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PCR differentiation of commercial yeast strains using intron splice site primers.

机译:使用内含子剪接位点引物对商业酵母菌株进行PCR分化。

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摘要

The increased use of pure starter cultures in the wine industry has made it necessary to develop a rapid and simple identification system for yeast strains. A method based upon the PCR using oligonucleotide primers that are complementary to intron splice sites has been developed. Since most introns are not essential for gene function, introns have evolved with minimal constraint. By targeting these highly variable sequences, the PCR has proved to be very effective in uncovering polymorphisms in commercial yeast strains. The speed of the method and the ability to analyze many samples in a single day permit the monitoring of specific yeast strains during fermentations. Furthermore, the simplicity of the technique, which does not require the isolation of DNA, makes it accessible to industrial laboratories that have limited molecular expertise and resources.
机译:在葡萄酒工业中越来越多地使用纯发酵剂培养物,因此有必要开发一种快速,简单的酵母菌株鉴定系统。已经开发了基于PCR的方法,该方法使用与内含子剪接位点互补的寡核苷酸引物。由于大多数内含子不是基因功能所必需的,因此内含子已经以最小的限制进化了。通过靶向这些高度可变的序列,PCR被证明在揭示商业酵母菌株中的多态性方面非常有效。该方法的速度和一天之内分析许多样品的能力允许在发酵过程中监测特定的酵母菌株。此外,该技术的简便性(不需要分离DNA)使分子专业知识和资源有限的工业实验室可以使用它。

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