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首页> 外文期刊>Protein engineering design & selection: PEDS >A system based on specific protein-RNA interactions for analysis of target protein-protein interactions in vitro: successful selection of membrane-bound Bak-Bcl-x(L) proteins in vitro
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A system based on specific protein-RNA interactions for analysis of target protein-protein interactions in vitro: successful selection of membrane-bound Bak-Bcl-x(L) proteins in vitro

机译:一个基于特定蛋白质-RNA相互作用的系统,用于体外分析目标蛋白质-蛋白质的相互作用:体外成功选择膜结合的Bak-Bcl-x(L)蛋白质

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摘要

Ribosome display systems are very effective and powerful tools for in vitro screening of transcribed mRNAs that encode proteins (or peptides) with specific (known or unknown) functions. We have modified such a system by exploiting the interaction between a tandemly fused MS2 coat-protein (MSp) dimer and the RNA sequence of the corresponding specific binding motif, C-variant (or Cv). We placed the MSp dimer at the N-terminus of a nascent protein and the Cv binding motif was attached to the 5' end of the protein's mRNA. This configuration enhanced the stability of the ribosome-mRNA complex. We demonstrate here that this improved ribosome display system provides an effective method for identifying the gene for a protein that binds to a protein of interest. We visualized the formation of polysome complexes in this advanced polysome display by atomic force microscopy (AFM) and found that the AFM images of polysomes in our system were different from those observed in the case of conventional ribosome display systems. Our results suggest that our technology might usefully complement yeast two-hybrid assays.
机译:核糖体展示系统是用于体外筛选编码具有特定(已知或未知)功能的蛋白质(或肽)的转录的mRNA的非常有效且功能强大的工具。我们已经通过利用串联融合的MS2外壳蛋白(MSp)二聚体和相应的特异性结合基序C变体(或Cv)的RNA序列之间的相互作用来修饰这种系统。我们将MSp二聚体置于新生蛋白质的N末端,并将Cv结合基序连接到蛋白质mRNA的5'末端。这种配置增强了核糖体-mRNA复合物的稳定性。我们在这里证明,这种改进的核糖体展示系统为鉴定与目的蛋白质结合的蛋白质的基因提供了一种有效的方法。我们通过原子力显微镜(AFM)可视化了这种高级多核糖体展示物中多核糖体复合物的形成,发现我们系统中多核糖体的AFM图像与常规核糖体展示系统中观察到的图像不同。我们的结果表明,我们的技术可能会有用地补充酵母双杂交检测方法。

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