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通过合成蛋白质支架实现合成代谢体的自组装:一步纯化、共固定和底物通道化。

Self-assembly of synthetic metabolons through synthetic protein scaffolds: one-step purification, co-immobilization, and substrate channeling.

作者信息

You Chun, Zhang Y-H Percival

机构信息

Biological Systems Engineering Department, Virginia Tech, Blacksburg, VA 24061, USA.

出版信息

ACS Synth Biol. 2013 Feb 15;2(2):102-10. doi: 10.1021/sb300068g. Epub 2012 Sep 12.

Abstract

One-step purification of a multi-enzyme complex was developed based on a mixture of cell extracts containing three dockerin-containing enzymes and one family 3 cellulose-binding module (CBM3)-containing scaffoldin through high-affinity adsorption on low-cost solid regenerated amorphous cellulose (RAC). The three-enzyme complex, called synthetic metabolon, was self-assembled through the high-affinity interaction between the dockerin in each enzyme and three cohesins in the synthetic scaffoldin. The metabolons were either immobilized on the external surface of RAC or free when the scaffoldin contained an intein between the CBM3 and three cohesins. The immobilized and free metabolons containing triosephosphate isomerase, aldolase, and fructose 1,6-biphosphatase exhibited initial reaction rates 48 and 38 times, respectively, that of the non-complexed three-enzyme mixture at the same enzyme loading. Such reaction rate enhancements indicated strong substrate channeling among synthetic metabolons due to the close spatial organization among cascade enzymes. These results suggested that the construction of synthetic metabolons by using cohesins, dockerins, and cellulose-binding modules from cellulosomes not only decreased protein purification labor and cost for in vitro synthetic biology projects but also accelerated reaction rates by 1 order of magnitude compared to non-complexed enzymes. Synthetic metabolons would be an important biocatalytic module for in vitro and in vivo synthetic biology projects.

摘要

基于含有三种含dockerin酶和一种含3型纤维素结合模块(CBM3)的支架蛋白的细胞提取物混合物,通过在低成本固体再生无定形纤维素(RAC)上的高亲和力吸附,开发了一种多酶复合物的一步纯化方法。这种三酶复合物,称为合成代谢体,通过每种酶中的dockerin与合成支架蛋白中的三种黏附素之间的高亲和力相互作用进行自组装。当支架蛋白在CBM3和三种黏附素之间含有一个内含肽时,代谢体要么固定在RAC的外表面,要么是游离的。含有磷酸丙糖异构酶、醛缩酶和果糖1,6-二磷酸酶的固定化和游离代谢体在相同酶负载量下的初始反应速率分别是非复合三酶混合物的48倍和38倍。这种反应速率的提高表明,由于级联酶之间紧密的空间组织,合成代谢体之间存在强烈的底物通道化。这些结果表明,利用来自纤维小体的黏附素、dockerin和纤维素结合模块构建合成代谢体,不仅减少了体外合成生物学项目中蛋白质纯化的工作量和成本,而且与非复合酶相比,反应速率提高了一个数量级。合成代谢体将成为体外和体内合成生物学项目的重要生物催化模块。

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