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一种用于定量测量溶液中有效蛋白质电荷和单离子结合的微流控平台。

A microfluidic platform for quantitative measurements of effective protein charges and single ion binding in solution.

作者信息

Herling Therese W, Arosio Paolo, Müller Thomas, Linse Sara, Knowles Tuomas P J

机构信息

Department of Chemistry, University of Cambridge, Cambridge, UK.

出版信息

Phys Chem Chem Phys. 2015 May 14;17(18):12161-7. doi: 10.1039/c5cp00746a.

Abstract

The charge state of proteins in solution is a key biophysical parameter that modulates both long and short range macromolecular interactions. However, unlike in the case of many small molecules, the effective charges of complex biomolecules in solution cannot in general be predicted reliably from their chemical structures alone. Here we present an approach for quantifying the effective charges of solvated biomolecules from independent measurements of their electrophoretic mobilities and diffusion coefficients in free solution within a microfluidic device. We illustrate the potential of this approach by determining the effective charges of a charge-ladder family of mutants of the calcium binding protein calbindin D9k in solution under native conditions. Furthermore, we explore ion-binding under native conditions, and demonstrate the ability to detect the chelation of a single calcium ion through the change that ion binding imparts on the effective charge of calbindin D9k. Our findings highlight the difference between the dry sequence charge and the effective charge of proteins in solution, and open up a route towards rapid and quantitative charge measurements in small volumes in the condensed phase.

摘要

溶液中蛋白质的电荷状态是一个关键的生物物理参数,它调节着长程和短程的大分子相互作用。然而,与许多小分子的情况不同,溶液中复杂生物分子的有效电荷通常不能仅从其化学结构可靠地预测出来。在这里,我们提出了一种方法,通过在微流控装置中对其在自由溶液中的电泳迁移率和扩散系数进行独立测量,来量化溶剂化生物分子的有效电荷。我们通过测定天然条件下溶液中钙结合蛋白钙结合蛋白D9k的电荷梯突变体系列的有效电荷,来说明这种方法的潜力。此外,我们探索了天然条件下的离子结合,并证明了通过离子结合对钙结合蛋白D9k有效电荷的影响变化来检测单个钙离子螯合的能力。我们的研究结果突出了蛋白质的干燥序列电荷与溶液中有效电荷之间的差异,并开辟了一条在凝聚相中进行小体积快速定量电荷测量的途径。

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