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首页> 外文期刊>ACS applied materials & interfaces >In Situ Monitoring of Membrane Protein Insertion into Block Copolymer Vesicle Membranes and Their Spreading via Potential-Assisted Approach
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In Situ Monitoring of Membrane Protein Insertion into Block Copolymer Vesicle Membranes and Their Spreading via Potential-Assisted Approach

机译:原位监测膜蛋白插入嵌段共聚物囊泡膜及其通过潜在辅助方法的扩散

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摘要

Synthosomes are polymer vesicles with trans membrane proteins incorporated into block copolymer membranes. They have been used for selective transport in or out of the vesicles as well as catalysis inside the compartments. However, both the insertion process of the membrane protein, forming nanopores, and the spreading of the vesicles on planar substrates to form solid-supported biomimetic membranes have been rarely studied yet. Herein, we address these two points and, first, shed light on the real-time monitoring of protein insertion via isothermal titration calorimetry. Second, the spreading process on different solid supports, namely, SiO2, glass, and gold, via different techniques like spin- and dip-coating as well as a completely new approach of potential-assisted spreading on gold surfaces was studied. While inhomogeneous layers occur via traditional methods, our proposed potential-assisted strategy to induce adsorption of positively charged vesicles by applying negative potential on the electrode leads to remarkable vesicle spreading and their further fusion to form more homogeneous planar copolymer films on gold. The polymer vesicles in our study are formed from amphiphilic copolymers poly(2-methyl oxazoline)-block-poly(dimethylsiloxane)-block-poly(2-methyl oxazoline) (PMOXA-b-PDMS-b-PMOXA). Engineered variants of the transmembrane protein ferric hydroxamate uptake protein component A (FhuA), one of the largest beta-barrel channel proteins, are used as model nanopores. The incorporation of FhuA Delta 1-160 is shown to facilitate the vesicle spreading process further. Moreover, high accessibility of cysteine inside the channel was proven by linkage of a fluorescent dye inside the engineered variant FhuA Delta CVFtev and hence preserved functionality of the channels after spreading. The porosity and functionality of the spread synthosomes on the gold plates have been examined by studying the passive ion transport response in the presence of Li+ and ClO4- ions and electrochemical impedance spectroscopy analysis. Our approach to form solid-supported biomimetic membranes via the potential-assisted strategy could be important for the development of new (bio-) sensors and membranes.
机译:合成蛋白是具有掺入嵌段共聚物膜中的反式膜蛋白的聚合物囊泡。它们已被用于在囊泡中或从囊泡中的选择性运输以及隔室内的催化。然而,膜蛋白质,形成纳米孔的插入过程以及在平面基材上的囊泡的展开以形成固体负载的仿菌膜。已经很少研究。在此,我们解决这两点,首先,通过等温滴定热法实时监测蛋白质插入的实时监测。其次,研究了不同固体载体的扩散过程,即SiO 2,玻璃和金,通过不同的技术,如旋涂和浸涂,以及在金表面上的潜在辅助扩散的全新方法。虽然非均匀层通过传统方法发生,但我们所提出的潜在辅助策略通过在电极上施加负电位而导致具有显着的囊泡展开和它们的进一步融合,以形成更均匀的平面共聚物膜在金上致囊泡的吸附。我们研究中的聚合物囊泡由两亲性共聚物聚(2-甲基恶唑啉) - Block-poly(二甲基硅氧烷) - Block-poly(2-甲基氧基)(PMOXA-B-PDMS-B-PMOXA)形成。跨膜蛋白丙烯酸蛋白的工程变体是最大的β-桶沟道蛋白质之一的跨膜蛋白丙烯酸锰丙烯酸酯的羟肟酸蛋白摄取蛋白组分A(FHUA)作为模型纳米孔。掺入FHUA DELTA 1-160的结合,以便进一步促进囊泡传播过程。此外,通过荧光染料在工程变体FHUA DELTA CVFTEV中的荧光染料联系,证明了通道内的半胱氨酸的高可访问性,因此在扩散后的通道的保存功能。通过在Li +和ClO4 - 离子存在下研究被动离子传输反应和电化学阻抗光谱分析,研究了金板上的涂抹合成物的孔隙率和功能。我们通过潜在辅助策略形成固体支持的仿生膜的方法对于开发新(生物)传感器和膜来说可能是重要的。

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