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Mitochondrial intermediate peptidase: expression in Escherichia coli and improvement of its enzymatic activity detection with FRET substrates.

机译:线粒体中间肽酶:在大肠杆菌中的表达及其使用FRET底物的酶活性检测的改进。

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摘要

In the present study, soluble, functionally-active, recombinant human mitochondrial intermediate peptidase (hMIP), a mitochondrial metalloendoprotease, was expressed in a prokaryotic system. The hMIP fusion protein, with a poly-His-tag (6x His), was obtained by cloning the coding region of hMIP cDNA into the pET-28a expression vector, which was then used to transform Escherichia coli BL21 (DE3) pLysS. After isolation and purification of the fusion protein by affinity chromatography using Ni-Sepharose resin, the protein was purified further using ion exchange chromatography with a Hi-trap resource Q column. The recombinant hMIP was characterized by Western blotting using three distinct antibodies, circular dichroism, and enzymatic assays that used the first FRET substrates developed for MIP and a series of protease inhibitors. The successful expression of enzymatically-active hMIP in addition to the FRET substrates will contribute greatly to the determination of substrate specificity of this protease and to the development of specific inhibitors that are essential for a better understanding of the role of this protease in mitochondrial functioning.
机译:在本研究中,可溶的,具有功能活性的重组人线粒体中间肽酶(hMIP),一种线粒体金属内切蛋白酶在原核系统中表达。通过将hMIP cDNA的编码区克隆到pET-28a表达载体中,获得具有多组氨酸标签(6x His)的hMIP融合蛋白,然后将其用于转化大肠杆菌BL21(DE3)pLysS。在通过使用Ni-Sepharose树脂的亲和色谱法分离和纯化融合蛋白之后,使用具有Hi-trap资源Q柱的离子交换色谱法进一步纯化蛋白。重组hMIP的特征是使用三种不同的抗体通过Western印迹,圆二色性和酶法测定来表征,该酶测定法使用了为MIP开发的首个FRET底物和一系列蛋白酶抑制剂。除FRET底物外,酶活性hMIP的成功表达将大大有助于确定该蛋白酶的底物特异性,并有助于开发特异性抑制剂,这些抑制剂对于更好地了解该蛋白酶在线粒体功能中的作用至关重要。

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