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作为蛋白质合成反应容器的多层巨型脂质体结构的定量研究。

Quantitative study of the structure of multilamellar giant liposomes as a container of protein synthesis reaction.

作者信息

Hosoda Kazufumi, Sunami Takeshi, Kazuta Yasuaki, Matsuura Tomoaki, Suzuki Hiroaki, Yomo Tetsuya

机构信息

Department of Bioinformatic Engineering, Graduate School of Information Science and Technology, Osaka University, Yamadaoka 2-1, Suita, Osaka 565-0871, Japan.

出版信息

Langmuir. 2008 Dec 2;24(23):13540-8. doi: 10.1021/la802432f.

Abstract

Liposomes are widely used as cell-sized compartments for encapsulation of biochemical reaction systems to construct model cell systems. However, liposomes are usually diverse in both size and structure, resulting in highly heterogeneous properties as microreactors. Here, we report the development of a strategy to investigate the internal structure of giant multilamellar vesicles (GMLVs) formed by the freeze-dried empty liposomes (FDEL) method as containers of an in vitro transcription/translation system. To evaluate the occurrence of the protein synthesis reaction in GMLVs, we designed a cascade reaction system in which a synthesized enzyme hydrolyzes the fluorescent substrate, and thus the space where the reaction takes place in liposomes becomes fluorescent. We found that only a part of the liposome was reactable and not the entire internal volume, i.e., the hydrolysis reaction took place in only a part of the fractured compartment volumes in GMLVs. Simultaneous measurement of the whole internal volume of the liposomes and the quantity of reaction product of more than 100 000 liposomes using a fluorescence-activated cell sorter (FACS) revealed that the distribution of reactable volume was proportional to the whole internal volume regardless of the liposome size, i.e., the relation between the quantity of whole and reactable volume in GMLV was found to be scale-free. This information would allow us to reduce the geometric parameters of GMLV for quantitative analysis of reaction kinetics in liposomes. The present measurement and analysis method will be an indispensable tool for exploring high-dimensional properties of a model cell system based on giant liposomes.

摘要

脂质体作为细胞大小的隔室被广泛用于封装生化反应系统,以构建模型细胞系统。然而,脂质体的大小和结构通常各不相同,导致其作为微反应器时具有高度异质性。在此,我们报告了一种策略的开发,用于研究通过冻干空脂质体(FDEL)方法形成的巨型多层囊泡(GMLV)的内部结构,该GMLV用作体外转录/翻译系统的容器。为了评估GMLV中蛋白质合成反应的发生情况,我们设计了一种级联反应系统,其中合成的酶水解荧光底物,从而使脂质体中发生反应的空间发出荧光。我们发现只有一部分脂质体可发生反应,而不是整个内部体积,即水解反应仅在GMLV中破裂隔室体积的一部分中发生。使用荧光激活细胞分选仪(FACS)同时测量脂质体的整个内部体积和超过100000个脂质体的反应产物数量,结果表明,无论脂质体大小如何,可反应体积的分布与整个内部体积成正比,即发现GMLV中整个体积与可反应体积之间的关系是无标度的。这些信息将使我们能够减少GMLV的几何参数,以便对脂质体中的反应动力学进行定量分析。目前的测量和分析方法将成为探索基于巨型脂质体的模型细胞系统高维特性的不可或缺的工具。

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