Getting Started with RNA Sequencing (RNA Seq) – The Basics

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Getting Started with RNA Sequencing (RNA Seq) – The Basics RNA sequencing or RNA seq is the process of obtaining the sequence information of a sample’s transcriptome, , including mRNA, rRNA, and tRNA, through Next Generation Sequencing (NGS). RNA sequencing provides information about gene expression in a given cell (in the case of single cell RNA sequencing) or sample set of cells (in the case of bulk-level molecular analysis). This information is important in many areas of research where gene expression is important, such as oncology, including instances of tumor heterogeneity, or virology, including RNA viruses such as coronavirus or HIV. There are several steps involved in RNA Sequencing: Sample Collection, Transport, Storage Before beginning any RNA seq experiment, the target sample needs to be carefully extracted, transported, and stored. Often a DNA RNA shield is used to facilitate both sample transport and storage at ambient temperature. CellCover is a DNA RNA shield with a non-toxic formulation that works for fast “one step” stabilizing of biomolecules in life science research. It is a gentle tool for RNA fixation, maintaining the status of expression in human and animal cells and solid tissues, including tumors and cultured cells (adherent, suspension, spheroids). DNA, RNA and proteins are all protected. Calling to mind the computer science expression “garbage in, garbage out” the collection, transport, and storage of samples are perhaps the most important of all. The entire downstream process relies on the integrity of the samples – without proper RNA fixation with a DNA RNA shield, all downstream sequencing and analysis can be compromised. RNA Isolation After RNA fixation with a DNA RNA shield such as CellCover, samples can then be processed for RNA isolation through extraction and purification. There are several kits on the market that achieve this in a relatively simple and straightforward way with centrifugation and a combination of company-specific buffers. The RNA sample can be left as-is, or can undergo selection and/or depletion, filtering it for the specific downstream analysis intended. Selection of particular RNA species (such


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