Integrity assay for messenger RNA in mouse and human brain samples and synaptosomal preparations

小鼠和人类大脑样本以及突触体制剂中信使 RNA 的完整性检测

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作者：Daina Bujanauskiene, Kajus Merkevicius, Ugne Kuliesiute, Jaroslav Denkovskij, Simonas Kutanovas, Gediminas Luksys, Saulius Rocka, Eiva Bernotiene, Urte Neniskyte

期刊：	iScience	影响因子：	4.600
时间：	2024	起止号：	2024 Jun 29;27(8):110419.
doi：	10.1016/j.isci.2024.110419	种属：	Mouse
研究方向：	信号转导

Abstract

Traditionally, RNA integrity evaluation is based on ribosomal RNAs (rRNAs). Nevertheless, gene expression studies are usually focused on protein-coding messenger RNAs (mRNAs). Here, we present an RT-qPCR-based assay, which estimates mRNA integrity by comparing the abundance of 3' and 5' mRNA fragments. The assay was validated using plasmids with cloned 3'- and 5'-ends of the cDNA reflecting different ratios of 3' and 5' cDNA amplicons in partially degraded RNA samples. The accuracy of integrity value was ensured by including primer efficiency. We used 5':3' assay to quantify RNA degradation in heat- and enzyme-degraded mouse and human brain tissue RNA as well as in clinical human brain RNA samples. In addition, the 5':3' assay was suitable for assessing mRNA integrity in synaptosomal preparations that lack rRNAs. We concluded that the 5':3' assay can be used as a reliable method to evaluate mRNA integrity in tissue and subcellular preparations.

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