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Rapid Identification and Enumeration of Saccharomyces cerevisiae Cells in Wine by Real-Time PCR

机译:实时荧光定量PCR快速鉴定和鉴定葡萄酒中的酿酒酵母细胞

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摘要

Despite the beneficial role of Saccharomyces cerevisiae in the food industry for food and beverage production, it is able to cause spoilage in wines. We have developed a real-time PCR method to directly detect and quantify this yeast species in wine samples to provide winemakers with a rapid and sensitive method to detect and prevent wine spoilage. Specific primers were designed for S. cerevisiae using the sequence information obtained from a cloned random amplified polymorphic DNA band that differentiated S. cerevisiae from its sibling species Saccharomyces bayanus, Saccharomyces pastorianus, and Saccharomyces paradoxus. The specificity of the primers was demonstrated for typical wine spoilage yeast species. The method was useful for estimating the level of S. cerevisiae directly in sweet wines and red wines without preenrichment when yeast is present in concentrations as low as 3.8 and 5 CFU per ml. This detection limit is in the same order as that obtained from glucose-peptone-yeast growth medium (GPY). Moreover, it was possible to quantify S. cerevisiae in artificially contaminated samples accurately. Limits for accurate quantification in wine were established, from 3.8 × 105 to 3.8 CFU/ml in sweet wine and from 5 × 106 to 50 CFU/ml in red wine.
机译:尽管酿酒酵母(Saccharomyces cerevisiae)在食品工业中用于食品和饮料生产具有有益作用,但它仍会导致葡萄酒变质。我们已经开发了一种实时PCR方法,可以直接检测和定量葡萄酒样品中的酵母菌种,从而为酿酒师提供一种快速灵敏的方法来检测和防止葡萄酒变质。使用从克隆的随机扩增的多态性DNA带获得的序列信息设计酿酒酵母的特异性引物,该DNA带将酿酒酵母与其同胞物种巴氏酵母,巴氏酿酒酵母和悖酒酵母区分开。证明了引物对典型的葡萄酒腐败酵母菌种的特异性。当酵母的浓度低至每毫升3.8和5 CFU时,该方法可用于直接估算甜葡萄酒和红葡萄酒中的酿酒酵母水平,而无需预先富集。该检测限与从葡萄糖-p-酵母生长培养基(GPY)获得的检测限相同。此外,有可能准确地量化人为污染样品中的酿酒酵母。确定了葡萄酒中准确定量的限度,甜葡萄酒为3.8×105至3.8 CFU / ml,红葡萄酒为5×106至50 CFU / ml。

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