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{"title":"RNA Fragmentation and Sequencing (RF-Seq): Cost-Effective, Time-Efficient, and High-Throughput 3′ mRNA Sequencing Library Construction in a Single Tube","authors":"Yaligara Veeranagouda, Anne Remaury, Jean-Claude Guillemot, Michel Didier","doi":"10.1002/cpmb.109","DOIUrl":null,"url":null,"abstract":"<p>Over the past decade, transcriptomic studies using next-generation sequencing (NGS)–based RNA sequencing (RNA-Seq) have greatly contributed to characterizing biochemical and physiological changes in cells and tissues across organisms and experimental conditions. Critical steps in RNA-Seq include the preparation of the sequencing library from extracted RNA. Currently, a large panoply of RNA-Seq kits are commercially available. In these kits, conversion of RNA into a sequencing library involves multiple steps, which are labor-intensive, and cost per sample for library preparation may limit routine use of RNA-Seq. Here we describe a simple method for RNA-Seq library construction, referred to as <span>R</span>NA <span>F</span>ragmentation and <span>Seq</span>uencing (RF-Seq). RF-Seq requires as little as 10 ng of total RNA and facilitates the sequencing of the 3′ end of mRNAs. RF-Seq involves the fragmentation of total RNA followed by reverse transcription in presence of the oligo(dT) primer/template switch oligonucleotide and a sample barcoding/enrichment within a single PCR tube/well. The sample barcoding/enrichment step provides more flexibility for individual sample handling. The use of just twenty orthogonal Illumina TruSeq HT barcoding primers facilitates the preparation of 96 uniquely labeled RF-Seq libraries in a single 96-well PCR plate. Twelve RF-Seq libraries can be prepared within 4 hr, with an approximate cost of $10/sample. We provide an example of using RF-Seq to measure gene expression upon activation of an innate immune pathway using STING activator in human blood cells, highlighting the potential usefulness of the proposed method in routine transcriptomic applications such as high-throughput drug screening and/or preclinical toxicity assays. © 2019 by John Wiley & Sons, Inc.</p><p><b>Basic Protocol</b>: RNA fragmentation and sequencing (RF-Seq): Cost-effective, time-efficient, and high-throughput 3′ mRNA sequencing library construction in a single tube</p>","PeriodicalId":10734,"journal":{"name":"Current Protocols in Molecular Biology","volume":"129 1","pages":""},"PeriodicalIF":0.0000,"publicationDate":"2019-10-09","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"https://sci-hub-pdf.com/10.1002/cpmb.109","citationCount":"2","resultStr":null,"platform":"Semanticscholar","paperid":null,"PeriodicalName":"Current Protocols in Molecular Biology","FirstCategoryId":"1085","ListUrlMain":"https://onlinelibrary.wiley.com/doi/10.1002/cpmb.109","RegionNum":0,"RegionCategory":null,"ArticlePicture":[],"TitleCN":null,"AbstractTextCN":null,"PMCID":null,"EPubDate":"","PubModel":"","JCR":"Q2","JCRName":"Biochemistry, Genetics and Molecular Biology","Score":null,"Total":0}
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Abstract
Over the past decade, transcriptomic studies using next-generation sequencing (NGS)–based RNA sequencing (RNA-Seq) have greatly contributed to characterizing biochemical and physiological changes in cells and tissues across organisms and experimental conditions. Critical steps in RNA-Seq include the preparation of the sequencing library from extracted RNA. Currently, a large panoply of RNA-Seq kits are commercially available. In these kits, conversion of RNA into a sequencing library involves multiple steps, which are labor-intensive, and cost per sample for library preparation may limit routine use of RNA-Seq. Here we describe a simple method for RNA-Seq library construction, referred to as R NA F ragmentation and Seq uencing (RF-Seq). RF-Seq requires as little as 10 ng of total RNA and facilitates the sequencing of the 3′ end of mRNAs. RF-Seq involves the fragmentation of total RNA followed by reverse transcription in presence of the oligo(dT) primer/template switch oligonucleotide and a sample barcoding/enrichment within a single PCR tube/well. The sample barcoding/enrichment step provides more flexibility for individual sample handling. The use of just twenty orthogonal Illumina TruSeq HT barcoding primers facilitates the preparation of 96 uniquely labeled RF-Seq libraries in a single 96-well PCR plate. Twelve RF-Seq libraries can be prepared within 4 hr, with an approximate cost of $10/sample. We provide an example of using RF-Seq to measure gene expression upon activation of an innate immune pathway using STING activator in human blood cells, highlighting the potential usefulness of the proposed method in routine transcriptomic applications such as high-throughput drug screening and/or preclinical toxicity assays. © 2019 by John Wiley & Sons, Inc.
Basic Protocol : RNA fragmentation and sequencing (RF-Seq): Cost-effective, time-efficient, and high-throughput 3′ mRNA sequencing library construction in a single tube
RNA片段化和测序(RF-Seq):成本效益,时间效率和高通量的3 ' mRNA测序文库建设在一个单管
在过去的十年中,使用基于下一代测序(NGS)的RNA测序(RNA- seq)的转录组学研究在生物和实验条件下对细胞和组织的生化和生理变化的表征做出了巨大贡献。RNA- seq的关键步骤包括从提取的RNA中制备测序文库。目前,市面上有大量的RNA-Seq试剂盒。在这些试剂盒中,将RNA转化为测序文库涉及多个步骤,这是劳动密集型的,并且每个样本文库制备的成本可能限制RNA- seq的常规使用。在这里,我们描述了一种简单的RNA- seq文库构建方法,称为RNA片段化和测序(RF-Seq)。RF-Seq只需要10 ng的总RNA,并有助于对mrna的3 '端进行测序。RF-Seq涉及总RNA的片段化,然后在寡核苷酸(dT)引物/模板开关寡核苷酸的存在下进行逆转录,并在单个PCR管/孔内进行样品条形码/富集。样品条形码/富集步骤为单个样品处理提供了更大的灵活性。仅使用20个正交Illumina TruSeq HT条形码引物,就可以在单个96孔PCR板上制备96个唯一标记的RF-Seq文库。12个RF-Seq文库可以在4小时内制备,每个样品的成本约为10美元。我们提供了一个使用RF-Seq来测量人类血细胞中使用STING激活剂激活先天免疫途径时基因表达的例子,强调了该方法在常规转录组学应用(如高通量药物筛选和/或临床前毒性分析)中的潜在有用性。©2019 by John Wiley &基本方案:RNA片段化和测序(RF-Seq):成本效益高,时间效率高,在单管中构建高通量3 ' mRNA测序文库
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