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使用基于探针的实时荧光定量PCR对感染蜜蜂的三种微孢子虫(apis微孢子虫、ceranae微孢子虫和bomb微孢子虫)进行特异性检测和定量分析。

Specific detection and quantification of three microsporidia infecting bees, Nosema apis, Nosema ceranae, and Nosema bombi, using probe-based real-time PCR.

作者信息

Babin Aurélie, Schurr Frank, Rivière Marie-Pierre, Chauzat Marie-Pierre, Dubois Eric

机构信息

ANSES, Sophia Antipolis Laboratory, Unit of Honey Bee Pathology, F-06902 Sophia Antipolis, France.

ANSES, Sophia Antipolis Laboratory, Unit of Honey Bee Pathology, F-06902 Sophia Antipolis, France.

出版信息

Eur J Protistol. 2022 Oct;86:125935. doi: 10.1016/j.ejop.2022.125935. Epub 2022 Oct 19.

DOI:10.1016/j.ejop.2022.125935
PMID:36334436
Abstract

Among stressors affecting bee health, Nosema microsporidia are prevalent intracellular parasites. Nosema apis and Nosema ceranae have been described in honey bees (Apis spp.), while Nosema bombi has been described in bumble bees (Bombus spp.). Although available molecular methods serve as a complement to microscopic diagnosis of nosemosis, they do not enable accurate quantification of these three Nosema species. We developed three quantitative real-time PCRs (qPCRs) starting from in silico design of specific primers, probes, and recombinant plasmids, to target the RNA polymerase II subunit B1 (RPB1) gene in the three species. The complete methods, including bee grinding, DNA purification, and qPCR, were validated in honey bee (Apis mellifera) homogenate. Specificity was assessed in silico and in vitro with several types of bee samples. The limit of detection was estimated at 4 log copies/honey bee. A small, systematic method bias was corrected for accurate quantification up to 10 log copies/honey bee. Method accuracy was also verified in bumble bee (Bombus terrestris) and mason bee (Osmia bicornis) homogenates in the range of 5 to 10 log copies/bee. These validated qPCR methods open perspectives in nosemosis diagnosis and in the study of the parasite's eco-dynamics in managed and wild bees.

摘要

在影响蜜蜂健康的应激源中,微孢子虫是普遍存在的细胞内寄生虫。蜜蜂微孢子虫和东方蜜蜂微孢子虫已在蜜蜂(Apis spp.)中被描述,而熊蜂微孢子虫已在熊蜂(Bombus spp.)中被描述。尽管现有的分子方法可作为微孢子虫病显微镜诊断的补充,但它们无法对这三种微孢子虫进行准确的定量分析。我们从特异性引物、探针和重组质粒的计算机辅助设计开始,开发了三种定量实时聚合酶链反应(qPCR),以靶向这三种微孢子虫的RNA聚合酶II亚基B1(RPB1)基因。包括蜜蜂研磨、DNA纯化和qPCR在内的完整方法在蜜蜂(Apis mellifera)匀浆中得到了验证。通过计算机模拟和使用几种类型的蜜蜂样本进行体外实验评估了特异性。检测限估计为每只蜜蜂4 log拷贝。校正了一个小的系统方法偏差,以实现每只蜜蜂高达10 log拷贝的准确定量。在熊蜂(Bombus terrestris)和壁蜂(Osmia bicornis)匀浆中,在5至10 log拷贝/只蜜蜂的范围内也验证了方法的准确性。这些经过验证的qPCR方法为微孢子虫病的诊断以及管理和野生蜜蜂中寄生虫生态动态的研究开辟了前景。

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