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利用一个强组成型启动子和一个茶碱激活的合成核糖开关构建枯草芽孢杆菌的诱导型基因表达系统。

Engineering an inducible gene expression system for Bacillus subtilis from a strong constitutive promoter and a theophylline-activated synthetic riboswitch.

作者信息

Cui Wenjing, Han Laichuang, Cheng Jintao, Liu Zhongmei, Zhou Li, Guo Junling, Zhou Zhemin

机构信息

School of Biotechnology, Jiangnan University, 1800 Lihu Road, Wuxi, 214122, Jiangsu, China.

Key Laboratory of Industrial Biotechnology (Ministry of Education), Jiangnan University, 1800 Lihu Road, Wuxi, 214122, Jiangsu, China.

出版信息

Microb Cell Fact. 2016 Nov 22;15(1):199. doi: 10.1186/s12934-016-0599-z.

Abstract

BACKGROUND

Synthetic riboswitches have been increasingly used to control and tune gene expression in diverse organisms. Although a set of theophylline-responsive riboswitches have been developed for bacteria, fully functional expression elements mediated by synthetic riboswitches in Bacillus subtilis are rarely used because of the host-dependent compatibility between the promoters and riboswitches.

RESULTS

A novel genetic element composed of the promoter P43 and a theophylline-riboswitch was developed and characterized in B. subtilis. When combined with a P43 promoter (P43'-riboE1), the theophylline-riboswitch successfully switched the constitutive expression pattern of P43 to an induced pattern. The expression mediated by the novel element could be activated at the translational level by theophylline with a relatively high induction ratio. The induction ratios for P43'-riboE1 by 4-mM theophylline were elevated during the induction period. The level of induced expression was dependent on the theophylline dose. Correspondingly, the induction ratios gradually increased in parallel with the elevated dose of theophylline. Importantly, the induced expression level was higher than three other strong constitutive promoters including P, P, and the native P43. It was found that the distance between the SD sequence within the expression element and the start codon significantly influenced both the level of induced expression and the induction ratio. A 9-bp spacer was suitable for producing desirable expression level and induction ratio. Longer spacer reduced the activation efficiency. Importantly, the system successfully overexpressed β-glucuronidase at equal levels, and induction ratio was similar to that of GFP.

CONCLUSION

The constructed theophylline-inducible gene expression system has broad compatibility and robustness, which has great potential in over-production of pharmaceutical and industrial proteins and utilization in building more complex gene circuits.

摘要

背景

合成核糖开关已越来越多地用于控制和调节多种生物体中的基因表达。尽管已经开发出了一组用于细菌的茶碱响应核糖开关,但由于启动子和核糖开关之间存在宿主依赖性兼容性,在枯草芽孢杆菌中由合成核糖开关介导的全功能表达元件很少被使用。

结果

在枯草芽孢杆菌中开发并表征了一种由启动子P43和茶碱核糖开关组成的新型遗传元件。当与P43启动子(P43'-riboE1)结合时,茶碱核糖开关成功地将P43的组成型表达模式转变为诱导型模式。该新型元件介导的表达可以在翻译水平上被茶碱激活,诱导率相对较高。在诱导期,4 mM茶碱对P43'-riboE1的诱导率有所提高。诱导表达水平取决于茶碱剂量。相应地,诱导率随着茶碱剂量的增加而逐渐平行增加。重要的是,诱导表达水平高于其他三个强组成型启动子,包括P、P和天然P43。研究发现,表达元件内的SD序列与起始密码子之间的距离显著影响诱导表达水平和诱导率。9 bp的间隔区适合产生理想的表达水平和诱导率。更长的间隔区会降低激活效率。重要的是,该系统成功地以相等水平过表达β-葡萄糖醛酸酶,诱导率与绿色荧光蛋白相似。

结论

构建的茶碱诱导型基因表达系统具有广泛的兼容性和稳健性,在药用和工业蛋白质的过量生产以及构建更复杂的基因回路方面具有巨大潜力。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/5bfa/5120567/46c9aa0bc6cf/12934_2016_599_Fig1_HTML.jpg

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