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A microRNA isolation method from clinical samples

机译:从临床样品中提取microRNA的方法

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摘要

>Introduction: microRNAs (miRNAs) are considered to be novel molecular biomakers that could be exploited in the diagnosis and treatment of different diseases. The present study aimed to develop an efficient miRNA isolation method from different clinical specimens. >Methods: Total RNAs were isolated by Trizol reagent followed by precipitation of the large RNAs with potassium acetate (KCH3COOH), polyethylene glycol (PEG) 4000 and 6000, and lithium chloride (LiCl). Then, small RNAs were enriched and recovered from the supernatants by applying a combination of LiCl and ethanol. The efficiency of the method was evaluated through the quality, quantity, and integrity of the recovered RNAs using the A260/280 absorbance ratio, reverse transcription PCR (RT-PCR), and quantitative real-time PCR (q-PCR). >Results: Comparison of different RNA isolation methods based on the precipitation of DNA and large RNAs, high miRNA recovery and PCR efficiency revealed that applying potassium acetate with final precipitation of small RNAs using 2.5 M LiCl plus ethanol can provide high yield and quality small RNAs that can be exploited for clinical purposes. >Conclusion: The current isolation method can be applied for most clinical samples including cells, formalin-fixed and paraffin-embedded (FFPE) tissues and even body fluids with a wide applicability in molecular biology investigations.
机译:>简介:microRNA(miRNA)被认为是可以用于诊断和治疗不同疾病的新型分子生物制造商。本研究旨在开发一种从不同临床标本中分离出有效miRNA的方法。 >方法:用Trizol试剂分离总RNA,然后用乙酸钾(KCH3COOH),聚乙二醇(PEG)4000和6000和氯化锂(LiCl)沉淀大RNA。然后,通过应用LiCl和乙醇的组合,从上清液中富集并回收小RNA。使用A260 / 280吸光度比,逆转录PCR(RT-PCR)和定量实时PCR(q-PCR),通过回收RNA的质量,数量和完整性评估了该方法的效率。 >结果:基于DNA和大RNA沉淀,高miRNA回收率和PCR效率的不同RNA分离方法的比较表明,使用乙酸钾和使用2.5 M LiCl加乙醇最终沉淀小RNA可以提供可用于临床目的的高产量和高质量的小RNA。 >结论:目前的分离方法可用于大多数临床样品,包括细胞,福尔马林固定和石蜡包埋(FFPE)组织,甚至体液,在分子生物学研究中具有广泛的适用性。

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