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从不同水凝胶包埋的间充质干细胞中一步提取RNA用于定量逆转录-聚合酶链反应分析。

Single-Step RNA Extraction from Different Hydrogel-Embedded Mesenchymal Stem Cells for Quantitative Reverse Transcription-Polymerase Chain Reaction Analysis.

作者信息

Köster Natascha, Schmiermund Alexandra, Grubelnig Stefan, Leber Jasmin, Ehlicke Franziska, Czermak Peter, Salzig Denise

机构信息

1 Institute of Bioprocess Engineering and Pharmaceutical Technology, University of Applied Sciences Mittelhessen , Giessen, Germany .

2 Department of Chemical Engineering, Kansas State University , Manhattan, Kansas.

出版信息

Tissue Eng Part C Methods. 2016 Jun;22(6):552-60. doi: 10.1089/ten.TEC.2015.0362. Epub 2016 May 23.

DOI:10.1089/ten.TEC.2015.0362
PMID:27094052
Abstract

For many tissue engineering applications, cells such as human mesenchymal stem cells (hMSCs) must be embedded in hydrogels. The analysis of embedded hMSCs requires RNA extraction, but common extraction procedures often produce low yields and/or poor quality RNA. We systematically investigated four homogenization methods combined with eight RNA extraction protocols for hMSCs embedded in three common hydrogel types (alginate, agarose, and gelatin). We found for all three hydrogel types that using liquid nitrogen or a rotor-stator produced low RNA yields, whereas using a microhomogenizer or enzymatic/chemical hydrogel digestion achieved better yields regardless of which extraction protocol was subsequently applied. The hot phenol extraction protocol generally achieved the highest A260 values (representing up to 40.8 μg RNA per 10(6) cells), but the cetyltrimethylammonium bromide (CTAB) method produced RNA of better quality, with A260/A280 and A260/A230 ratios and UV spectra similar to the pure RNA control. The RNA produced by this method was also suitable as a template for endpoint and quantitative reverse transcription-PCR (qRT-PCR), achieving low Ct values of ∼20. The prudent choice of hydrogel homogenization and RNA extraction methods can ensure the preparation of high-quality RNA that generates reliable endpoint and quantitative RT-PCR data. We therefore propose a universal method that is suitable for the extraction of RNA from cells embedded in all three hydrogel types commonly used for tissue engineering.

摘要

对于许多组织工程应用而言,诸如人间充质干细胞(hMSCs)之类的细胞必须嵌入水凝胶中。对嵌入的hMSCs进行分析需要提取RNA,但常见的提取方法往往产量较低和/或RNA质量较差。我们系统地研究了四种匀浆方法与八种RNA提取方案,用于提取嵌入三种常见水凝胶类型(海藻酸盐、琼脂糖和明胶)中的hMSCs的RNA。我们发现,对于所有三种水凝胶类型,使用液氮或转子-定子匀浆器会导致RNA产量较低,而使用微匀浆器或酶促/化学水凝胶消化法无论随后应用哪种提取方案都能获得更好的产量。热酚提取方案通常能获得最高的A260值(每10^6个细胞可达40.8μg RNA),但十六烷基三甲基溴化铵(CTAB)法产生的RNA质量更好,其A260/A280和A260/A230比值以及紫外光谱与纯RNA对照相似。该方法产生的RNA也适合作为终点和定量逆转录PCR(qRT-PCR)的模板,Ct值低至约20。谨慎选择水凝胶匀浆和RNA提取方法可确保制备出高质量的RNA,从而产生可靠的终点和定量RT-PCR数据。因此,我们提出了一种通用方法,适用于从嵌入组织工程常用的所有三种水凝胶类型中的细胞中提取RNA。

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