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使用磁悬浮测量蛋白质与凝胶结合配体的结合。

Measuring binding of protein to gel-bound ligands using magnetic levitation.

机构信息

Department of Chemistry & Chemical Biology, Harvard University, Cambridge, Massachusetts 02138, United States.

出版信息

J Am Chem Soc. 2012 Mar 28;134(12):5637-46. doi: 10.1021/ja211788e. Epub 2012 Mar 13.

Abstract

This paper describes the use of magnetic levitation (MagLev) to measure the association of proteins and ligands. The method starts with diamagnetic gel beads that are functionalized covalently with small molecules (putative ligands). Binding of protein to the ligands within the bead causes a change in the density of the bead. When these beads are suspended in a paramagnetic aqueous buffer and placed between the poles of two NbFeB magnets with like poles facing, the changes in the density of the bead on binding of protein result in changes in the levitation height of the bead that can be used to quantify the amount of protein bound. This paper uses a reaction-diffusion model to examine the physical principles that determine the values of rate and equilibrium constants measured by this system, using the well-defined model system of carbonic anhydrase and aryl sulfonamides. By tuning the experimental protocol, the method is capable of quantifying either the concentration of protein in a solution, or the binding affinities of a protein to several resin-bound small molecules simultaneously. Since this method requires no electricity and only a single piece of inexpensive equipment, it may find use in situations where portability and low cost are important, such as in bioanalysis in resource-limited settings, point-of-care diagnosis, veterinary medicine, and plant pathology. It still has several practical disadvantages. Most notably, the method requires relatively long assay times and cannot be applied to large proteins (>70 kDa), including antibodies. The design and synthesis of beads with improved characteristics (e.g., larger pore size) has the potential to resolve these problems.

摘要

本文描述了利用磁悬浮(MagLev)来测量蛋白质和配体的结合。该方法起始于经共价键功能化的顺磁凝胶珠,这些凝胶珠小分子(假定的配体)。当蛋白质与珠内的配体结合时,珠的密度会发生变化。当这些珠子悬浮在顺磁性水性缓冲液中,并放置在两块 NbFeB 磁铁之间,两块磁铁的相同磁极相对时,珠的密度在结合蛋白质时的变化会导致珠的悬浮高度发生变化,从而可以定量结合的蛋白质的量。本文使用反应-扩散模型来检验决定该系统测量的速率和平衡常数的物理原理,使用碳酸酐酶和芳基磺酰胺的明确模型系统。通过调整实验方案,该方法能够定量测量溶液中蛋白质的浓度,或同时测量蛋白质与几种树脂结合的小分子的结合亲和力。由于该方法不需要电力,并且只需要一件便宜的设备,因此它可能在需要便携性和低成本的情况下得到应用,例如在资源有限环境中的生物分析、即时诊断、兽医和植物病理学。它仍然存在几个实际的缺点。最显著的是,该方法需要相对较长的测定时间,并且不能应用于大蛋白(>70 kDa),包括抗体。具有改进特性(例如,更大的孔径)的珠子的设计和合成具有解决这些问题的潜力。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/60f4/3319098/07fc25741f10/nihms363873f1.jpg

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