Considerations for Reverse Transcriptase: Single-cell RNA Sequencing

Authors
Johannes W. Bagnoli 1, Christoph Ziegenhain , Aleksandar Janjic , Lucas E. Wange, Beate Vieth, Swati Parekh, Johanna Geuder, Ines Hellmann 1 & Wolfgang Enard
09-26-2018 HSW 1057
12:00pm
PST
Categories
New Technologies
Speaker
Abstract

Single-cell RNA sequencing (scRNA-seq) has emerged as a central genome-wide method to characterize cellular identities and processes. Consequently, improving its sensitivity, flexibility, and cost-efficiency can advance many research questions. Among the flexible platebased methods, single-cell RNA barcoding and sequencing (SCRB-seq) is highly sensitive and efficient. Here, we systematically evaluate experimental conditions of this protocol and find that adding polyethylene glycol considerably increases sensitivity by enhancing cDNA synthesis. Furthermore, using Terra polymerase increases efficiency due to a more even cDNA amplification that requires less sequencing of libraries. We combined these and other improvements to develop a scRNA-seq library protocol we call molecular crowding SCRB-seq
(mcSCRB-seq), which we show to be one of the most sensitive, efficient, and flexible scRNAseq methods to date.