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RNA干扰的RNA测序验证确定了赤拟谷盗(鞘翅目:拟步甲科)中的其他基因连接性。

RNA-Seq Validation of RNAi Identifies Additional Gene Connectivity in Tribolium castaneum (Coleoptera: Tenebrionidae).

作者信息

Perkin Lindsey C, Gerken Alison R, Oppert Brenda

机构信息

USDA, Agricultural Research Service, Center for Grain and Animal Health Research, 1515 College Avenue, Manhattan, KS 66502 (

出版信息

J Insect Sci. 2017 Jan 1;17(2). doi: 10.1093/jisesa/iex026.

Abstract

RNA interference (RNAi) is a functional genomics tool to correlate genotype and phenotype by delivering targeted, gene-specific, and complementary dsRNA into a host via injection, feeding, or other means in order to reduce gene expression. In the red flour beetle, Tribolium castaneum, RNAi has been successful via injected dsRNA at all life stages. Traditionally, successful transcript knockdown has been quantified by qPCR on a gene-by-gene basis, where only expression of the target gene and normalization genes are evaluated. In this study, RNA-Seq was used to quantify transcript expression in larvae injected with dsRNA for aspartate 1-decarboxylase (ADC), which gives a reliable phenotype of an adult with a black cuticle instead of the wild-type red-brown. ANOVA of control, mock-injected, and ADC-dsRNA injected larvae indicated that target gene expression was significantly (P = 0.002) reduced 4-fold, and the black phenotype was achieved in all adults injected with ADC-dsRNA as larvae. In a pairwise analysis, significant (P < 0.05) differential expression of other genes in ADC-injected larvae suggested connections between gene pathways. One gene, dopamine receptor 2, was increased in expression 227-fold (P = 0.025), presumably connected to previous data that showed a reduction in expression of ADC results in increased levels of dopamine. To evaluate the hypothesis that increased dopamine levels can affect mobility, T. castaneum adults injected with ADC-dsRNA as larvae were significantly impaired in movement tests compared to controls, similar to black mutants in Drosophila melanogaster. The data demonstrate that RNA-Seq can reveal gene connectivity and provide more complete data validation and analysis compared to qPCR.

摘要

RNA干扰(RNAi)是一种功能基因组学工具,通过注射、喂食或其他方式将靶向的、基因特异性的互补双链RNA(dsRNA)导入宿主,以降低基因表达,从而将基因型与表型关联起来。在赤拟谷盗(Tribolium castaneum)中,通过在所有生命阶段注射dsRNA,RNA干扰已取得成功。传统上,成功的转录本敲低是通过逐个基因的定量PCR(qPCR)来量化的,其中仅评估靶基因和标准化基因的表达。在本研究中,RNA测序(RNA-Seq)用于量化注射了天冬氨酸1-脱羧酶(ADC)dsRNA的幼虫中的转录本表达,ADC基因敲低会使成虫产生可靠的黑色表皮表型,而非野生型的红棕色。对对照、模拟注射和注射ADC-dsRNA的幼虫进行方差分析(ANOVA)表明,靶基因表达显著降低了4倍(P = 0.002),并且所有在幼虫期注射ADC-dsRNA的成虫均呈现黑色表型。在成对分析中,注射ADC的幼虫中其他基因的显著差异表达(P < 0.05)表明基因途径之间存在联系。其中一个基因,多巴胺受体2,表达增加了227倍(P = 0.025),推测这与之前的数据相关,即ADC表达降低会导致多巴胺水平升高。为了评估多巴胺水平升高会影响活动能力这一假设,与对照组相比,在幼虫期注射ADC-dsRNA的赤拟谷盗成虫在运动测试中明显受损,类似于黑腹果蝇(Drosophila melanogaster)中的黑色突变体。数据表明,与qPCR相比,RNA-Seq可以揭示基因连接性,并提供更完整的数据验证和分析。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3566/5416897/a1c63dc7ea37/iex026f1p.jpg

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