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编码前克拉维酸脒水解酶基因的鉴定、克隆、测序、过表达及在克拉维酸生物合成中蛋白质功能的表征

Identification, cloning, sequencing, and overexpression of the gene encoding proclavaminate amidino hydrolase and characterization of protein function in clavulanic acid biosynthesis.

作者信息

Wu T K, Busby R W, Houston T A, McIlwaine D B, Egan L A, Townsend C A

机构信息

Department of Chemistry, Johns Hopkins University, Baltimore, Maryland 21218, USA.

出版信息

J Bacteriol. 1995 Jul;177(13):3714-20. doi: 10.1128/jb.177.13.3714-3720.1995.

Abstract

Proclavaminate amidino hydrolase (PAH) catalyzes the reaction of guanidinoproclavaminic acid to proclavaminic acid and urea, a central step in the biosynthesis of the beta-lactamase inhibitor clavulanic acid. The gene encoding this enzyme (pah) was tentatively identified within the clavulanic acid biosynthetic cluster in Streptomyces clavuligerus by translation to a protein of the correct molecular mass (33 kDa) and appreciable sequence homology to agmatine ureohydrolase (M.B.W. Szumanski and S.M. Boyle, J. Bacteriol. 172:538-547, 1990) and several arginases, a correlation similarly recognized by Aidoo et al. (K. A. Aidoo, A. Wong, D. C. Alexander, R. A. R. Rittammer, and S. E. Jensen, Gene 147:41-46, 1994). Overexpression of the putative open reading frame as a 76-kDa fusion to the maltose-binding protein gave a protein having the catalytic activity sought. Cleavage of this protein with factor Xa gave PAH whose N terminus was slightly modified by the addition of four amino acids but exhibited unchanged substrate specificity and kinetic properties. Directly downstream of pah lies the gene encoding clavaminate synthase 2, an enzyme that carries out three distinct oxidative transformations in the in vivo formation of clavulanic acid. After the first of these oxidations, however, no further reaction was found to occur in vitro without the intervention of PAH. We have demonstrated that concurrent use of recombinant clavaminate synthase 2 and PAH results in the successful conversion of deoxyguanidinoproclavaminic acid to clavaminic acid, a four-step transformation. PAH has a divalent metal requirement, pH activity profile, and kinetic properties similar to those of other proteins of the broader arginase class.

摘要

前棒酸脒水解酶(PAH)催化胍基前棒酸转化为前棒酸和尿素的反应,这是β-内酰胺酶抑制剂克拉维酸生物合成中的关键步骤。通过翻译出正确分子量(33 kDa)的蛋白质以及与胍丁胺尿素水解酶(M.B.W. 苏曼斯基和S.M. 博伊尔,《细菌学杂志》172:538 - 547,1990年)和几种精氨酸酶有明显的序列同源性,初步确定了编码该酶的基因(pah)位于棒状链霉菌克拉维酸生物合成簇中,艾杜等人也同样认识到了这种相关性(K.A. 艾杜、A. 王、D.C. 亚历山大、R.A.R. 里塔默和S.E. 詹森,《基因》147:41 - 46,1994年)。将推定的开放阅读框作为与麦芽糖结合蛋白的76 kDa融合蛋白进行过表达,得到了具有所需催化活性的蛋白质。用因子Xa切割该蛋白质得到PAH,其N端因添加了四个氨基酸而略有修饰,但底物特异性和动力学性质未变。pah的直接下游是编码棒酸合酶2的基因,该酶在克拉维酸的体内形成过程中进行三种不同的氧化转化。然而,在这些氧化反应的第一步之后,如果没有PAH的干预,在体外未发现进一步的反应。我们已经证明,同时使用重组棒酸合酶2和PAH可成功地将脱氧胍基前棒酸转化为克拉维酸,这是一个四步转化过程。PAH对二价金属有需求,其pH活性曲线和动力学性质与更广泛的精氨酸酶类中的其他蛋白质相似。

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