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定量实时 PCR 参考基因的验证和解毒相关基因在农药诱导下的空间表达谱在蜜蜂,Apis mellifera 中的研究。

Validation of quantitative real-time PCR reference genes and spatial expression profiles of detoxication-related genes under pesticide induction in honey bee, Apis mellifera.

机构信息

Department of Ecological Science, Kyungpook National University, Sangju, Gyeongbuk, Republic of Korea.

Department of Applied Biology, Kyungpook National University, Sangju, Gyeongbuk, Republic of Korea.

出版信息

PLoS One. 2022 Nov 10;17(11):e0277455. doi: 10.1371/journal.pone.0277455. eCollection 2022.

Abstract

Recently, pesticides have been suggested to be one of the factors responsible for the large-scale decline in honey bee populations, including colony collapse disorder. The identification of the genes that respond to pesticide exposure based on their expression is essential for understanding the xenobiotic detoxification metabolism in honey bees. For the accurate determination of target gene expression by quantitative real-time PCR, the expression stability of reference genes should be validated in honey bees exposed to various pesticides. Therefore, in this study, to select the optimal reference genes, we analyzed the amplification efficiencies of five candidate reference genes (RPS5, RPS18, GAPDH, ARF1, and RAD1a) and their expression stability values using four programs (geNorm, NormFinder, BestKeeper, and RefFinder) across samples of five body parts (head, thorax, gut, fat body, and carcass) from honey bees exposed to seven pesticides (acetamiprid, imidacloprid, flupyradifurone, fenitrothion, carbaryl, amitraz, and bifenthrin). Among these five candidate genes, a combination of RAD1a and RPS18 was suggested for target gene normalization. Subsequently, expression levels of six genes (AChE1, CYP9Q1, CYP9Q2, CYP9Q3, CAT, and SOD1) were normalized with a combination of RAD1a and RPS18 in the different body parts from honey bees exposed to pesticides. Among the six genes in the five body parts, the expression of SOD1 in the head, fat body, and carcass was significantly induced by six pesticides. In addition, among seven pesticides, flupyradifurone statistically induced expression levels of five genes in the fat body.

摘要

最近,有研究表明,杀虫剂是导致蜜蜂种群大规模减少的因素之一,包括蜂群崩溃失调症。基于表达谱来鉴定对农药暴露有反应的基因对于了解蜜蜂中外源化学物质的解毒代谢至关重要。为了通过定量实时 PCR 准确确定靶基因的表达,应该在暴露于各种杀虫剂的蜜蜂中验证参考基因的表达稳定性。因此,在这项研究中,为了选择最佳的参考基因,我们分析了五个候选参考基因(RPS5、RPS18、GAPDH、ARF1 和 RAD1a)在五个身体部位(头部、胸部、肠道、脂肪体和尸体)的样本中的扩增效率,并使用四个程序(geNorm、NormFinder、BestKeeper 和 RefFinder)评估了它们的表达稳定性值,这些样本来自于暴露于七种杀虫剂(乙酰甲胺磷、吡虫啉、氟吡呋喃酮、三唑磷、西维因、咪鲜胺和联苯菊酯)的蜜蜂。在这五个候选基因中,RAD1a 和 RPS18 的组合被建议用于靶基因的归一化。随后,用 RAD1a 和 RPS18 的组合对暴露于杀虫剂的蜜蜂不同身体部位的六个基因(AChE1、CYP9Q1、CYP9Q2、CYP9Q3、CAT 和 SOD1)的表达水平进行了归一化。在五个身体部位的六个基因中,SOD1 在头部、脂肪体和尸体中的表达被六种杀虫剂显著诱导。此外,在七种杀虫剂中,氟吡呋喃酮在脂肪体中统计学上诱导了五个基因的表达水平。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/0769/9648776/f3fce11a3568/pone.0277455.g001.jpg

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