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RNA-seq 样品制备试剂盒强烈影响产气菌的转录组谱。

RNA-seq Sample Preparation Kits Strongly Affect Transcriptome Profiles of a Gas-Fermenting Bacterium.

机构信息

ERA Chair in Gas Fermentation Technologies, Institute of Technology, University of Tartu, Tartu, Estonia.

Australian Institute for Bioengineering and Nanotechnology, The University of Queenslandgrid.1003.2, St. Lucia, Australia.

出版信息

Microbiol Spectr. 2022 Aug 31;10(4):e0230322. doi: 10.1128/spectrum.02303-22. Epub 2022 Jul 27.

Abstract

Transcriptome analysis via RNA sequencing (RNA-seq) has become a standard technique employed across various biological fields of study. The rapid adoption of the RNA-seq approach has been mediated, in part, by the development of different commercial RNA-seq library preparation kits compatible with standard next-generation sequencing (NGS) platforms. Generally, the essential steps of library preparation, such as rRNA depletion and first-strand cDNA synthesis, are tailored to a specific group of organisms (e.g., eukaryotes versus prokaryotes) or genomic GC content. Therefore, the selection of appropriate commercial products is of crucial importance to capture the transcriptome of interest as closely to the native state as possible without introduction of technical bias. However, researchers rarely have the resources and time to test various commercial RNA-seq kits for their samples. This work reports a side-by-side comparison of RNA-seq data from obtained using three commercial rRNA removal and strand-specific library construction products of NuGEN Technologies, Qiagen, and Zymo Research and assesses their performance relative to published data. While all three vendors advertise their products as suitable for prokaryotes, we found significant differences in their performance regarding rRNA removal, strand specificity, and most importantly, transcript abundance distribution profiles. Notably, RNA-seq data obtained with Qiagen products were most similar to published data and delivered the best results in terms of library strandedness and transcript abundance distribution range. Our results highlight the importance of finding appropriate organism-specific workflows and library preparation products for RNA-seq studies. RNA-seq is a powerful technique for transcriptome profiling while involving elaborate sample processing before library sequencing. We show that RNA-seq library preparation kits can strongly affect the outcome of an RNA-seq experiment. Although library preparation benefits from the availability of various commercial kits, choosing appropriate products for the specific samples can be challenging for new users or for users working with unconventional organisms. Evaluating the performance of different commercial products requires significant financial and time investments infeasible for most researchers. Therefore, users are often guided in their choice of kits by published data involving similar input samples. We conclude that important consideration should be given to selecting sample processing workflows for any given organism.

摘要

通过 RNA 测序(RNA-seq)进行转录组分析已成为各个生物研究领域的标准技术。RNA-seq 方法的快速采用部分归因于不同商业 RNA-seq 文库制备试剂盒的发展,这些试剂盒与标准的下一代测序(NGS)平台兼容。通常,文库制备的基本步骤,如 rRNA 耗尽和第一链 cDNA 合成,都针对特定的生物群体(例如真核生物与原核生物)或基因组 GC 含量进行了定制。因此,选择合适的商业产品对于尽可能接近自然状态地捕获感兴趣的转录组并避免引入技术偏差至关重要。然而,研究人员很少有资源和时间来为他们的样本测试各种商业 RNA-seq 试剂盒。本研究报告了使用 NuGEN Technologies、Qiagen 和 Zymo Research 的三种商业 rRNA 去除和链特异性文库构建产品获得的 RNA-seq 数据的并排比较,并评估了它们相对于已发表数据的性能。虽然所有三个供应商都宣称他们的产品适用于原核生物,但我们发现它们在 rRNA 去除、链特异性以及最重要的是转录本丰度分布谱方面的性能存在显著差异。值得注意的是,使用 Qiagen 产品获得的 RNA-seq 数据与已发表数据最为相似,并且在文库链特异性和转录本丰度分布范围方面的结果最佳。我们的研究结果强调了为 RNA-seq 研究找到合适的特定于生物体的工作流程和文库制备产品的重要性。RNA-seq 是一种强大的转录组分析技术,但在进行文库测序之前需要进行精细的样品处理。我们表明,RNA-seq 文库制备试剂盒会强烈影响 RNA-seq 实验的结果。尽管文库制备得益于各种商业试剂盒的可用性,但对于新用户或使用非常规生物体的用户来说,选择适合特定样本的产品可能具有挑战性。评估不同商业产品的性能需要大量的财务和时间投入,这对于大多数研究人员来说是不可行的。因此,用户通常会根据涉及类似输入样本的已发表数据来指导他们对试剂盒的选择。我们得出的结论是,对于任何给定的生物体,都应考虑选择合适的样品处理工作流程。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/cfac/9431689/6080e423735f/spectrum.02303-22-f001.jpg

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