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利用固态纳米孔对泛素及泛素链进行直接传感与区分

Direct Sensing and Discrimination among Ubiquitin and Ubiquitin Chains Using Solid-State Nanopores.

作者信息

Nir Iftach, Huttner Diana, Meller Amit

机构信息

Department of Biomedical Engineering, The Technion-Israel Institute of Technology, Haifa, Israel.

Department of Biomedical Engineering, The Technion-Israel Institute of Technology, Haifa, Israel.

出版信息

Biophys J. 2015 May 5;108(9):2340-9. doi: 10.1016/j.bpj.2015.03.025.

Abstract

Nanopore sensing involves an electrophoretic transport of analytes through a nanoscale pore, permitting label-free sensing at the single-molecule level. However, to date, the detection of individual small proteins has been challenging, primarily due to the poor signal/noise ratio that these molecules produce during passage through the pore. Here, we show that fine adjustment of the buffer pH, close to the isoelectric point, can be used to slow down the translocation speed of the analytes, hence permitting sensing and characterization of small globular proteins. Ubiquitin (Ub) is a small protein of 8.5 kDa, which is well conserved in all eukaryotes. Ub conjugates to proteins as a posttranslational modification called ubiquitination. The immense diversity of Ub substrates, as well as the complexity of Ub modification types and the numerous physiological consequences of these modifications, make Ub and Ub chains an interesting and challenging subject of study. The ability to detect Ub and to identify Ub linkage type at the single-molecule level may provide a novel tool for investigation in the Ub field. This is especially adequate because, for most ubiquitinated substrates, Ub modifies only a few molecules in the cell at a given time. Applying our method to the detection of mono- and poly-Ub molecules, we show that we can analyze their characteristics using nanopores. Of particular importance is that two Ub dimers that are equal in molecular weight but differ in 3D structure due to their different linkage types can be readily discriminated. Thus, to our knowledge, our method offers a novel approach for analyzing proteins in unprecedented detail using solid-state nanopores. Specifically, it provides the basis for development of single-molecule sensing of differently ubiquitinated substrates with different biological significance. Finally, our study serves as a proof of concept for approaching nanopore detection of sub-10-kDa proteins and demonstrates the ability of this method to differentiate among native and untethered proteins of the same mass.

摘要

纳米孔传感涉及分析物通过纳米级孔隙的电泳传输,从而实现单分子水平的无标记传感。然而,迄今为止,检测单个小蛋白质一直具有挑战性,主要原因是这些分子在通过孔隙时产生的信噪比很低。在这里,我们表明,将缓冲液pH值微调至接近等电点,可以用来减缓分析物的转运速度,从而实现对小球形蛋白质的传感和表征。泛素(Ub)是一种8.5 kDa的小蛋白质,在所有真核生物中都高度保守。Ub作为一种称为泛素化的翻译后修饰与蛋白质结合。Ub底物的巨大多样性,以及Ub修饰类型的复杂性和这些修饰的众多生理后果,使得Ub和Ub链成为一个有趣且具有挑战性的研究课题。在单分子水平上检测Ub并识别Ub连接类型的能力可能为Ub领域的研究提供一种新工具。这一点尤为适用,因为对于大多数泛素化底物而言,在给定时间内,Ub仅修饰细胞中的少数分子。将我们的方法应用于单泛素和多泛素分子的检测,我们表明可以使用纳米孔分析它们的特性。特别重要的是,两个分子量相等但由于连接类型不同而三维结构不同的Ub二聚体可以很容易地被区分开来。因此,据我们所知,我们的方法提供了一种使用固态纳米孔以前所未有的细节分析蛋白质的新方法。具体而言,它为开发具有不同生物学意义的不同泛素化底物的单分子传感提供了基础。最后,我们的研究为接近10 kDa以下蛋白质的纳米孔检测提供了概念验证,并证明了该方法区分相同质量的天然蛋白质和非束缚蛋白质的能力。

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