Establishing Gene Expression and Knockout Methods in Esteya vermicola CBS115803.

IF 2.4 4区 生物学 Q3 BIOCHEMISTRY & MOLECULAR BIOLOGY Molecular Biotechnology Pub Date : 2024-10-01 Epub Date: 2023-10-01 DOI:10.1007/s12033-023-00898-6
Zhijuan Hu, Chi Chen, Xinyao Zheng, Jingjie Yuan, Run Zou, Chengjian Xie
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Abstract

Pine wilt disease, which is caused by the nematode Bursaphelenchus xylophilus, is one of the most destructive forest diseases worldwide. Esteya vermicola, a nematophagous fungus, has emerged as a promising biological control agent. However, the limited availability of gene function analysis techniques hinders further genetic modification of this fungus. In this study, we employed a combination of enzymes (driselase, snailase, and cellulase) to enzymatically degrade the cell wall of the fungus, resulting in a high yield of protoplasts. Furthermore, by utilizing 0.6 M sucrose as an osmotic pressure stabilizer, we achieved a significant protoplast regeneration rate of approximately 31%. Subsequently, we employed the polyethylene glycol-mediated protoplast transformation method to successfully establish a genetic transformation technique for E. vermicola CBS115803. Additionally, through our investigation, we identified the Olic promoter from Aspergillus nidulans, which effectively enhanced the expression of the DsRed gene encoding a red fluorescent protein in E. vermicola CBS115803. Moreover, we successfully implemented a split-marker strategy to delete the EvIPMD gene in E. vermicola CBS115803. In summary, our findings present valuable experimental methodologies for gene function analysis in E. vermicola CBS115803.

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建立粉丝Esteya CBS115803。
松材线虫引起的松材枯萎病是世界范围内最具破坏性的森林病害之一。蠕虫Esteya是一种食线虫真菌,已成为一种很有前途的生物防治剂。然而,基因功能分析技术的有限可用性阻碍了这种真菌的进一步遗传修饰。在这项研究中,我们使用了一种酶(driselase、snailase和纤维素酶)的组合来酶促降解真菌的细胞壁,从而获得高产原生质体。此外,通过使用0.6M蔗糖作为渗透压稳定剂,我们实现了约31%的显著原生质体再生率。随后,我们采用聚乙二醇介导的原生质体转化方法,成功地建立了粉丝大肠杆菌CBS115803的遗传转化技术。此外,通过我们的研究,我们从构巢曲霉中鉴定了Olic启动子,它有效地增强了编码红色荧光蛋白的DsRed基因在蠕虫大肠杆菌CBS115803中的表达。此外,我们成功地实现了一种分离标记策略,以删除蠕虫大肠杆菌CBS115803中的EvIPMD基因。总之,我们的发现为粉丝大肠杆菌CBS115803的基因功能分析提供了有价值的实验方法。
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来源期刊
Molecular Biotechnology
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.
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