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黑曲霉草酰乙酸酶的部分纯化及某些性质

Partial purification and some properties of oxalacetase from Aspergillus niger.

作者信息

Lenz H, Wunderwald P, Eggerer H

出版信息

Eur J Biochem. 1976 May 17;65(1):225-36. doi: 10.1111/j.1432-1033.1976.tb10409.x.

DOI:10.1111/j.1432-1033.1976.tb10409.x
PMID:179820
Abstract
  1. Oxalacetase from Asperigillus niger was found to be an inducible enzyme, the induction being dependent not only on neutralisation of the acidic growth medium but also on the presence of carbonate. An explanation is proposed. 2. Three methods were established for the quantitative determination of oxalacetase activity. These are based on the determination of the product acetate, on the absorbance of oxaloacetate and on coupling the hydrolysis of oxaloacetate to the oxidation of malate by NAD in the presence of malate dehydrogenase. 3. Oxalacetase was purified about 50-fold from cell-free extracts of A. niger and used to determine some of its properties such as kinetic constants. 4. 2S-[U-14C, 3-2H2] Malate in the presence of oxalacetase, NAD and malate dehydrogenase was partially converted to acetate and oxalate. The 3H/14C ratio of the isolated acetate was nearly twice as high as that of the malate used initially. The result demonstrates that the keto form of oxaloacetate, not the enol, is the substrate of the enzyme. 5. Equimolecular mixtures of 2S, 3S-[3-2H1] malate + 2S-[2-2H1] malate (mixture 1) and 2S, 3R-[3-2H1, 3H1] malate + 2S, 3R-[2-2H1, 3-3H1] malate (mixture 2) were prepared from 2S-[3-3H2] malate by incubation with fumarase in normal and tritiated water, respectively. The isolated mixture 1, in the presence of oxalacetase, NAD and malate dehydrogenase was incubated in tritiated water for formation of acetate and oxalate; the isolated mixture 2 was treated likewise in normal water. 6. The mixtures of symmetrically labelled [3H1] acetate and chiral acetates thus produced were isolated and the configuration of the [3H1, 3H1] acetate specimens was determined in the sequence acetate leads to malate leads to fumarate, as usual. The [2H1, 3H1] acetate derived from 2S, 3S-[3-2H1] malate (present in mixture 1( yielded a malate which on incubation with fumarase retained 65.0% of its total tritium content. This chiral acetate, therefore, had the R configuration. The [2H1, 3H1] acetate derived from 2S, 3R-[2-2H1, 3-3H1] malate produced a malate which retained 35% of its total tritium content, and therefore had the S configuration. 7. It was concluded that the detachment of the oxaloyl residue from oxaloacetate and its replacement by a proton proceed with inversion of configuration at the methylene group which becomes methyl during the hydrolysis.
摘要
  1. 发现黑曲霉中的草酰乙酸酶是一种诱导酶,其诱导不仅取决于酸性生长培养基的中和,还取决于碳酸盐的存在。提出了一种解释。2. 建立了三种定量测定草酰乙酸酶活性的方法。这些方法基于对产物乙酸盐的测定、草酰乙酸的吸光度以及在苹果酸脱氢酶存在下将草酰乙酸的水解与苹果酸被NAD氧化相偶联。3. 从黑曲霉的无细胞提取物中纯化草酰乙酸酶约50倍,并用于测定其一些性质,如动力学常数。4. 在草酰乙酸酶、NAD和苹果酸脱氢酶存在下,2S-[U-14C, 3-2H2]苹果酸部分转化为乙酸盐和草酸盐。分离得到的乙酸盐的3H/14C比值几乎是最初使用的苹果酸的两倍。结果表明,草酰乙酸的酮式而非烯醇式是该酶的底物。5. 分别通过在普通水和氚化水中与延胡索酸酶孵育,由2S-[3-3H2]苹果酸制备了2S, 3S-[3-2H1]苹果酸 + 2S-[2-2H1]苹果酸(混合物1)和2S, 3R-[3-2H1, 3H1]苹果酸 + 2S, 3R-[2-2H1, 3-3H1]苹果酸(混合物2)的等分子混合物。将分离得到的混合物1在草酰乙酸酶、NAD和苹果酸脱氢酶存在下于氚化水中孵育以形成乙酸盐和草酸盐;分离得到的混合物2在普通水中同样处理。6. 分离得到由此产生的对称标记的[3H1]乙酸盐和手性乙酸盐混合物,并按照乙酸盐生成苹果酸生成延胡索酸的顺序,像往常一样测定[3H1, 3H1]乙酸盐样品的构型。源自2S, 3S-[3-2H1]苹果酸(存在于混合物1中)的[2H1, 3H1]乙酸盐产生一种苹果酸,该苹果酸在与延胡索酸酶孵育时保留了其总氚含量的65.0%。因此,这种手性乙酸盐具有R构型。源自2S, 3R-[2-2H1, 3-3H1]苹果酸的[2H1, 3H1]乙酸盐产生一种保留了其总氚含量35%的苹果酸,因此具有S构型。7. 得出的结论是,草酰基残基从草酰乙酸上脱离并被质子取代的过程中,在水解过程中变为甲基的亚甲基处发生了构型反转。

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