为杜纳利藻开发叶绿体表达系统

IF 3.4 3区 生物学 Q2 BIOTECHNOLOGY & APPLIED MICROBIOLOGY
Hao-Hong Chen , Qian-Xi Zheng , Fan Yu , Shan-Rong Xie , Jian-Guo Jiang
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引用次数: 0

摘要

盐生杜莎藻具有耐盐性强、不易受污染和无细胞壁等独特优势,是一种创新的表达系统。虽然核转化已被广泛研究,但有关盐生杜莎藻叶绿体转化的研究仍处于初步阶段。在这项研究中,我们利用金门组装技术建立了一种高效的盐湖水稻叶绿体表达系统。我们开发了一个由叶绿体特异性启动子、终止子、同源片段和各种载体等基本元件组成的 D. salina 工具包。我们通过表达 EGFP 蛋白证实了其功能。此外,我们还详细介绍了整个构建过程的方法。该表达系统可通过简单的同源重组实现外来基因的特异性定位,从而在叶绿体中稳定表达。该工具包在较短的实验周期内实现了较高的转化效率。因此,该工具包的构建和利用有可能提高盐湖藻转基因工程的效率,推动微藻生物工厂的发展。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

Development of a chloroplast expression system for Dunaliella salina

Development of a chloroplast expression system for Dunaliella salina

Dunaliella salina is an innovative expression system due to its distinct advantages such as high salt tolerance, low susceptibility to contamination, and the absence of the cell wall. While nuclear transformation has been extensively studied, research on D. salina chloroplast transformation remains in the preliminary stages. In this study, we established an efficient chloroplast expression system for D. salina using Golden Gate assembly. We developed a D. salina toolkit comprising essential components such as chloroplast-specific promoters, terminators, homologous fragments, and various vectors. We confirmed its functionality by expressing the EGFP protein. Moreover, we detailed the methodology of the entire construction process. This expression system enables the specific targeting of foreign genes through simple homologous recombination, resulting in stable expression in chloroplasts. The toolkit achieved a relatively high transformation efficiency within a shorter experimental cycle. Consequently, the construction and utilization of this toolkit have the potential to enhance the efficiency of transgenic engineering in D. salina and advance the development of microalgal biofactories.

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来源期刊
Enzyme and Microbial Technology
Enzyme and Microbial Technology 生物-生物工程与应用微生物
CiteScore
7.60
自引率
5.90%
发文量
142
审稿时长
38 days
期刊介绍: Enzyme and Microbial Technology is an international, peer-reviewed journal publishing original research and reviews, of biotechnological significance and novelty, on basic and applied aspects of the science and technology of processes involving the use of enzymes, micro-organisms, animal cells and plant cells. We especially encourage submissions on: Biocatalysis and the use of Directed Evolution in Synthetic Biology and Biotechnology Biotechnological Production of New Bioactive Molecules, Biomaterials, Biopharmaceuticals, and Biofuels New Imaging Techniques and Biosensors, especially as applicable to Healthcare and Systems Biology New Biotechnological Approaches in Genomics, Proteomics and Metabolomics Metabolic Engineering, Biomolecular Engineering and Nanobiotechnology Manuscripts which report isolation, purification, immobilization or utilization of organisms or enzymes which are already well-described in the literature are not suitable for publication in EMT, unless their primary purpose is to report significant new findings or approaches which are of broad biotechnological importance. Similarly, manuscripts which report optimization studies on well-established processes are inappropriate. EMT does not accept papers dealing with mathematical modeling unless they report significant, new experimental data.
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