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A method for extracting high-quality RNA from diverse plants for next-generation sequencing and gene expression analyses

机译:一种从多种植物中提取高质量RNA用于下一代测序和基因表达分析的方法

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摘要

• Premise of the study: To study gene expression in plants, high-quality RNA must be extracted in quantities sufficient for subsequent cDNA library construction. Field-based collections are often limited in quantity and quality of tissue and are typically preserved in RNAlater. Obtaining sufficient and high-quality yield from variously preserved samples is essential to studies of comparative biology. We present a protocol for the extraction of high-quality RNA from even the most recalcitrant plant tissues.• Methods and Results: Tissues from mosses, cycads, and angiosperm floral organs and leaves were preserved in RNAlater or frozen fresh at −80°C. Extractions were performed and quality was measured for yield and purity.• Conclusions: This protocol results in the extraction of high-quality RNA from a variety of plant tissues representing vascular and nonvascular plants. RNA was used for cDNA synthesis to generate libraries for next-generation sequencing and for expression studies using quantitative PCR (qPCR) and semiquantitative reverse transcription PCR (RT-PCR).
机译:•研究前提:要研究植物中的基因表达,必须提取足够数量的高质量RNA,以用于随后的cDNA文库构建。基于野外的采集通常在组织的数量和质量上受到限制,通常保存在RNAlater中。从各种保存的样品中获得足够的高质量产量对于比较生物学的研究至关重要。我们提出了从最顽强的植物组织中提取高质量RNA的方案。•方法和结果:来自苔藓,苏铁和被子植物花器官和叶片的组织被保存在RNAlater中或在-80°C冷冻新鲜。进行提取并测量产量和纯度的质量。•结论:该方案可从代表血管和非血管植物的多种植物组织中提取高质量RNA。 RNA用于cDNA合成,以生成用于下一代测序的文库,并使用定量PCR(qPCR)和半定量逆转录PCR(RT-PCR)进行表达研究。

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