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在酿酒酵母中克隆布鲁塞尔德克酵母乙烯基苯酚还原酶的假定基因。

Cloning the putative gene of vinyl phenol reductase of Dekkera bruxellensis in Saccharomyces cerevisiae.

作者信息

Romano Diego, Valdetara Federica, Zambelli Paolo, Galafassi Silvia, De Vitis Valerio, Molinari Francesco, Compagno Concetta, Foschino Roberto, Vigentini Ileana

机构信息

Department of Food, Environmental and Nutritional Sciences, Università degli Studi di Milano, Italy.

Department of Food, Environmental and Nutritional Sciences, Università degli Studi di Milano, Italy.

出版信息

Food Microbiol. 2017 May;63:92-100. doi: 10.1016/j.fm.2016.11.003. Epub 2016 Nov 3.

DOI:10.1016/j.fm.2016.11.003
PMID:28040186
Abstract

Vinylphenol reductase of Dekkera bruxellensis, the characteristic enzyme liable for "Brett" sensory modification of wine, has been recently recognized to belong to the short chain dehydrogenases/reductases family. Indeed, a preliminary biochemical characterisation has conferred to the purified protein a dual significance acting as superoxide dismutase and as a NADH-dependent reductase. The present study aimed for providing a certain identification of the enzyme by cloning the VPR gene in S. cerevisiae, a species not producing ethyl phenols. Transformed clones of S. cerevisiae resulted capable of expressing a biologically active form of the heterologous protein, proving its role in the conversion of 4-vinyl guaiacol to 4-ethyl guaiacol. A VPR specific protein activity of 9 ± 0.6 mU/mg was found in crude extracts of S. cerevisiae recombinant strain. This result was confirmed in activity trials carried out with the protein purified from transformant cells of S. cerevisiae by a his-tag purification approach; in particular, VPR-enriched fractions showed a specific activity of 1.83 ± 0.03 U/mg at pH 6.0. Furthermore, in agreement with literature, the purified protein behaves like a SOD, with a calculated specific activity of approximatively 3.41 U/mg. The comparative genetic analysis of the partial VPR gene sequences from 17 different D. bruxellesis strains suggested that the observed polymorphism (2.3%) and the allelic heterozygosity state of the gene do not justify the well described strain-dependent character in producing volatile phenols of this species. Actually, no correlation exists between genotype membership of the analysed strains and their capability to release off-flavours. This work adds valuable knowledge to the study of D. bruxellensis wine spoilage and prepare the ground for interesting future industrial applications.

摘要

布鲁塞尔德克酵母的乙烯基苯酚还原酶是导致葡萄酒产生“布雷特”感官变化的特征酶,最近被认定属于短链脱氢酶/还原酶家族。事实上,初步的生化特性分析表明,纯化后的该蛋白具有双重作用,既作为超氧化物歧化酶,又作为NADH依赖的还原酶。本研究旨在通过在不产生乙基苯酚的酿酒酵母中克隆VPR基因来对该酶进行明确鉴定。酿酒酵母的转化克隆能够表达具有生物活性的异源蛋白形式,证明了其在将4-乙烯基愈创木酚转化为4-乙基愈创木酚中的作用。在酿酒酵母重组菌株的粗提物中发现VPR的比蛋白活性为9±0.6 mU/mg。通过His标签纯化方法从酿酒酵母转化细胞中纯化得到的蛋白进行活性试验,证实了这一结果;特别是,富含VPR的组分在pH 6.0时的比活性为1.83±0.03 U/mg。此外,与文献一致,纯化后的蛋白表现出超氧化物歧化酶的特性,计算得出的比活性约为3.41 U/mg。对17个不同的布鲁塞尔德克酵母菌株的部分VPR基因序列进行的比较遗传分析表明,观察到的多态性(2.3%)和该基因的等位基因杂合状态并不能解释该物种在产生挥发性酚类方面所描述的菌株依赖性特征。实际上,分析菌株的基因型与它们释放异味的能力之间不存在相关性。这项工作为布鲁塞尔德克酵母导致葡萄酒变质的研究增添了有价值的知识,并为未来有趣的工业应用奠定了基础。

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