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光激活的连接子纳米孔在合成细胞中的组装。

Light-Activated Assembly of Connexon Nanopores in Synthetic Cells.

机构信息

McKetta Department of Chemical Engineering, University of Texas at Austin, Austin, Texas 78712, United States.

Department of Chemistry, University of Texas at Austin, Austin, Texas 78712, United States.

出版信息

J Am Chem Soc. 2023 Feb 15;145(6):3561-3568. doi: 10.1021/jacs.2c12491. Epub 2023 Feb 1.

Abstract

During developmental processes and wound healing, activation of living cells occurs with spatiotemporal precision and leads to rapid release of soluble molecular signals, allowing communication and coordination between neighbors. Nonliving systems capable of similar responsive release hold great promise for information transfer in materials and site-specific drug delivery. One nonliving system that offers a tunable platform for programming release is synthetic cells. Encased in a lipid bilayer structure, synthetic cells can be outfitted with molecular conduits that span the bilayer and lead to material exchange. While previous work expressing membrane pore proteins in synthetic cells demonstrated content exchange, user-defined control over release has remained elusive. In mammalian cells, connexon nanopore structures drive content release and have garnered significant interest since they can direct material exchange through intercellular contacts. Here, we focus on connexon nanopores and present activated release of material from synthetic cells in a light-sensitive fashion. To do this, we re-engineer connexon nanopores to assemble after post-translational processing by a protease. By encapsulating proteases in light-sensitive liposomes, we show that assembly of nanopores can be triggered by illumination, resulting in rapid release of molecules encapsulated within synthetic cells. Controlling connexon nanopore activity provides an opportunity for initiating communication with extracellular signals and for transferring molecular agents to the cytoplasm of living cells in a rapid, light-guided manner.

摘要

在发育过程和伤口愈合过程中,活细胞的激活具有时空精确性,并导致可溶性分子信号的快速释放,从而允许相邻细胞之间进行通讯和协调。能够进行类似响应性释放的非生命系统在信息传递和靶向药物输送方面具有巨大的应用前景。一种提供可编程释放平台的非生命系统是合成细胞。合成细胞被包裹在脂质双层结构中,可以配备跨越双层的分子通道,从而实现物质交换。虽然以前在合成细胞中表达膜孔蛋白的工作已经证明了物质交换,但对释放的用户定义控制仍然难以捉摸。在哺乳动物细胞中,连接子纳米孔结构驱动物质释放,并且自它们可以通过细胞间接触来指导物质交换以来,已经引起了人们的极大兴趣。在这里,我们专注于连接子纳米孔,并以光敏感的方式展示了合成细胞中物质的激活释放。为此,我们重新设计了连接子纳米孔,使其在蛋白酶的翻译后加工后进行组装。通过将蛋白酶封装在光敏感的脂质体中,我们表明纳米孔的组装可以通过光照触发,从而导致封装在合成细胞内的分子快速释放。控制连接子纳米孔的活性为与细胞外信号进行通信以及以快速、光控的方式将分子试剂转移到活细胞的细胞质提供了机会。

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