为迷宫甲烷虫的诱导基因表达编译多功能工具箱。

microLife Pub Date : 2024-10-10 eCollection Date: 2024-01-01 DOI:10.1093/femsml/uqae019
Johanna Hüttermann, Ruth Schmitz
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引用次数: 0

摘要

迷宫甲壳动物是一种模式生物,为探索甲壳动物在转录和翻译水平上的调控机制提供了一个平台。本研究调查和评估了多种分子工具,以实现马兹甲烷虫的诱导基因表达。(i) 利用 TetR/TetO 系统诱导表达设计的针对 sRNA154 的反义 RNA,使 asRNA154 的转录本增加(500 倍),导致 sRNA154 水平显著下降(四环素诱导的基因敲除突变体)。在基因敲除突变体中,nifH、glnK1 和 glnA1 的转录本水平降低了 50 倍,进一步证实了 sRNA154 的大幅降低,而 sRNA154 可提高这些基因的稳定性。(ii) 在翻译调控方面,设计了一种 RNA 温度计,并首次在古生生物中使用,该温度计插入报告基因的 5'- 非翻译区,当温度从 30°C 升至 40°C 时,报告基因的蛋白质表达增强。(iii) 我们评估并研究了三甲胺(TMA)诱导的多聚核 mRNA 的长 5'-UTR,将其作为在翻译水平上诱导基因表达的潜在遗传工具。然而,我们发现 TMA 依赖性调控很可能发生在转录本水平。(iv) 利用链霉素乙酰转移酶基因为马泽霉菌建立了一个新的选择标记(耐诺索三嗪)。综上所述,我们的研究结果为未来探索马泽氏菌和其他元古细菌的遗传调控和诱导基因表达奠定了基础,推动了这些生物的遗传研究,并提高了它们在生物技术应用方面的潜力。
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Compiling a versatile toolbox for inducible gene expression in Methanosarcina mazei.

Methanosarcina mazei is a model organism, providing a platform to explore methanoarchaeal regulation mechanisms on the transcriptional and translational level. This study investigates and evaluates various molecular tools to allow inducible gene expression in M. mazei. (i) The TetR/TetO system was utilized to induce expression of a designed antisense RNA directed against sRNA154 allowing to increase transcripts of asRNA154 (500-fold), resulting in a significant decrease of sRNA154 levels (tetracycline-induced knockdown mutant). Strong reduction of sRNA154 was further confirmed in the knockdown mutant by up to 50-fold decreased transcript levels of the genes nifH, glnK1 , and glnA1 , the stability of which is increased by sRNA154. (ii) For translational regulation, an RNA thermometer was designed and first-ever utilized in an archaeon, inserted into the 5'-untranslated region of a reporter gene, which showed enhanced protein expression upon a temperature shift from 30°C to 40°C. (iii) The long 5'-UTR of a trimethylamine (TMA)-inducible polycistronic mRNA was evaluated and studied as a potential genetic tool for induced gene expression on the translational level. However, we discovered TMA-dependent regulation occurs most likely on the transcript level. (iv) A new selection marker (nourseothricin resistance) was established for M. mazei using the streptothricin acetyltransferase gene. Taken together, our findings provide a foundation for future exploration of genetic regulation and inducible gene expression in M. mazei and other methanoarchaea, advancing genetic studies in these organisms and enhancing their potential for biotechnology applications.

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