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利用 CRISPR-Cas9 系统探究杆状病毒载体基因对外源基因表达的必要性。

Probing Baculovirus Vector Gene Essentiality for Foreign Gene Expression Using a CRISPR-Cas9 System.

机构信息

Department of Chemical Engineering, Faculty of Engineering, University of Waterloo, Waterloo, ON, Canada.

Department of Biology, Faculty of Science, University of Waterloo, Waterloo, ON, Canada.

出版信息

Methods Mol Biol. 2024;2829:127-156. doi: 10.1007/978-1-0716-3961-0_9.

Abstract

The baculovirus expression vector system (BEVS) has now found acceptance in both research laboratories and industry, which can be attributed to many of its key features including the limited host range of the vectors, their non-pathogenicity to humans, and the mammalian-like post-translational modification (PTMs) that can be achieved in insect cells. In fact, this system acts as a middle ground between prokaryotes and higher eukaryotes to produce complex biologics. Still, industrial use of the BEVS lags compared to other platforms. We have postulated that one reason for this has been a lack of genetic tools that can complement the study of baculovirus vectors, while a second reason is the co-production of the baculovirus vector with the desired product. While some genetic enhancements have been made to improve the BEVS as a production platform, the genome remains under-scrutinized. This chapter outlines the methodology for a CRISPR-Cas9-based transfection-infection assay to probe the baculovirus genome for essential/nonessential genes that can potentially maximize foreign gene expression under a promoter of choice.

摘要

杆状病毒表达载体系统 (BEVS) 现在在研究实验室和工业界都得到了认可,这可以归因于其许多关键特征,包括载体的宿主范围有限、对人类无致病性,以及可以在昆虫细胞中实现类似哺乳动物的翻译后修饰 (PTMs)。实际上,该系统在原核生物和高等真核生物之间起到了桥梁作用,可用于生产复杂的生物制剂。尽管如此,BEVS 的工业应用仍落后于其他平台。我们推测,造成这种情况的一个原因是缺乏能够补充杆状病毒载体研究的遗传工具,另一个原因是杆状病毒载体与所需产物的共同生产。虽然已经对 BEVS 进行了一些遗传增强以改善其作为生产平台的性能,但基因组仍未得到充分研究。本章概述了一种基于 CRISPR-Cas9 的转染-感染测定方法,用于探测杆状病毒基因组中潜在的必需/非必需基因,这些基因可以在选择的启动子下最大限度地提高外源基因的表达。

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