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提高从基质胶培养物中分离RNA完整性的方法。

Method for improved integrity of RNA isolated from Matrigel cultures.

作者信息

Da Silva Lais, Bray Julie K, Bulut Gamze, Jiang Jinmai, Schmittgen Thomas D

机构信息

Department of Pharmaceutics, College of Pharmacy, University of Florida, Gainesville, FL USA.

Department of Pathology, Immunology, and Laboratory Medicine, College of Medicine, University of Florida, Gainesville, FL USA.

出版信息

MethodsX. 2020 Jun 20;7:100966. doi: 10.1016/j.mex.2020.100966. eCollection 2020.

Abstract

Matrigel is a commercially available substrate that is derived from the extracellular matrix. Matrigel is widely used in cell culture experiments such as the transdifferentiation of primary pancreatic acini to ductal epithelial-like cells. Difficulty arises during gene expression analysis for cells cultured on Matrigel because residual RNA in the Matrigel will not only contribute to the poor integrity of RNA isolated from Matrigel cultures, but also will impact the gene expression data. We report here a simple method of removing Matrigel from primary cultures of human or mouse pancreatic acini. Following the experiment, the cultures are placed on wet ice to liquefy the Matrigel. The cell and Matrigel mixture is then centrifuged at low speed to separate the pancreatic cells from the Matrigel solution that resides in the supernatant. RNA isolated from the pelleted cells has high integrity and may be readily used for gene expression analysis such as quantitative reverse transcription PCR.

摘要

基质胶是一种可从细胞外基质中提取的商品化底物。基质胶广泛应用于细胞培养实验,比如原代胰腺腺泡向导管上皮样细胞的转分化。在对培养于基质胶上的细胞进行基因表达分析时会遇到困难,因为基质胶中的残留RNA不仅会导致从基质胶培养物中分离出的RNA完整性差,还会影响基因表达数据。我们在此报告一种从人或小鼠胰腺腺泡原代培养物中去除基质胶的简单方法。实验结束后,将培养物置于湿冰上以使基质胶液化。然后将细胞与基质胶的混合物低速离心,以将胰腺细胞与上清液中的基质胶溶液分离。从沉淀细胞中分离出的RNA具有高完整性,可很容易地用于基因表达分析,如定量逆转录PCR。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/75fe/7327238/c5cef9688a7c/fx1.jpg

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