QIAseq FastSelect is a novel method for ribosomal RNA removal that involves neutralization of the rRNA during the reverse transcription reaction as opposed to the traditional hybridization-capture or hybridization-enzymatic digestion methods – which are commonly used for this purpose. The QIAseq FastSelect method ensures increased ribosomal RNA removal compared to other methods – and only requires a few pipetting steps and a 14-minute incubation. Following the QIAseq FastSelect protocol, the resulting cDNA can be used for RNA-seq library construction using both the traditional dUTP method or the QIAseq Quick-seq method of selective, strand-specific ligation.

Join us for a discussion on how researchers are using QIAseq FastSelect technology with fragmented and high-quality RNA for both short and long-read RNA-seq analysis. Find out how QIAseq FastSelect can speed up and streamline your RNA-seq workflow and allow you to increase the unique reads you generate so you can achieve deeper insights faster. We will also illustrate how QIAseq FastSelect ribosomal RNA removal technology is successfully used for bacterial, mammalian and mixed samples.

Speaker:
Samuel Rulli, Ph.D., Senior Global Product Manager, RNA Profiling, Genomics, QIAGEN

Details About the Webinar

Cost: Free

About the Speaker

59211b63-c5a1-40ef-b141-4cf6a40b7124 Dr. Samuel Rulli, Ph.D.
Senior Global Product Manager, RNA Profiling

Samuel Rulli is a Global Product Manager for RNA-seq technologies and applications at QIAGEN focusing on gene expression applications using whole transcriptome and targeted RNA panel workflows. Dr. Rulli received his Ph.D. in 2002 from Tulane University studying the gastric proton pump, and performed post-doctoral research at Johns Hopkins University and the National Cancer Institute in Frederick, MD. Trained as a molecular biologist, Dr. Rulli has worked on different assay detection technologies for gene expression and nucleic acid analysis.

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