The Novo Nordisk Foundation Center for Biosustainability, Technical University of Denmark, Denmark.
Nanion Technologies GmbH, München, Germany.
Bioelectrochemistry. 2024 Oct;159:108732. doi: 10.1016/j.bioelechem.2024.108732. Epub 2024 May 23.
Functional characterization of transporters is impeded by the high cost and technical challenges of current transporter assays. Thus, in this work, we developed a new characterization workflow that combines cell-free protein synthesis (CFPS) and solid supported membrane-based electrophysiology (SSME). For this, membrane protein synthesis was accomplished in a continuous exchange cell-free system (CECF) in the presence of nanodiscs. The resulting transporters expressed in nanodiscs were incorporated into proteoliposomes and assayed in the presence of different substrates using the surface electrogenic event reader. As a proof of concept, we validated this workflow to express and characterize five diverse transporters: the drug/H-coupled antiporters EmrE and SugE, the lactose permease LacY, the Na/H antiporter NhaA from Escherichia coli, and the mitochondrial carrier AAC2 from Saccharomyces cerevisiae. For all transporters kinetic parameters, such as K, I, and pH dependency, were evaluated. This robust and expedite workflow (e.g., can be executed within only five workdays) offers a convenient direct functional assessment of transporter protein activity and has the ability to facilitate applications of transporters in medical and biotechnological research.
功能鉴定转运蛋白受到当前转运体测定方法成本高和技术挑战的阻碍。因此,在这项工作中,我们开发了一种新的鉴定工作流程,将无细胞蛋白合成(CFPS)和基于固体支撑膜的电生理学(SSME)结合起来。为此,在纳米盘的存在下,在连续交换无细胞系统(CECF)中完成膜蛋白的合成。在纳米盘中表达的所得转运蛋白被掺入到质体中,并在存在不同底物的情况下使用表面电致发生事件读取器进行测定。作为概念验证,我们验证了此工作流程,以表达和鉴定五种不同的转运蛋白:药物/H 偶联的反向转运蛋白 EmrE 和 SugE、乳糖通透酶 LacY、来自大肠杆菌的 Na/H 反向转运蛋白 NhaA 和来自酿酒酵母的线粒体载体 AAC2。对所有转运蛋白的动力学参数,如 K、I 和 pH 依赖性进行了评估。这种强大且快速的工作流程(例如,可在短短五天内完成)提供了一种方便的直接转运蛋白活性功能评估方法,并具有促进转运蛋白在医学和生物技术研究中的应用的能力。
