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Fast method for identifying inter- and intra-species Saccharomyces hybrids in extensive genetic improvement programs based on yeast breeding

机译:基于酵母育种的广泛遗传改善计划中鉴定物种间酿酒酵母和物种内糖酵母的快速方法

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摘要

Aims: The present work proposes a two-step molecular strategy to select inter- and intra-species Saccharomyces hybrids obtained by spore-to-spore mating, one of the most used methods for generating improved hybrids from homothallic wine yeasts. Methods and Results: As low spore viability and haplo-selfing are the main causes of failed mating, at first, we used colony screening PCR (csPCR) of discriminative gene markers to select hybrids directly on dissection plate and discard homozygous diploid colonies arisen from one auto-diploidized progenitor. Then, pre-selected candidates were submitted to recursive streaking and conventional PCR in order to discriminate between the hybrids with stable genomic background and the false-positive admixtures of progenitor cells both undergone haplo-selfing. csPCRs of internal transcribed spacer (ITS) 1 or 2, and the subsequent digestion with diagnostic endonucleases HaeIII and RsaI, respectively, were efficient to select six new Saccharomyces cerevisiae × Saccharomyces uvarum hybrids from 64 crosses. Intragenic minisatellite regions in PIR3, HSP150, and DAN4 genes showed high inter-strain size variation detectable by cost-effective agarose gel electrophoresis and were successful to validate six new intra-species S. cerevisiae hybrids from 34 crosses. Conclusions: Both protocols reduce significantly the number of massive DNA extractions, prevent misinterpretations caused by one or both progenitors undergone haplo-selfing, and can be easily implemented in yeast labs without any specific instrumentation. Significance and Impact of the Study: The study provides a method for the marker-assisted selection of several inter- and intra-species yeast hybrids in a cost-effective, rapid and reproducible manner.
机译:目的:本作者提出了一种两步的分子策略,可选择通过孢子孢子交配获得的和物种内糖酵母杂种,其中最多使用的方法是从本质的葡萄酒酵母产生改善的杂种的方法之一。方法和结果:由于低孢子活力和单夹自行度是交配失效的主要原因,首先,我们使用菌落筛选PCR(CSPCR)的鉴别性基因标记物,直接在解剖板上选择杂种,并丢弃一个来自一个的纯合二倍体菌落自动代款祖先。然后,将预选的候选物提交给递归条纹和常规PCR,以区分具有稳定的基因组背景的杂交体和祖细胞的假阳性混合物经过HAPLO自行。内部转录的间隔物(其)1或2的CSPCR分别与诊断内切核酸酶HaeIII和RSAI的后续消化,有效地选择六种新的糖酵母酿酒酵母×Saccharomyces从64次交叉中的血清杂交物。 PiR3,HSP150和DAN4基因中的腺细胞小型舒适岩区域显示出通过成本效益的琼脂糖凝胶电泳检测的高间应变间尺寸变化,并且成功地验证34个十字架的六种新的物种内部酿酒酵母杂交物。结论:两种方案显着降低了大量DNA提取的数量,防止由一种或两种祖先造成的吞噬渗透,经过HAPLO自行,并且可以在没有任何特定仪器的酵母实验室中容易地实施。该研究的意义和影响:该研究提供了一种以成本效益,快速可重复的方式进行了辅助选择几种和内外酵母杂种的方法。

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