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利用聚集诱导发射生物探针原位监测涡旋流介导的蛋白质折叠/去折叠。

In Situ Monitored Vortex Fluidic-Mediated Protein Refolding/Unfolding Using an Aggregation-Induced Emission Bioprobe.

机构信息

Medical Device Research Institute, College of Science and Engineering, Flinders University, Adelaide, SA 5042, Australia.

Flinders Institute for Nanoscale Science and Technology, College of Science and Engineering, Flinders University, Adelaide, SA 5042, Australia.

出版信息

Molecules. 2021 Jul 14;26(14):4273. doi: 10.3390/molecules26144273.

Abstract

Protein folding is important for protein homeostasis/proteostasis in the human body. We have established the ability to manipulate protein unfolding/refolding for β-lactoglobulin using the induced mechanical energy in the thin film microfluidic vortex fluidic device (VFD) with monitoring as such using an aggregation-induced emission luminogen (AIEgen), TPE-MI. When denaturant (guanidine hydrochloride) is present with β-lactoglobulin, the VFD accelerates the denaturation reaction in a controlled way. Conversely, rapid renaturation of the unfolded protein occurs in the VFD in the absence of the denaturant. The novel TPE-MI reacts with exposed cysteine thiol when the protein unfolds, as established with an increase in fluorescence intensity. TPE-MI provides an easy and accurate way to monitor the protein folding, with comparable results established using conventional circular dichroism. The controlled VFD-mediated protein folding coupled with in situ bioprobe AIEgen monitoring is a viable methodology for studying the denaturing of proteins.

摘要

蛋白质折叠对于人体蛋白质的内稳态/稳定性非常重要。我们已经建立了使用薄膜微流控涡旋流控装置(VFD)中的诱导机械能来操纵β-乳球蛋白的蛋白质展开/重折叠的能力,并使用聚集诱导发射发光团(AIEgen)TPE-MI 进行监测。当存在β-乳球蛋白的变性剂(盐酸胍)时,VFD 以可控的方式加速变性反应。相反,在没有变性剂的情况下,未折叠的蛋白质在 VFD 中迅速复性。如荧光强度增加所证实的,当蛋白质展开时,新型 TPE-MI 与暴露的半胱氨酸巯基反应。TPE-MI 提供了一种简单而准确的监测蛋白质折叠的方法,与使用传统圆二色性所建立的结果相当。与原位生物探针 AIEgen 监测相结合的受控 VFD 介导的蛋白质折叠是研究蛋白质变性的可行方法。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/0d05/8306882/e792368cd5b6/molecules-26-04273-g001.jpg

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