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利用细菌微区室技术构建无壳酶聚集体以增强大肠杆菌中1,2-丙二醇的生产

Employing bacterial microcompartment technology to engineer a shell-free enzyme-aggregate for enhanced 1,2-propanediol production in Escherichia coli.

作者信息

Lee Matthew J, Brown Ian R, Juodeikis Rokas, Frank Stefanie, Warren Martin J

机构信息

School of Biosciences, University of Kent, Giles Lane, Canterbury, Kent CT2 7NJ, UK.

School of Biosciences, University of Kent, Giles Lane, Canterbury, Kent CT2 7NJ, UK.

出版信息

Metab Eng. 2016 Jul;36:48-56. doi: 10.1016/j.ymben.2016.02.007. Epub 2016 Mar 8.

Abstract

Bacterial microcompartments (BMCs) enhance the breakdown of metabolites such as 1,2-propanediol (1,2-PD) to propionic acid. The encapsulation of proteins within the BMC is mediated by the presence of targeting sequences. In an attempt to redesign the Pdu BMC into a 1,2-PD synthesising factory using glycerol as the starting material we added N-terminal targeting peptides to glycerol dehydrogenase, dihydroxyacetone kinase, methylglyoxal synthase and 1,2-propanediol oxidoreductase to allow their inclusion into an empty BMC. 1,2-PD producing strains containing the fused enzymes exhibit a 245% increase in product formation in comparison to un-tagged enzymes, irrespective of the presence of BMCs. Tagging of enzymes with targeting peptides results in the formation of dense protein aggregates within the cell that are shown by immuno-labelling to contain the vast majority of tagged proteins. It can therefore be concluded that these protein inclusions are metabolically active and facilitate the significant increase in product formation.

摘要

细菌微区室(BMCs)可增强代谢物(如1,2 - 丙二醇(1,2 - PD))向丙酸的分解。BMC内蛋白质的封装由靶向序列介导。为了尝试将Pdu BMC重新设计成以甘油为起始原料的1,2 - PD合成工厂,我们将N端靶向肽添加到甘油脱氢酶、二羟基丙酮激酶、甲基乙二醛合酶和1,2 - 丙二醇氧化还原酶中,以使它们能够被纳入空的BMC中。与未标记的酶相比,含有融合酶的1,2 - PD生产菌株的产物形成增加了245%,无论是否存在BMCs。用靶向肽标记酶会导致细胞内形成致密的蛋白质聚集体,免疫标记显示其中包含绝大多数标记蛋白。因此可以得出结论,这些蛋白质内含物具有代谢活性,并有助于产物形成的显著增加。

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