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芯片上蛋白质等电点的无梯度测定

Gradient-free determination of isoelectric points of proteins on chip.

作者信息

Łapińska Urszula, Saar Kadi L, Yates Emma V, Herling Therese W, Müller Thomas, Challa Pavan K, Dobson Christopher M, Knowles Tuomas P J

机构信息

Department of Chemistry, University of Cambridge, Lensfield Road, Cambridge CB2 1EW, UK.

出版信息

Phys Chem Chem Phys. 2017 Aug 30;19(34):23060-23067. doi: 10.1039/c7cp01503h.

Abstract

The isoelectric point (pI) of a protein is a key characteristic that influences its overall electrostatic behaviour. The majority of conventional methods for the determination of the isoelectric point of a molecule rely on the use of spatial gradients in pH, although significant practical challenges are associated with such techniques, notably the difficulty in generating a stable and well controlled pH gradient. Here, we introduce a gradient-free approach, exploiting a microfluidic platform which allows us to perform rapid pH change on chip and probe the electrophoretic mobility of species in a controlled field. In particular, in this approach, the pH of the electrolyte solution is modulated in time rather than in space, as in the case for conventional determinations of the isoelectric point. To demonstrate the general approachability of this platform, we have measured the isoelectric points of representative set of seven proteins, bovine serum albumin, β-lactoglobulin, ribonuclease A, ovalbumin, human transferrin, ubiquitin and myoglobin in microlitre sample volumes. The ability to conduct measurements in free solution thus provides the basis for the rapid determination of isoelectric points of proteins under a wide variety of solution conditions and in small volumes.

摘要

蛋白质的等电点(pI)是影响其整体静电行为的关键特性。大多数测定分子等电点的传统方法依赖于利用pH值的空间梯度,尽管这些技术存在重大实际挑战,尤其是难以产生稳定且可控的pH梯度。在此,我们引入一种无梯度方法,利用微流控平台,使我们能够在芯片上快速改变pH值,并在可控电场中探测物质的电泳迁移率。特别是,在这种方法中,电解质溶液的pH值是随时间而非像传统等电点测定那样随空间进行调制的。为证明该平台的通用性,我们在微升样品体积中测量了一组七种代表性蛋白质的等电点,即牛血清白蛋白、β-乳球蛋白、核糖核酸酶A、卵清蛋白、人转铁蛋白、泛素和肌红蛋白。因此,在自由溶液中进行测量的能力为在各种溶液条件下和小体积中快速测定蛋白质的等电点提供了基础。

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