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A toolkit for rapid CRISPR-SpCas9 assisted construction of hexose-transport-deficient Saccharomyces cerevisiae strains

机译:用于快速CRISPR-SPCAS9的工具包辅助构建Hexose-Transport缺乏酿酒酵母菌菌株

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摘要

Hexose transporter-deficient yeast strains are valuable testbeds for the study of sugar transport by native and heterologous transporters. In the popular Saccharomyces cerevisiae strain EBY.VW4000, deletion of 21 transporters completely abolished hexose transport. However, repeated use of the LoxP/Cre system in successive deletion rounds also resulted in major chromosomal rearrangements, gene loss and phenotypic changes. In the present study, CRISPR/SpCas9 was used to delete the 21 hexose transporters in an S. cerevisiae strain from the CEN.PK family in only three deletion rounds, using 11 unique guide RNAs. Even upon prolonged cultivation, the resulting strain IMX1812 (CRISPR-Hxt(0)) was unable to consume glucose, while its growth rate on maltose was the same as that of a strain equipped with a full set of hexose transporters. Karyotyping and whole-genome sequencing of the CRISPR-Hxt(0) strain with Illumina and Oxford Nanopore technologies did not reveal chromosomal rearrangements or other unintended mutations besides a few SNPs. This study provides a new, genetically unaltered' hexose transporter-deficient strain and supplies a CRISPR toolkit for removing all hexose transporter genes from most S. cerevisiae laboratory strains in only three transformation rounds.
机译:己糖转运蛋白缺乏酵母菌株是通过天然和异源转运蛋白研究糖类的有价值的试验台。在流行的酿酒酵母菌菌株Eby.vw4000中,删除了21种运输司机完全废除了己糖运输。然而,在连续缺失循环中重复使用LOXP / CRE系统也导致了主要的染色体重排,基因丧失和表型变化。在本研究中,使用11个独特的指南RNA,CrisPr / SPCAS9用于从CEN.PK系列中删除S.Cereiae菌株中的21个六叶草转运蛋白。即使在长时间培养后,所得菌株IMX1812(CRISPR-HXT(0))也无法消耗葡萄糖,而其对麦芽糖的生长速率与配备有全套己糖转运蛋白的菌株的生长速率相同。 Sillumina和牛津纳米孔技术的CRISPR-HXT(0)菌株的核型和全基因组测序没有揭示除了几个SNP之外的染色体重排或其他意外突变。本研究提供了一种新的遗传淘汰的“己糖转运蛋白缺乏菌株,并供应仅在三次转化回合中从大多数S.酿酒岛实验室菌株中除去所有己糖转运蛋白的粘度蛋白。

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