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在大肠杆菌中生产人线粒体 ABC 转运蛋白。

Production of a human mitochondrial ABC transporter in E. coli.

机构信息

Department of Molecular Cell Biology, School of Natural Sciences, University of California Merced, 5200 North Lake Rd, Merced, CA, 95343, USA.

Department of Molecular Cell Biology, School of Natural Sciences, University of California Merced, 5200 North Lake Rd, Merced, CA, 95343, USA.

出版信息

Protein Expr Purif. 2021 Feb;178:105778. doi: 10.1016/j.pep.2020.105778. Epub 2020 Oct 15.

Abstract

Membrane proteins play important roles in health and disease. Despite their importance, the study of membrane proteins has been significantly limited by the difficulties inherent to their successful expression, purification, and stabilization once they have been extracted from the cell membrane. In addition, expression of human membrane proteins commonly requires the use of expensive and/or time-consuming eukaryotic systems, hence their successful expression in bacteria will be obviously beneficial for experimental research. Furthermore, since lipids can have critical effects on the activity of membrane proteins and given the composition similarities between the inner mitochondrial membrane and the bacterial plasma membrane, production of mitochondrial membrane proteins in E. coli represents a logical choice. Here, we present a novel protocol to produce a human mitochondrial ATP-Binding Cassette (ABC) transporter in E. coli. The function of the three known human mitochondrial ABC transporters is not fully understood, but X-ray crystallography models of ABCB10 produced in insect cells are available. We have successfully expressed and purified ABCB10 from E. coli. The yield is close to that of another bacterial ABC transporter routinely produced in our laboratory under similar conditions. In addition, we can efficiently reconstitute detergent purified ABCB10 into lipid nanodiscs. Measurements of ATPase activity of ABCB10 produced in E. coli show an ATP hydrolysis rate similar to other human ABC transporters. This novel protocol facilitates the production of this human mitochondrial transporter for biochemical, structural, and functional analysis, and can likely be adjusted for production of other mitochondrial transporters.

摘要

膜蛋白在健康和疾病中发挥着重要作用。尽管它们很重要,但由于从细胞膜中提取后成功表达、纯化和稳定的固有困难,对膜蛋白的研究受到了很大限制。此外,人源膜蛋白的表达通常需要使用昂贵和/或耗时的真核系统,因此在细菌中成功表达将明显有利于实验研究。此外,由于脂质对膜蛋白的活性有重要影响,并且考虑到线粒体内膜和细菌质膜之间的组成相似性,在大肠杆菌中生产线粒体膜蛋白是一个合理的选择。在这里,我们提出了一种在大肠杆菌中生产人线粒体 ATP 结合盒(ABC)转运蛋白的新方案。三种已知的人线粒体 ABC 转运蛋白的功能尚未完全了解,但已可获得在昆虫细胞中生产的 ABCB10 的 X 射线晶体结构模型。我们已经成功地从大肠杆菌中表达和纯化了 ABCB10。产量接近我们在类似条件下在实验室中常规生产的另一种细菌 ABC 转运蛋白。此外,我们可以有效地将去污剂纯化的 ABCB10 重新组装到脂质纳米盘中。用大肠杆菌生产的 ABCB10 的 ATP 酶活性测量显示出与其他人类 ABC 转运蛋白相似的 ATP 水解速率。该新方案促进了这种人源线粒体转运蛋白的生化、结构和功能分析的生产,并且可能可以针对其他线粒体转运蛋白进行调整。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/5389/7709767/d031a8ccfac7/nihms-1641018-f0002.jpg

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