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渗透剂二 - 肌醇磷酸完整生物合成途径的基因组鉴定及体外重建

Genomic identification and in vitro reconstitution of a complete biosynthetic pathway for the osmolyte di-myo-inositol-phosphate.

作者信息

Rodionov Dmitry A, Kurnasov Oleg V, Stec Boguslaw, Wang Yan, Roberts Mary F, Osterman Andrei L

机构信息

Burnham Institute for Medical Research, 10901 North Torrey Pines Road, La Jolla, CA 92037, USA.

出版信息

Proc Natl Acad Sci U S A. 2007 Mar 13;104(11):4279-84. doi: 10.1073/pnas.0609279104. Epub 2007 Mar 2.

Abstract

Di-myo-inositol 1,1'-phosphate (DIP) is a major osmoprotecting metabolite in a number of hyperthermophilic species of archaea and bacteria. Although the DIP biosynthesis pathway was previously proposed, genes encoding only two of the four required enzymes, inositol-1-phosphate synthase and inositol monophosphatase, were identified. In this study we used a comparative genomic analysis to predict two additional genes of this pathway (termed dipA and dipB) that remained missing. In Thermotoga maritima both candidate genes (in an originally misannotated locus TM1418) form an operon with the inositol-1-phosphate synthase encoding gene (TM1419). A predicted inositol-mono-phosphate cytidylyltransferase activity was directly confirmed for the purified product of T. maritima gene dipA cloned and expressed in Escherichia coli. The entire DIP pathway was reconstituted in E. coli by cloning of the TM1418-TM1419 operon in pBAD expression vector and confirmed to function in the crude lysate. (31)P NMR and MS analysis revealed that DIP synthesis proceeds via a phosphorylated DIP intermediate, P-DIP, which is generated by the dipB-encoded enzyme, now termed P-DIP synthase. This previously unknown intermediate is apparently converted to the final product, DIP, by an inositol monophosphatase-like phosphatase. These findings allowed us to revise the previously proposed DIP pathway. The genomic survey confirmed its presence in the species known to use DIP for osmoprotection. Among several newly identified species with a postulated DIP pathway, Aeropyrum pernix was directly proven to produce this osmolyte.

摘要

二肌醇1,1'-磷酸酯(DIP)是许多嗜热古菌和细菌中的一种主要渗透保护代谢物。尽管先前已提出DIP生物合成途径,但仅鉴定出了四种所需酶中的两种的编码基因,即肌醇-1-磷酸合酶和肌醇单磷酸酶。在本研究中,我们使用比较基因组分析来预测该途径中另外两个缺失的基因(称为dipA和dipB)。在海栖热袍菌中,两个候选基因(位于最初错误注释的基因座TM1418中)与编码肌醇-1-磷酸合酶的基因(TM1419)形成一个操纵子。对在大肠杆菌中克隆和表达的海栖热袍菌基因dipA的纯化产物直接证实了其预测的肌醇单磷酸胞苷转移酶活性。通过将TM1418-TM1419操纵子克隆到pBAD表达载体中,在大肠杆菌中重建了整个DIP途径,并证实在粗裂解物中起作用。(31)P NMR和MS分析表明,DIP合成通过磷酸化的DIP中间体P-DIP进行,P-DIP由dipB编码的酶(现称为P-DIP合酶)产生。这种先前未知的中间体显然被一种肌醇单磷酸酶样磷酸酶转化为最终产物DIP。这些发现使我们能够修订先前提出的DIP途径。基因组调查证实了它在已知使用DIP进行渗透保护的物种中的存在。在几个新鉴定出的具有假定DIP途径的物种中,直接证明了嗜酸热硫化叶菌能产生这种渗透溶质。

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