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首页> 外文期刊>Journal of Biotechnology >Functional display of family 11 endoxylanases on the surface of phage M13
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Functional display of family 11 endoxylanases on the surface of phage M13

机译:在噬菌体M13表面上功能性显示11族内切木聚糖酶

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摘要

Two family 11 endoxylanases (EC 3.2.1.8) were functionally displayed on the surface of bacteriophage M13. The genes encoding endo-1,4-xylanase I from Aspergillus niger (ExlA) and endo-1,4-xylanase A from Bacillus subtilis (XynA) were fused to the gene encoding the minor coat protein g3p in phagemid vector pHOS31. Phage rescue resulted in functional monovalent display of the enzymes as was demonstrated by three independent tests. Firstly, purified recombinant phage particles showed a clear hydrolytic activity in an activity assay based on insoluble, chromagenic arabinoxylan substrate. Secondly, specific binding of endoxylanase displaying phages to immobilized endoxylanase inhibitors was demonstrated by interaction ELISA. Finally, two rounds of selection and amplification in a biopanning procedure against immobilized endoxylanase inhibitor were performed. Phages displaying endoxylanases were strongly enriched from background phages displaying unrelated proteins. These results open perspectives to use phage display for analysing protein-protein interactions at the interface between endoxylanases and their inhibitors. In addition, this technology should enable engineering of endoxylanases into novel variants with altered binding properties towards endoxylanase inhibitors.
机译:在噬菌体M13的表面上功能性地展示了两个11族内切木聚糖酶(EC 3.2.1.8)。将来自黑曲霉(ExlA)的编码内切1,4-木聚糖酶I的基因和枯草芽孢杆菌(XynA)的编码内切1,4-木聚糖酶A的基因与噬菌粒载体pHOS31中编码次要外壳蛋白g3p的基因融合。噬菌体抢救导致了酶的功能性单价展示,如三个独立的测试所示。首先,纯化的重组噬菌体颗粒在基于不溶性发色的阿拉伯木聚糖底物的活性测定中显示出明显的水解活性。其次,通过相互作用ELISA证明了展示内切木聚糖酶的噬菌体与固定化内切木聚糖酶抑制剂的特异性结合。最后,在针对固定化内切木聚糖酶抑制剂的生物淘选程序中进行了两轮选择和扩增。展示内切木聚糖酶的噬菌体从展示无关蛋白的背景噬菌体中大量富集。这些结果为使用噬菌体展示分析内切木聚糖酶及其抑制剂之间的界面处的蛋白质相互作用提供了广阔的前景。另外,该技术应能够将内切木聚糖酶工程化为具有对内切木聚糖酶抑制剂改变的结合特性的新变体。

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