| 解脂亚罗酵母P12单倍体的制备 |
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| 引用本文: | 屈亦潇,张雅欣,张天,郝顺水,张昕炜,郭蓓. 解脂亚罗酵母P12单倍体的制备[J]. 微生物学通报, 2021, 48(5): 1674-1680 |
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| 作者姓名: | 屈亦潇 张雅欣 张天 郝顺水 张昕炜 郭蓓 |
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| 作者单位: | 1 北京农学院生物与资源环境学院 北京 102206;1 北京农学院生物与资源环境学院 北京 102206;2 农业农村部华北都市农业重点实验室 北京 102206 |
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| 基金项目: | 山东省重大科技创新工程项目(2019JZZY011005) |
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| 摘 要: | [背景]目前解脂亚罗酵母在实验研究和工业生产方面的应用越来越广泛,但相较于常规酵母而言,解脂亚罗酵母缺乏简便有效的遗传转化体系,致使其在基因表达调控方面存在较大困难.同时,酵母的染色体倍性也会对基因敲除效果产生影响,选择单倍体细胞作为功能基因改造的受体可以避免等位基因之间相互作用的影响,解决多倍体细胞基因敲除不完全的问...
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| 关 键 词: | 解脂亚罗酵母P12 子囊孢子 单倍体 MATA/MATB |
Preparation of Yarrowia lipolytica P12 haploid |
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| QU Yixiao,ZHANG Yaxin,ZHANG Tian,HAO Shunshui,ZHANG Xinwei,GUO Bei. Preparation of Yarrowia lipolytica P12 haploid[J]. Microbiology China, 2021, 48(5): 1674-1680 |
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| Authors: | QU Yixiao ZHANG Yaxin ZHANG Tian HAO Shunshui ZHANG Xinwei GUO Bei |
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| Affiliation: | 1 College of Bioscience and Resources Environment, Beijing University of Agriculture, Beijing 102206, China; 1 College of Bioscience and Resources Environment, Beijing University of Agriculture, Beijing 102206, China;2 Key Laboratory of Urban Agriculture in North China, Ministry of Agriculture and Rural Affairs, Beijing 102206, China |
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| Abstract: | [Background] Currently, with the in-depth study of the yeast and the completion of the whole genome and mitochondrial gene sequence determination, Yarrowia lipolytica is popular for using in experimental research and industrial production. However, compared with conventional yeasts, the lack of effective genetic transformation system is also difficulties in gene regulation for Y. lipolytica. At the same time, the chromosome ploidy of yeast will also affect the transformation. When the haploid cells are as receptors for functional gene modification, it can avoid the effect of interaction between alleles. Solve the problem of incomplete gene knockout in polyploid cells. [Objective] The mutant strain P12 of Y. lipolytica was used as the research object. The haploid protease was isolated by different methods, with the aim of establishing a method of preparing haploid strains of Y. lipolytica. [Methods] Y. lipolytica strain was induced to produce ascospores by solid McClary sporulation medium with the culture condition at 30 °C for 7?14 d and liquid McClary sporulation medium with the culture condition at 200 r/min for 2?4 d, respectively. Then the ascospore cell wall was lysed with 2% snail enzyme at 33 °C for 3 h. Finally, the haploid cells were screened and identified by staining microscopy and PCR. [Results] The growth rate of Y. lipolytica was faster in liquid sporulation medium, and the quality of sporulation was better in solid sporulation medium. In the same field of view, the number of spores in the liquid sporulation medium was about 3.7 times higher than in the solid sporulation medium. Moreover, six strains of Y. lipolytica P12 type B haploid were obtained through preliminary exploration and screening. [Conclusion] This research laid the foundation for the subsequent continued operations of genetic engineering. |
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| Keywords: | Yarrowia lipolytica P12 ascospores haploid MATA/MATB |
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