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Development of bicistronic expression system for the enhanced and reliable production of recombinant proteins in Leuconostoc citreum

机译:双顺反子表达系统的开发用于增强和可靠地生产柠檬色隐球菌中的重组蛋白

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摘要

The lactic acid bacteria (LAB) Leuconostoc citreum are non-sporulating hetero-fermentative bacteria that play an important role in the fermented food industry. In this study, for the enhanced and reliable production of recombinant proteins in L. citreum, we developed a bicistronic design (BCD) expression system which includes a short leader peptide (1st cistron) followed by target genes (2nd cistron) under the control of a single promoter. Using superfolder green fluorescent protein (sfGFP) as a reporter, the functionality of BCD in L. citreum was verified. Further, to improve the expression in BCD, we tried to engineer a Shine-Dalgarno sequence (SD2) for the 2nd cistron and a promoter by FACS screening of random libraries, and both strong SD2 (eSD2) and promoter (P710V4) were successfully isolated. The usefulness of the engineered BCD with P710V4 and eSD2 was further validated using three model proteins—glutathione-s-transferase, human growth hormone, and α-amylase. All examined proteins were successfully produced with levels highly increased compared with those in the original BCD as well as the monocistronic design (MCD) expression system.
机译:乳酸菌(LAB)柠檬色隐球菌是无孢子的异质发酵菌,在发酵食品工业中起着重要的作用。在这项研究中,为增强和可靠地在柠檬酸乳杆菌中生产重组蛋白,我们开发了双顺反子设计(BCD)表达系统,该系统包括一个短前导肽(1 st 顺反子),后接靶基因(2 nd 顺反子)在单个启动子的控制下。使用超级文件夹绿色荧光蛋白(sfGFP)作为报告基因,验证了柠檬酸杆菌中BCD的功能。此外,为了改善在BCD中的表达,我们尝试通过FACS筛选随机文库和强SD2(eSD2)来设计2 sup顺反子和启动子的Shine-Dalgarno序列(SD2)。成功分离了启动子(P710V4)。使用三种模型蛋白(谷胱甘肽-S-转移酶,人类生长激素和α-淀粉酶)进一步验证了带有P710V4和eSD2的BCD工程菌的有用性。与原始BCD以及单顺反子设计(MCD)表达系统相比,所有检测的蛋白质均成功生产,并且水平大大提高。

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