical arrangement of SRP at the peptide exit of the 50S ribosomal subunit.
机译:大肠杆菌的信号识别颗粒(SRP)由Ffh蛋白和4.5S RNA组成,可介导具有信号或信号锚序列的翻译核糖体的膜靶向。 SRP在大核糖体亚基的肽出口结合。相互作用的结构细节未知。在这里,Ffh或SRP在核糖体上的位置是通过使用位点特异性UV诱导的对位叠氮苯甲酰溴(AzP)附着在工程化为Ffh表面位置的半胱氨酸残基上来探测的。 Ffh和SRP均从Ffh N域的两个位置(AzP17和AzP25)高效交联至空核糖体。 AzP17和AzP25都主要与位于50S亚基肽出口处的核糖体蛋白L23交联。 SRP受体FtsY不会改变交联模式,而核糖体上新生信号肽的存在导致Ffh(AzP17)与蛋白L23之间发生第二次交联,表明与新生信号肽的结合引起了稍有不同SRP在核糖体上的排列。这些结果表明了在50S核糖体亚基的肽出口处SRP的拓扑结构的模型。

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