Optimization of RNA Extraction Protocol for Rat Skeletal Muscle Samples

S. Felipe, Christina Pacheco, J. E. R. Martins, Raquel Martins de Freitas, Paulo Elesson Oliveira, S. V. D. Mendes, J. Alves, V. Ceccatto
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Abstract

Aims: The present study aimed to stablish and characterize an optimized protocol conformation to obtain adequate RNA quality from rodents skeletal muscle samples for sequencing studies. Place and Duration of Study: The in vivo experiments and analyses were performed in the Laboratory of Biochemistry and Gene Expression – LABIEX of the Superior Institute of Biomedical Science – ISCB from the State University of Ceará - UECE. Between 2017-2020. Methodology: Were used 23 samples from male Wistar rat skeletal muscle, specifically from soleus muscle. Total RNA extraction was performed using the classic TRIzol® method and commercial kit, merging steps from both. Capillary electrophoresis in the Bioanalyzer platform was used for RNA quality evaluation. Results: (C) Analyzes of adapted protocol RNA concentration, RIN and rate 28S/18S showed satisfactory results. 28S/18S Ribosomal bands appear well defined, without small traces, which indicates RNA with high integrity and without contamination of genomic DNA. Conclusion: Obtained RNA quality and integrity data satisfied the exigencies for posterior RNA-seq.
大鼠骨骼肌RNA提取工艺的优化
目的:本研究旨在建立和表征一种优化的方案构象,以从啮齿动物骨骼肌样本中获得足够的RNA质量,用于测序研究。研究地点和时间:体内实验和分析在ceear州立大学生物医学科学高级研究所生物化学和基因表达实验室(LABIEX)进行。在2017 - 2020之间。方法:选取23例雄性Wistar大鼠骨骼肌,特别是比目鱼肌。总RNA提取使用经典的TRIzol®方法和商业试剂盒,合并两者的步骤。生物分析仪平台毛细管电泳用于RNA质量评价。结果:(C)对适应方案的RNA浓度、RIN和28S/18S率进行分析,结果令人满意。28S/18S核糖体条带清晰,没有小的痕迹,表明RNA具有高完整性,没有基因组DNA的污染。结论:获得的RNA质量和完整性数据满足后路RNA测序的要求。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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