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来自黄色杆菌属菌株Py2的丙酮羧化酶的纯化与特性分析

Purification and characterization of acetone carboxylase from Xanthobacter strain Py2.

作者信息

Sluis M K, Ensign S A

机构信息

Department of Chemistry and Biochemistry, Utah State University, Logan, UT 84322-0300, USA.

出版信息

Proc Natl Acad Sci U S A. 1997 Aug 5;94(16):8456-61. doi: 10.1073/pnas.94.16.8456.

Abstract

Acetone metabolism in the aerobic bacterium Xanthobacter strain Py2 proceeds by a carboxylation reaction forming acetoacetate as the first detectable product. In this study, acetone carboxylase, the enzyme catalyzing this reaction, has been purified to homogeneity and characterized. Acetone carboxylase was comprised of three polypeptides with molecular weights of 85,300, 78,300, and 19,600 arranged in an alpha2beta2gamma2 quaternary structure. The carboxylation of acetone was coupled to the hydrolysis of ATP and formation of 1 mol AMP and 2 mol inorganic phosphate per mol acetoacetate formed. ADP was also formed during the course of acetone consumption, but only accumulated at low, substoichiometric levels ( approximately 10% yield) relative to acetoacetate. Inorganic pyrophosphate could not be detected as an intermediate or product of acetone carboxylation. In the absence of CO2, acetone carboxylase catalyzed the acetone-dependent hydrolysis of ATP to form both ADP and AMP, with ADP accumulating to higher levels than AMP during the course of the assays. Acetone carboxylase did not have inorganic pyrophosphatase activity. Acetone carboxylase exhibited a Vmax for acetone carboxylation of 0.225 micromol acetoacetate formed min-1.mg-1 at 30 degrees C and pH 7.6 and apparent Km values of 7.80 microM (acetone), 122 microM (ATP), and 4. 17 mM (CO2 plus bicarbonate). These studies reveal molecular properties of the first bacterial acetone-metabolizing enzyme to be isolated and suggest a novel mechanism of acetone carboxylation coupled to ATP hydrolysis and AMP and inorganic phosphate formation.

摘要

需氧细菌黄杆菌菌株Py2中的丙酮代谢通过羧化反应进行,形成乙酰乙酸作为第一个可检测到的产物。在本研究中,催化该反应的丙酮羧化酶已被纯化至同质并进行了表征。丙酮羧化酶由分子量分别为85,300、78,300和19,600的三种多肽组成,呈α2β2γ2四级结构。丙酮的羧化与ATP的水解以及每摩尔乙酰乙酸形成1摩尔AMP和2摩尔无机磷酸盐相偶联。在丙酮消耗过程中也会形成ADP,但相对于乙酰乙酸,其仅以低的、亚化学计量水平(约10%产率)积累。未检测到无机焦磷酸作为丙酮羧化的中间体或产物。在没有CO2的情况下,丙酮羧化酶催化依赖于丙酮的ATP水解形成ADP和AMP,在测定过程中ADP积累的水平高于AMP。丙酮羧化酶不具有无机焦磷酸酶活性。丙酮羧化酶在30℃和pH 7.6时对丙酮羧化的Vmax为0.225微摩尔乙酰乙酸形成·分钟-1·毫克-1,表观Km值分别为7.80微摩尔(丙酮)、122微摩尔(ATP)和4.17毫摩尔(CO2加碳酸氢盐)。这些研究揭示了首个被分离的细菌丙酮代谢酶的分子特性,并提出了一种与ATP水解以及AMP和无机磷酸盐形成相偶联的丙酮羧化新机制。

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