Jones Laura, Sanders Christopher, England Marion, Cameron Mary, Carpenter Simon
The Pirbright Institute, Ash Road, Woking, Surrey, GU24 0NF, England.
London School of Hygiene and Tropical Medicine, Keppel Street, London, WC1E 7HT, England.
Biol Proced Online. 2024 Jun 18;26(1):17. doi: 10.1186/s12575-024-00246-1.
Culex pipiens L. is a principal vector of zoonotic arboviruses in Europe, acting in both an amplification role in enzootic transmission between avian hosts and as a bridge vector between avian hosts and mammals. The species consists of two forms which are indistinguishable using morphological methods but possess varying ecological and physiological traits that influence their vector capacity. In this study we validate methods that can be used to extract trace DNA from single pupal exuviae of Cx. pipiens for use in molecular speciation of samples. These DNA extraction methods are compared using measurement of the total yield and successful identification using a real-time polymerase chain reaction (PCR) assay.
Genomic DNA was initially extracted from colony-derived individuals using an ethanol precipitation method, two commercially available DNA extraction kits: DNeasy® Blood & Tissue Kit (Qiagen, UK) and Wizard® SV Genomic DNA Purification System (Promega, UK) and a direct real-time PCR method. Time elapsed between eclosion and processing of pupae significantly influenced Cx. pipiens form identification as nucleic acid concentration and PCR amplification success decreased with increased time elapsed. Real-time PCR amplification success, however, was not shown to vary significantly between the three extraction methods, with all methods successfully identifying all samples, but the direct real-time PCR method achieved a lesser amplification success rate of 70% (n = 20 for each treatment). More variable results were produced when field-derived exuviae were used, with no significant difference in real-time PCR amplification success found across the four methods and a lower overall rate of successful identification of 55-80%.
This study shows that both colony and field derived Cx. pipiens pupal exuviae can be a useful non-invasive source of trace DNA permitting accurate biotype differentiation for at least twenty-four hours post-eclosion. The significance and utility of this technique in ecological and behavioural studies of Cx. pipiens is discussed and recommendations made for use according to experimental scenario.
尖音库蚊是欧洲人畜共患虫媒病毒的主要传播媒介,在鸟类宿主间的动物源性传播中起扩增作用,并作为鸟类宿主与哺乳动物之间的桥梁媒介。该物种由两种形态组成,用形态学方法无法区分,但具有不同的生态和生理特征,影响其传播能力。在本研究中,我们验证了可用于从尖音库蚊单个蛹蜕中提取微量DNA以用于样本分子分类的方法。使用总产量测量和实时聚合酶链反应(PCR)测定法成功鉴定对这些DNA提取方法进行了比较。
最初使用乙醇沉淀法、两种市售DNA提取试剂盒:DNeasy®血液和组织试剂盒(Qiagen,英国)和Wizard®SV基因组DNA纯化系统(Promega,英国)以及直接实时PCR方法从群体来源的个体中提取基因组DNA。羽化与蛹处理之间的时间间隔显著影响尖音库蚊形态的鉴定,因为核酸浓度和PCR扩增成功率随时间间隔增加而降低。然而,实时PCR扩增成功率在三种提取方法之间未显示出显著差异,所有方法均成功鉴定了所有样本,但直接实时PCR方法的扩增成功率较低,为70%(每种处理n = 20)。当使用野外来源的蜕时,产生的结果更具变异性,四种方法的实时PCR扩增成功率没有显著差异,总体成功鉴定率较低,为55 - 80%。
本研究表明,群体和野外来源的尖音库蚊蛹蜕都可以是有用的微量DNA非侵入性来源,允许在羽化后至少二十四小时内进行准确的生物型分化。讨论了该技术在尖音库蚊生态和行为研究中的意义和实用性,并根据实验场景提出了使用建议。
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