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通过脱水和浸泡在蛹中进行RNA干扰介导的沉默导致表皮发育中的多种缺陷。

RNAi-Mediated Silencing of in Pupae via Dehydration and Soaking Results in Multiple Defects in Cuticular Development.

作者信息

Naumenko Anastasia N, Fritz Megan L

机构信息

Department of Entomology, University of Maryland, College Park, MD 20742, USA.

出版信息

Insects. 2024 Mar 14;15(3):193. doi: 10.3390/insects15030193.

Abstract

Mosquitoes transmit a range of pathogens, causing devastating effects on human health. Population genetic control strategies have been developed and successfully used for several mosquito species. The most important step in identifying potential targets for mosquito control is the understanding of gene function. RNA interference (RNAi) is a powerful tool for gene silencing which has been widely used to study gene function in insects via knockdown of expression. The success of RNAi in insects depends on the efficient delivery of dsRNA into the cells, with microinjections being the most commonly used to study mosquito gene function. However, microinjections in the pupal stage lead to significant mortality in and species, and few studies have performed microinjections in Culicinae pupae. Advanced techniques, such as CRISPR/Cas9 knockout, require establishing individual mosquito lines for each gene studied, and maintaining such lines may be limited by the insect-rearing capacity of a laboratory. Moreover, at times gene knockout during early development (embryo stage) has a deleterious effect on mosquito development, precluding the analysis of gene function in the pupal and adult stages and its potential for mosquito control. There is a need for a simple procedure that can be used for the fast and reliable examination of adult gene function via RNAi knockdown. Here, we focus on the aquatic stages of the mosquito life cycle and suggest a quick and easy assay for screening the functional role of genes in mosquitoes without using microinjections. By dehydration of early stage pupae and subsequent rehydration in highly concentrated dsRNA, we achieved a moderate knockdown of , a gene that turns on in the pupal stage and is responsible for melanization and sclerotization of the adult cuticle.

摘要

蚊子传播多种病原体,对人类健康造成毁灭性影响。人们已经制定了种群遗传控制策略,并成功应用于几种蚊子。确定蚊子控制潜在目标的最重要步骤是了解基因功能。RNA干扰(RNAi)是一种强大的基因沉默工具,已被广泛用于通过敲低表达来研究昆虫的基因功能。RNAi在昆虫中的成功取决于双链RNA(dsRNA)有效递送至细胞内,显微注射是研究蚊子基因功能最常用的方法。然而,在蛹期进行显微注射会导致某些蚊种出现显著死亡率,且很少有研究对库蚊亚科蛹进行显微注射。先进技术,如CRISPR/Cas9基因敲除,需要为每个研究的基因建立单独的蚊子品系,而维持这些品系可能会受到实验室昆虫饲养能力的限制。此外,有时早期发育(胚胎期)的基因敲除会对蚊子发育产生有害影响,从而排除了对蛹期和成虫期基因功能及其在蚊子控制方面潜力的分析。因此,需要一种简单的程序,可用于通过RNAi敲低快速可靠地检测成虫基因功能。在此,我们聚焦于蚊子生命周期的水生阶段,并提出一种快速简便的检测方法,无需显微注射即可筛选基因在库蚊中的功能作用。通过对早期蛹进行脱水处理,随后在高浓度dsRNA中复水,我们实现了对一个在蛹期开启且负责成虫表皮黑化和硬化的基因的适度敲低。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/d9c3/10971320/e67490a9edde/insects-15-00193-g001.jpg

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