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利用FraC纳米孔对肽和蛋白质生物标志物进行电渗捕获和离子鉴别。

Electro-osmotic capture and ionic discrimination of peptide and protein biomarkers with FraC nanopores.

作者信息

Huang Gang, Willems Kherim, Soskine Misha, Wloka Carsten, Maglia Giovanni

机构信息

Groningen Biomolecular Sciences & Biotechnology Institute, University of Groningen, 9747 AG, Groningen, The Netherlands.

KU Leuven Department of Chemistry, Celestijnenlaan 200G, 3001, Leuven, Belgium.

出版信息

Nat Commun. 2017 Oct 16;8(1):935. doi: 10.1038/s41467-017-01006-4.

Abstract

Biological nanopores are nanoscale sensors employed for high-throughput, low-cost, and long read-length DNA sequencing applications. The analysis and sequencing of proteins, however, is complicated by their folded structure and non-uniform charge. Here we show that an electro-osmotic flow through Fragaceatoxin C (FraC) nanopores can be engineered to allow the entry of polypeptides at a fixed potential regardless of the charge composition of the polypeptide. We further use the nanopore currents to discriminate peptide and protein biomarkers from 25 kDa down to 1.3 kDa including polypeptides differing by one amino acid. On the road to nanopore proteomics, our findings represent a rationale for amino-acid analysis of folded and unfolded polypeptides with nanopores.Biological nanopore-based protein sequencing and recognition is challenging due to the folded structure or non-uniform charge of peptides. Here the authors show that engineered FraC nanopores can overcome these problems and recognize biomarkers in the form of oligopeptides, polypeptides and folded proteins.

摘要

生物纳米孔是用于高通量、低成本和长读长DNA测序应用的纳米级传感器。然而,蛋白质的分析和测序因其折叠结构和电荷不均一性而变得复杂。在此,我们表明,可以设计通过草莓毒素C(FraC)纳米孔的电渗流,使多肽在固定电位下进入,而不管多肽的电荷组成如何。我们进一步利用纳米孔电流从25 kDa至1.3 kDa区分肽和蛋白质生物标志物,包括相差一个氨基酸的多肽。在通往纳米孔蛋白质组学的道路上,我们的发现为利用纳米孔对折叠和未折叠多肽进行氨基酸分析提供了理论依据。基于生物纳米孔的蛋白质测序和识别由于肽的折叠结构或电荷不均一性而具有挑战性。在此,作者表明,工程化的FraC纳米孔可以克服这些问题,并识别寡肽、多肽和折叠蛋白形式的生物标志物。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/d0d4/5715100/0fc48b1cc923/41467_2017_1006_Fig1_HTML.jpg

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