The First Introduction of an Exogenous 5ʹ Untranslated Region for Control of Plastid Transgene Expression in Chlamydomonas reinhardtii

IF 2.4 4区生物学 Q3 BIOCHEMISTRY & MOLECULAR BIOLOGY

Molecular Biotechnology Pub Date : 2024-09-13 DOI:10.1007/s12033-024-01279-3

Mohammad Ali Abbasi-Vineh, Masoumeh Emadpour

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Abstract

The utilization of heterologous 5' untranslated regions (5′UTRs) for expressing foreign proteins in the chloroplast of Chlamydomonas reinhardtii (C. reinhardtii) has posed a persistent challenge over the years. This challenge stems from the lack of a defined and comprehensive set of translational cis-elements responsible for stability, ribosome binding, and translation initiation, which are mediated by trans-acting factors native to C. reinhardtii. In the current study, we aimed to address this bottleneck by employing the 5′UTR from gene 10 of the T7 bacteriophage (T7g10 5'UTR), fused to the promoter of C. reinhardtii small subunit ribosomal RNA (rrnS), to facilitate the translation of a reporter gene, YFP. Using a chimeric construct, the YFP mRNA was efficiently translated utilizing the heterologous T7g10 5′UTR. Furthermore, the accumulation of YFP protein under the control of the T7g10 5′UTR was approximately one third of that observed under the control of the endogenous psaA promoter/5′UTR in the C. reinhardtii chloroplast. The results of computational analyses demonstrated that the T7g10 5ʹUTR sequence shares common elements with the endogenous 5ʹUTRs of the chloroplast genes. Moreover, the findings of the current study highlighted the potential of employing bacteriophage 5′UTRs for the foreign protein accumulation from the chloroplast genome of C. reinhardtii.

Graphical Abstract

Abstract Image

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首次引入外源 5ʹ 非翻译区控制衣藻质粒转基因的表达

多年来，利用异源 5' 非翻译区（5′UTR）在衣藻叶绿体中表达外来蛋白质一直是个难题。这一挑战源于缺乏一套确定的、全面的翻译顺式元件，这些元件负责稳定性、核糖体结合和翻译起始，并由 C. reinhardtii 原生的反式作用因子介导。在目前的研究中，我们利用噬菌体 T7 基因 10 的 5′UTR（T7g10 5'UTR）与 C. reinhardtii 小亚基核糖体 RNA（rrnS）的启动子融合，来促进报告基因 YFP 的翻译，从而解决这一瓶颈问题。通过嵌合构建体，YFP mRNA 利用异源 T7g10 5′UTR 进行了高效翻译。此外，在 T7g10 5′UTR 的控制下，YFP 蛋白的积累量大约是在 C. reinhardtii 叶绿体中内源 psaA 启动子/5′UTR 控制下所观察到的积累量的三分之一。计算分析的结果表明，T7g10的5ʹUTR序列与叶绿体基因的内源5ʹUTR具有共同的元素。此外，本研究的结果凸显了利用噬菌体5′UTR从叶绿体基因组中积累外来蛋白质的潜力。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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来源期刊

Molecular Biotechnology 医学-生化与分子生物学

CiteScore

4.10

自引率

3.80%

发文量

165

审稿时长

6 months

期刊介绍： Molecular Biotechnology publishes original research papers on the application of molecular biology to both basic and applied research in the field of biotechnology. Particular areas of interest include the following: stability and expression of cloned gene products, cell transformation, gene cloning systems and the production of recombinant proteins, protein purification and analysis, transgenic species, developmental biology, mutation analysis, the applications of DNA fingerprinting, RNA interference, and PCR technology, microarray technology, proteomics, mass spectrometry, bioinformatics, plant molecular biology, microbial genetics, gene probes and the diagnosis of disease, pharmaceutical and health care products, therapeutic agents, vaccines, gene targeting, gene therapy, stem cell technology and tissue engineering, antisense technology, protein engineering and enzyme technology, monoclonal antibodies, glycobiology and glycomics, and agricultural biotechnology.