RNA extraction for RNA sequencing of archival renal tissues

核糖核酸 RNA提取 生物 核酸 分子生物学 DNA 生物化学 基因
作者
Lea Landolt,Hans‐Peter Marti,Christian Beisland,Arnar Flatberg,Øystein Eikrem
出处
期刊:Scandinavian Journal of Clinical & Laboratory Investigation [Taylor & Francis]
卷期号:76 (5): 426-434 被引量:59
标识
DOI:10.1080/00365513.2016.1177660
摘要

BACKGROUND: Next generation sequencing (NGS) and especially ribonucleic acid (RNA) sequencing is a powerful tool to acquire insights into molecular disease mechanisms. Therefore, it is of interest to optimize methods for RNA extraction from archival, formalin fixed and paraffin embedded (FFPE) tissues. This is challenging due to RNA degradation and chemical modifications. The aim of this study was to find the most appropriate method to extract RNA from FFPE renal tissue to enable NGS. METHOD: We evaluated seven commercially available RNA extraction kits: High Pure FFPE RNA Isolation (Roche), ExpressArt Clear FFPE RNAready (Amsbio), miRNeasy FFPE, RNeasy FFPE (Qiagen), PureLink FFPE Total RNA (Invitrogen), RecoverAll Total Nucleic Acid Isolation (Ambion) and Absolutely RNA FFPE Kit (Agilent). RNA was obtained from tissue blocks of two healthy, male Wistar rats and from normal renal tissue of patients undergoing nephrectomy. Yield and quality of RNA extracted from rat whole kidney sections, human kidney core biopsies and laser capture microdissected (LCM) glomerular cross-sections were assessed: Analyses of RNA quantity were performed using NanoDrop and Qubit. RNA quality is reflected by DV200 values (% of RNA fragments >200 nucleotides) utilizing the Agilent 2100 BioAnalyzer. RNA of human LCM samples was subsequently sequenced using the Illumina TruSeq(®) RNA Access Library Preparation Kit. CONCLUSION: Total RNA can be extracted from archival renal biopsies in sufficient quality and quantity from one human kidney biopsy section and from around 100 LCM glomerular cross-sections to enable successful RNA library preparation and sequencing using commercially available RNA extraction kits.

科研通智能强力驱动
Strongly Powered by AbleSci AI
科研通是完全免费的文献互助平台,具备全网最快的应助速度,最高的求助完成率。 对每一个文献求助,科研通都将尽心尽力,给求助人一个满意的交代。
实时播报
传奇3应助xy采纳,获得10
刚刚
共享精神应助创新小达人采纳,获得10
刚刚
刚刚
Lucas应助认真的山兰采纳,获得10
1秒前
领导范儿应助远方采纳,获得10
1秒前
学术废物发布了新的文献求助10
1秒前
长zyzy完成签到,获得积分10
2秒前
谨慎咖啡豆关注了科研通微信公众号
2秒前
2秒前
优美的SCI发布了新的文献求助10
2秒前
2秒前
香蕉觅云应助悬停之翼采纳,获得10
3秒前
小柠发布了新的文献求助10
4秒前
4秒前
5秒前
sanvva举报PziPzi求助涉嫌违规
5秒前
Lusteri发布了新的文献求助10
5秒前
5秒前
5秒前
zyt完成签到,获得积分20
5秒前
赘婿应助唠叨的以冬采纳,获得10
5秒前
wanci应助唠叨的以冬采纳,获得10
6秒前
6秒前
Owen应助唠叨的以冬采纳,获得10
6秒前
6秒前
6秒前
6秒前
6秒前
科研通AI2S应助唠叨的以冬采纳,获得10
6秒前
HEYATIAN完成签到 ,获得积分10
7秒前
7秒前
天天快乐应助唠叨的以冬采纳,获得10
7秒前
7秒前
7秒前
小lai发布了新的文献求助10
8秒前
小二郎应助colatea采纳,获得10
8秒前
科研通AI6.2应助HEHONGBIN采纳,获得150
8秒前
9秒前
刘欣发布了新的文献求助10
9秒前
9秒前
高分求助中
(应助此贴封号)【重要!!请各用户(尤其是新用户)详细阅读】【科研通的精品贴汇总】 10000
48V Low-voltage Power Distribution Network (PDN) Architecture Industry Report, 2024 800
Fundamentals of Pharmaceutical and Biologics Regulations: A Global Perspective, Second Edition 700
Matrix Methods in Data Mining and Pattern Recognition Second Edition 610
适配Micro-LED色转换的高兼容性量子点负性光刻胶制备与工艺研究 500
Direct and Iterative Linear System Solvers 500
Vander's Renal Physiology第10版 500
热门求助领域 (近24小时)
化学 材料科学 医学 生物 纳米技术 工程类 有机化学 化学工程 生物化学 计算机科学 内科学 物理 复合材料 催化作用 细胞生物学 无机化学 光电子学 物理化学 电极 基因
热门帖子
关注 科研通微信公众号,转发送积分 7309068
求助须知:如何正确求助?哪些是违规求助? 8926290
关于积分的说明 18917861
捐赠科研通 6971294
什么是DOI,文献DOI怎么找? 3212929
关于科研通互助平台的介绍 2381391
邀请新用户注册赠送积分活动 2190698