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利用同源依赖性修复的 CRISPR/Cas-9 介导基因敲入技术在西尼罗河病毒载体库蚊中实现。

CRISPR/Cas-9 mediated knock-in by homology dependent repair in the West Nile Virus vector Culex quinquefasciatus Say.

机构信息

Arthropod Genetics, The Pirbright Institute, Ash Road, Pirbright, GU24 0NF, Surrey, UK.

出版信息

Sci Rep. 2021 Jul 22;11(1):14964. doi: 10.1038/s41598-021-94065-z.

Abstract

Culex quinquefasciatus Say is a mosquito distributed in both tropical and subtropical regions of the world. It is a night-active, opportunistic blood-feeder and vectors many animal and human diseases, including West Nile Virus and avian malaria. Current vector control methods (e.g. physical/chemical) are increasingly ineffective; use of insecticides also imposes hazards to both human and ecosystem health. Advances in genome editing have allowed the development of genetic insect control methods, which are species-specific and, theoretically, highly effective. CRISPR/Cas9 is a bacteria-derived programmable gene editing tool that is functional in a range of species. We describe the first successful germline gene knock-in by homology dependent repair in C. quinquefasciatus. Using CRISPR/Cas9, we integrated an sgRNA expression cassette and marker gene encoding a fluorescent protein fluorophore (Hr5/IE1-DsRed, Cq7SK-sgRNA) into the kynurenine 3-monooxygenase (kmo) gene. We achieved a minimum transformation rate of 2.8%, similar to rates in other mosquito species. Precise knock-in at the intended locus was confirmed. Insertion homozygotes displayed a white eye phenotype in early-mid larvae and a recessive lethal phenotype by pupation. This work provides an efficient method for engineering C. quinquefasciatus, providing a new tool for developing genetic control tools for this vector.

摘要

致倦库蚊是一种分布在世界热带和亚热带地区的蚊子。它是一种夜行性、机会主义的吸血昆虫,传播多种动物和人类疾病,包括西尼罗河病毒和禽疟原虫。目前的病媒控制方法(如物理/化学方法)的效果越来越差;杀虫剂的使用也对人类和生态系统健康造成危害。基因组编辑技术的进步使得遗传昆虫控制方法得以发展,这种方法具有物种特异性,理论上非常有效。CRISPR/Cas9 是一种源自细菌的可编程基因编辑工具,在多种物种中都具有功能。我们描述了在致倦库蚊中首次通过同源依赖性修复实现的生殖系基因敲入。我们使用 CRISPR/Cas9 将 sgRNA 表达盒和标记基因(编码荧光蛋白荧光团(Hr5/IE1-DsRed,Cq7SK-sgRNA))整合到色氨酸 3-单加氧酶(kmo)基因中。我们实现了 2.8%的最低转化率,与其他蚊子物种的转化率相似。在预期的基因座上进行了精确的敲入,得到了确认。插入纯合子在早期中期幼虫中表现出白眼表型,在蛹化时表现出隐性致死表型。这项工作提供了一种有效的致倦库蚊工程方法,为开发这种病媒的遗传控制工具提供了新工具。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e0f6/8298393/732515ec2e27/41598_2021_94065_Fig1_HTML.jpg

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