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改造解脂耶氏酵母以表达带有强FBA1IN启动子的分泌型转化酶。

Engineering Yarrowia lipolytica to express secretory invertase with strong FBA1IN promoter.

作者信息

Hong Seung-Pyo, Seip John, Walters-Pollak Dana, Rupert Ross, Jackson Raymond, Xue Zhixiong, Zhu Quinn

机构信息

Central Research and Development, DuPont Co., Wilmington, DE, USA.

出版信息

Yeast. 2012 Feb;29(2):59-72. doi: 10.1002/yea.1917. Epub 2011 Dec 29.

Abstract

Oleaginous yeast Yarrowia lipolytica is an important host for the production of lipid-derived compounds or heterologous proteins. Selection of strong promoters and effective expression systems is critical for heterologous protein secretion. To search for a strong promoter in Y. lipolytica, activities of FBA1, TDH1 and GPM1 promoters were compared to that of TEF1 promoter by constructing GUS reporter fusions. The FBA1 promoter activity was 2.2 and 5.5 times stronger than the TDH1 and GPM1 promoters, respectively. The FBA1IN promoter (FBA1 sequence of -826 to +169) containing an intron (+64 to +165) showed five-fold higher expression than the FBA1 promoter (-831 to -1). The transcriptional enhancement by the 5'-region within the FBA1 gene was confirmed by GPM1::FBA1 chimeric promoter construction. Using the strong FBA1IN promoter, four different S. cerevisiae SUC2 expression cassettes were tested for the SUC+ phenotype in Y. lipolytica. Functional invertase secretion was facilitated by the Xpr2 prepro-region with an additional 13 amino acids of mature Xpr2, or by the native Suc2 signal sequence. However, these two secretory signals in tandem, or the mature Suc2 with no secretory signal, did not direct secretion of functional invertase. Unlike previously reported Y. lipolytica SUC+ strains, our engineered stains secreted most of invertase into the medium.

摘要

产油酵母解脂耶氏酵母是生产脂质衍生化合物或异源蛋白的重要宿主。选择强启动子和有效的表达系统对于异源蛋白分泌至关重要。为了在解脂耶氏酵母中寻找强启动子,通过构建GUS报告基因融合体,将FBA1、TDH1和GPM1启动子的活性与TEF1启动子的活性进行了比较。FBA1启动子活性分别比TDH1和GPM1启动子强2.2倍和5.5倍。含有内含子(+64至+165)的FBA1IN启动子(-826至+169的FBA1序列)的表达比FBA1启动子(-831至-1)高5倍。通过构建GPM1::FBA1嵌合启动子证实了FBA1基因内5'区域的转录增强。使用强FBA1IN启动子,测试了四种不同的酿酒酵母SUC2表达盒在解脂耶氏酵母中的SUC+表型。Xpr2前原区加上成熟Xpr2的另外13个氨基酸,或天然Suc2信号序列促进了功能性转化酶的分泌。然而,这两个分泌信号串联,或没有分泌信号的成熟Suc2,都不能指导功能性转化酶的分泌。与先前报道的解脂耶氏酵母SUC+菌株不同,我们构建的菌株将大部分转化酶分泌到培养基中。

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