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In Vitro Characterization and Concerted Function of Three Core Enzymes of a Glycyl Radical Enzyme - Associated Bacterial Microcompartment

机译:三种糖基酶相关细菌微量分量的三核酶的体外表征和齐节函数

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Many bacteria encode proteinaceous bacterial microcompartments (BMCs) that encapsulate sequential enzymatic reactions of diverse metabolic pathways. Well-characterized BMCs include carboxysomes for CO2-fixation, and propanediol- and ethanolamine-utilizing microcompartments that contain B12-dependent enzymes. Genes required to form BMCs are typically organized in gene clusters, which promoted their distribution across phyla by horizontal gene transfer. Recently, BMCs associated with glycyl radical enzymes (GREs) were discovered; these are widespread and comprise at least three functionally distinct types. Previously, we predicted one type of these GRE-associated microcompartments (GRMs) represents a B12-independent propanediol-utilizing BMC. Here we functionally and structurally characterize enzymes of the GRM of Rhodopseudomonas palustris BisB18 and demonstrate their concerted function in vitro. The GRM signature enzyme, the GRE, is a dedicated 1,2-propanediol dehydratase with a new type of intramolecular encapsulation peptide. It forms a complex with its activating enzyme and, in conjunction with an aldehyde dehydrogenase, converts 1,2-propanediol to propionyl-CoA. Notably, homologous GRMs are also encoded in pathogenic Escherichia coli strains. Our high-resolution crystal structures of the aldehyde dehydrogenase lead to a revised reaction mechanism. The successful in vitro reconstitution of a part of the GRM metabolism provides insights into the metabolic function and steps in the assembly of this BMC.
机译:许多细菌编码蛋白质细菌微量组分(BMC),其包封了不同代谢途径的顺序酶促反应。特征良好的BMC包括用于CO2固定的羧脲和丙二醇胺和乙醇胺利用含有B12依赖性酶的微型组分。形成BMCs所需的基因通常在基因簇中组织,通过水平基因转移在基因簇中组织它们在培养基上促进其分布。最近,发现了与甘糖基酶(GRES)相关的BMC;这些是广泛的并且包括至少三种功能性不同的类型。以前,我们预测了一种类型的这些GRE相关的微型组分(GRMS)代表了一种与B12无关的丙二醇利用BMC。在这里,我们在功能上且结构性地表征了罗多麦莫巴斯巴尔斯特BISB18的GRM的酶,并在体外证明了它们的齐齐欲。 GRM签名酶,GRE,是具有新型分子内包封肽的专用1,2-丙二醇脱水酶。它形成具有其活化酶的复合物,与醛脱氢酶结合,将1,2-丙二醇转化为丙酰基-CoA。值得注意的是,同源grms也在致病大肠杆菌菌株中编码。我们的醛脱氢酶的高分辨率晶体结构导致修订后的反应机制。成功的体外重建于GRM代谢的一部分提供了洞察力,进入该BMC组装中的代谢功能和步骤。

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