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Single-molecule spectroscopy of amino acids and peptides by recognition tunnelling

机译:通过识别隧道技术对氨基酸和多肽进行单分子光谱分析

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The human proteome has millions of protein variants due to alternative RNA splicing and post-translational modifications, and variants that are related to diseases are frequently present in minute concentrations. For DNA and RNA, low concentrations can be amplified using the polymerase chain reaction, but there is no such reaction for proteins. Therefore, the development of single-molecule protein sequencing is a critical step in the search for protein biomarkers. Here, we show that single amino acids can be identified by trapping the molecules between two electrodes that are coated with a layer of recognition molecules, then measuring the electron tunnelling current across the junction. A given molecule can bind in more than one way in the junction, and we therefore use a machine-learning algorithm to distinguish between the sets of electronic 'fingerprints' associated with each binding motif. With this recognition tunnelling technique, we are able to identify D and L enantiomers, a methylated amino acid, isobaric isomers and short peptides. The results suggest that direct electronic sequencing of single proteins could be possible by sequentially measuring the products of processive exopeptidase digestion, or by using a molecular motor to pull proteins through a tunnel junction integrated with a nanopore.
机译:由于替代的RNA剪接和翻译后修饰,人类蛋白质组具有数百万个蛋白质变异体,与疾病相关的变异体通常以微量存在。对于DNA和RNA,可以使用聚合酶链式反应扩增低浓度的蛋白质,但对于蛋白质则没有这种反应。因此,单分子蛋白质测序的发展是寻找蛋白质生物标志物的关键步骤。在这里,我们表明可以通过在两个电极之间捕获分子来识别单个氨基酸,该电极涂有一层识别分子,然后测量跨结的电子隧穿电流。一个给定的分子可以在连接处以多种方式结合,因此我们使用机器学习算法来区分与每个结合基序相关的电子“指纹”组。通过这种识别隧穿技术,我们能够鉴定D和L对映异构体,甲基化氨基酸,同量异构体和短肽。结果表明,可以通过顺序测量进行性外肽酶消化的产物,或通过使用分子马达将蛋白质拉出与纳米孔整合的隧道结,来对单个蛋白质进行直接电子测序。

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