首页> 外文期刊>Proceedings of the National Academy of Sciences of the United States of America >Genetically encoded short peptide tag for versatile protein labeling by Sfp phosphopantetheinyl transferase
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Genetically encoded short peptide tag for versatile protein labeling by Sfp phosphopantetheinyl transferase

机译:遗传编码的短肽标签,可通过Sfp磷酸泛肽基转移酶进行多功能蛋白质标记

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摘要

An 11-residue peptide with the sequence DSLEFIASKLA was identified from a genomic library of Bacillus subtilis by phage display as an efficient substrate for Sfp phosphopantetheinyl transferase-catalyzed protein labeling by small molecule-CoA conjugates. We name this peptide the "ybbR tag," because part of its sequence is derived from the ybbR ORF in the B. subtilis genome. The site of Sfp-catalyzed ybbR tag labeling was mapped to the underlined Ser residue, and the ybbR tag was found to have a strong tendency for adopting an α-helical conformation in solution. Here we demonstrate that the ybbR tag can be fused to the N or C termini of target proteins or inserted in a flexible loop in the middle of a target protein for site-specific protein labeling by Sfp. The short size of the ybbR tag and its compatibility with various target proteins, the broad substrate specificity of Sfp for labeling the ybbR tag with small-molecule probes of diverse structures, and the high specificity and efficiency of the labeling reaction make Sfp-catalyzed ybbR tag labeling an attractive tool for expanding protein structural and functional diversities by posttranslational modification.
机译:通过噬菌体展示,从枯草芽孢杆菌的基因组文库中鉴定出具有序列DSLEFIASKLA的11个残基的肽,作为通过小分子CoA共轭物标记Sfp磷酸泛肽亚基转移酶催化的蛋白的有效底物。我们将此肽命名为“ ybbR标签”,因为其部分序列来源于枯草芽孢杆菌基因组中的ybbR ORF。 Sfp催化的ybbR标签标记的位点被映射到带下划线的Ser残基,并且发现ybbR标签在溶液中具有采用α-螺旋构象的强烈趋势。在这里,我们证明了ybbR标签可以与靶蛋白的N或C末端融合或插入目标蛋白中间的柔性环中,以通过Sfp标记位点特异性蛋白。 ybbR标签的短尺寸及其与各种靶蛋白的相容性,Sfp用于用各种结构的小分子探针标记ybbR标签的广泛底物特异性,以及标记反应的高特异性和高效率使Sfp催化了ybbR标签标记是通过翻译后修饰扩展蛋白质结构和功能多样性的有吸引力的工具。

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