Simple and rapid protocol for isolation of chromosomal and plasmid DNA from Saccharomyces cerevisiae suitable for polymerase chain reaction analysis

D. Theertha Prasad

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Simple and rapid protocol for isolation of chromosomal and plasmid DNA from Saccharomyces cerevisiae suitable for polymerase chain reaction analysis

机译：简单快捷的方案，用于将染色体和质粒DNA分离，来自适用于聚合酶链反应分析的酿酒酵母

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Majority of the shuttle vectors developed for the metabolic engineering of yeast have low copy number, hence the need to be rescued and optimized in?Escherichia coli?prior to genetic manipulation studies. Methods that are currently available are complicated, contain lot of detergents, time consuming and often yield poor quality plasmid DNA. The present method describes a simple and rapid protocol for isolation of plasmids from yeast using buffer without any detergents. The plasmids isolated by this protocol can be transformed efficiently in?E. coli. Further, we also demonstrate that?Saccharomyces cerevisiae?DNA preparations are best suited for PCR amplification.

机译：为酵母代谢工程开发的大多数穿梭矢量具有低拷贝数，因此需要在遗传操纵研究之前救出和优化。目前可用的方法复杂，含有大量洗涤剂，耗时，通常产生差的质量质粒DNA。本方法描述了一种简单而快速的方案，用于使用没有任何洗涤剂的缓冲液从酵母中分离质粒。该方案分离的质粒可以有效地转化为Δe。大肠杆菌。此外，我们还证明了酿酒酵母酿酒酵母酿酒酵母最适合于PCR扩增。

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《African Journal of Microbiology Research》 |2012年第43期|共5页
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D. Theertha Prasad;
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Saccharomyces cerevisiaeplasmidchromosomal DNAplasmid rescuePCRtransformation;

机译：Saccharomyces酿酒酵母蛋白咪素体DNAPLASMID RescuepcrAnsformation;

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Simple and rapid protocol for isolation of chromosomal and plasmid DNA from Saccharomyces cerevisiae suitable for polymerase chain reaction analysis

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