对保留关键形态凭证的自然种群的基于rna的研究取样摇尾虫的注释

M. Krosch, L. M. Bryant
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引用次数: 3

摘要

转录组学方法在淡水生态学中的迅速应用,已经产生了大量关于生物在分子水平上与其环境相互作用方式的数据。通常,这类研究要么集中在群落水平,因此不需要物种鉴定,要么集中在已知物种身份的实验室菌株或大型自然种群,容易识别的分类群。对摇尾拟鱼来说,由于其体型较小,而且往往需要耗费大量时间对溪流材料进行二次分类,并准备形态证明以确定物种诊断,因此将这些技术应用于自然种群仍然存在障碍。这些程序限制了在这些生物体中维持RNA数量和质量的能力,因为RNA降解迅速,基因表达在生物体中可以迅速改变;从而限制了这些分类群在转录组学研究中的纳入。在这里,我们证明了这些限制是可以克服的,并概述了一种收集、分类和保存摇蚊幼虫的优化方案,该方案能够保留形态凭证和RNA,用于随后的转录组学目的。通过确保在收集后4小时内完成分选和凭证制备,并始终保持样品低温,我们成功地保留了所有标本的RNA和形态凭证。虽然在具体方法上没有规定,但我们预计本文将有助于促进水生环境变化对摇尾鱼基因表达亚致死影响的转录组学研究。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
A note on sampling chironomids for RNA-based studies of natural populations that retains critical morphological vouchers
The rapid uptake of transcriptomic approaches in freshwater ecology has seen a wealth of data produced concerning the ways in which organisms interact with their environment on a molecular level. Typically, such studies focus either at the community level and so don’t require species identifications, or on laboratory strains of known species identity or natural populations of large, easily identifiable taxa. For chironomids, impediments still exist for applying these technologies to natural populations because they are small-bodied and often require time-consuming secondary sorting of stream material and morphological voucher preparation to confirm species diagnosis. These procedures limit the ability to maintain RNA quantity and quality in such organisms because RNA degrades rapidly and gene expression can be altered rapidly in organisms; thereby limiting the inclusion of such taxa in transcriptomic studies. Here, we demonstrate that these limitations can be overcome and outline an optimised protocol for collecting, sorting and preserving chironomid larvae that enables retention of both morphological vouchers and RNA for subsequent transcriptomics purposes. By ensuring that sorting and voucher preparation are completed within <4 hours after collection and that samples are kept cold at all times, we successfully retained both RNA and morphological vouchers from all specimens. Although not prescriptive in specific methodology, we anticipate that this paper will assist in promoting transcriptomic investigations of the sublethal impact on chironomid gene expression of changes to aquatic environments.
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