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对于 Pseudomonas sp. strain Chol1 菌株利用甾体化合物胆酸盐生长来说,其水合酶和醛脱氢酶基因的基本功能表明侧链去乙酰化的反应步骤为醛裂解反应。

The essential function of genes for a hydratase and an aldehyde dehydrogenase for growth of Pseudomonas sp. strain Chol1 with the steroid compound cholate indicates an aldolytic reaction step for deacetylation of the side chain.

机构信息

University of Münster, Institute of Molecular Microbiology and Biotechnology, Münster, Germany.

出版信息

J Bacteriol. 2013 Aug;195(15):3371-80. doi: 10.1128/JB.00410-13. Epub 2013 May 24.

Abstract

In the bacterial degradation of steroid compounds, the enzymes initiating the breakdown of the steroid rings are well known, while the reactions for degrading steroid side chains attached to C-17 are largely unknown. A recent in vitro analysis with Pseudomonas sp. strain Chol1 has shown that the degradation of the C5 acyl side chain of the C24 steroid compound cholate involves the C22 intermediate 7α,12α-dihydroxy-3-oxopregna-1,4-diene-20S-carbaldehyde (DHOPDCA) with a terminal aldehyde group. In the present study, candidate genes with plausible functions in the formation and degradation of this aldehyde were identified. All deletion mutants were defective in growth with cholate but could transform it into dead-end metabolites. A mutant with a deletion of the shy gene, encoding a putative enoyl coenzyme A (CoA) hydratase, accumulated the C24 steroid (22E)-7α,12α-dihydroxy-3-oxochola-1,4,22-triene-24-oate (DHOCTO). Deletion of the sal gene, formerly annotated as the steroid ketothiolase gene skt, resulted in the accumulation of 7α,12α,22-trihydroxy-3-oxochola-1,4-diene-24-oate (THOCDO). In cell extracts of strain Chol1, THOCDO was converted into DHOPDCA in a coenzyme A- and ATP-dependent reaction. A sad deletion mutant accumulated DHOPDCA, and expression in Escherichia coli revealed that sad encodes an aldehyde dehydrogenase for oxidizing DHOPDCA to the corresponding acid 7α,12α-dihydroxy-3-oxopregna-1,4-diene-20-carboxylate (DHOPDC) with NAD(+) as the electron acceptor. These results clearly show that the degradation of the acyl side chain of cholate proceeds via an aldolytic cleavage of an acetyl residue; they exclude a thiolytic cleavage for this reaction step. Based on these results and on sequence alignments with predicted aldolases from other bacteria, we conclude that the enzyme encoded by sal catalyzes this aldolytic cleavage.

摘要

在类固醇化合物的细菌降解中,起始破坏类固醇环的酶是众所周知的,而附着在 C-17 上的类固醇侧链的降解反应则在很大程度上是未知的。最近,用假单胞菌属 Chol1 进行的体外分析表明,C24 类固醇化合物胆酸盐的 C5 酰基侧链的降解涉及 C22 中间产物 7α,12α-二羟基-3-氧代孕甾-1,4-二烯-20S-醛(DHOPDCA),具有末端醛基。在本研究中,鉴定了在形成和降解该醛中具有合理功能的候选基因。所有缺失突变体在胆酸盐生长中都有缺陷,但可以将其转化为无出路的代谢物。shy 基因缺失突变体,编码一种假定的烯酰辅酶 A(CoA)水合酶,积累了 C24 类固醇(22E)-7α,12α-二羟基-3-氧代胆甾烷-1,4,22-三烯-24-酯(DHOCTO)。以前注释为类固醇酮硫解酶基因 skt 的 sal 基因缺失导致 7α,12α,22-三羟基-3-氧代胆甾烷-1,4-二烯-24-酯(THOCDO)的积累。在 Chol1 菌株的细胞提取物中,THOCDO 在辅酶 A 和 ATP 依赖性反应中转化为 DHOPDCA。sad 缺失突变体积累 DHOPDCA,在大肠杆菌中的表达表明 sad 编码一种醛脱氢酶,用于将 DHOPDCA 氧化为相应的酸 7α,12α-二羟基-3-氧代孕甾烷-1,4-二烯-20-羧酸(DHOPDC),以 NAD(+)作为电子受体。这些结果清楚地表明,胆酸盐的酰基侧链的降解是通过乙酰基残基的醛裂解进行的;它们排除了该反应步骤的硫裂解。基于这些结果以及与其他细菌预测的醛缩酶的序列比对,我们得出结论,sal 编码的酶催化这种醛裂解。

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