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FraC nanopores with adjustable diameter identify the mass of opposite-charge peptides with 44 dalton resolution

机译:直径可调的FraC纳米孔可识别分辨率为44道尔顿的反向电荷肽的质量

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摘要

A high throughput single-molecule method for identifying peptides and sequencing proteins based on nanopores could reduce costs and increase speeds of sequencing, allow the fabrication of portable home-diagnostic devices, and permit the characterization of low abundance proteins and heterogeneity in post-translational modifications. Here we engineer the size of Fragaceatoxin C (FraC) biological nanopore to allow the analysis of a wide range of peptide lengths. Ionic blockades through engineered nanopores distinguish a variety of peptides, including two peptides differing only by the substitution of alanine with glutamate. We also find that at pH 3.8 the depth of the peptide current blockades scales with the mass of the peptides irrespectively of the chemical composition of the analyte. Hence, this work shows that FraC nanopores allow direct readout of the mass of single peptide in solution, which is a crucial step towards the developing of a real-time and single-molecule protein sequencing device.
机译:基于纳米孔鉴定肽和蛋白质的高通量单分子方法可以降低成本并提高测序速度,允许制造便携式家庭诊断设备,并可以表征低丰度蛋白质和翻译后修饰中的异质性。在这里,我们设计了Fragaceatoxin C(FraC)生物纳米孔的大小,以允许分析各种长度的肽。通过工程化的纳米孔进行的离子阻断可区分多种肽,包括仅通过谷氨酸取代丙氨酸而不同的两种肽。我们还发现,在pH值为3.8时,肽电流的封锁深度与肽的质量成比例,而与分析物的化学组成无关。因此,这项工作表明,FraC纳米孔可以直接读出溶液中单个肽的质量,这是开发实时单分子蛋白质测序设备的关键步骤。

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