High-throughput RNA isoform sequencing using programmable cDNA concatenation

Author:

Al’Khafaji Aziz M.ORCID,Smith Jonathan T.ORCID,Garimella Kiran VORCID,Babadi Mehrtash,Sade-Feldman MosheORCID,Gatzen Michael,Sarkizova Siranush,Schwartz Marc A.ORCID,Popic Victoria,Blaum Emily M.,Day Allyson,Costello Maura,Bowers Tera,Gabriel Stacey,Banks Eric,Philippakis Anthony A.,Boland Genevieve M.,Blainey Paul C.ORCID,Hacohen Nir

Abstract

AbstractAlternative splicing is a core biological process that enables profound and essential diversification of gene function. Short-read RNA sequencing approaches fail to resolve RNA isoforms and therefore primarily enable gene expression measurements - an isoform unaware representation of the transcriptome. Conversely, full-length RNA sequencing using long-read technologies are able to capture complete transcript isoforms, but their utility is deeply constrained due to throughput limitations. Here, we introduce MAS-ISO-seq, a technique for programmably concatenating cDNAs into single molecules optimal for long-read sequencing, boosting the throughput >15 fold to nearly 40 million cDNA reads per run on the Sequel IIe sequencer. We validated unambiguous isoform assignment with MAS-ISO-seq using a synthetic RNA isoform library and applied this approach to single-cell RNA sequencing of tumor-infiltrating T cells. Results demonstrated a >30 fold boosted discovery of differentially spliced genes and robust cell clustering, as well as canonical PTPRC splicing patterns across T cell subpopulations and the concerted expression of the associated hnRNPLL splicing factor. Methods such as MAS-ISO-seq will drive discovery of novel isoforms and the transition from gene expression to transcript isoform expression analyses.

Publisher

Cold Spring Harbor Laboratory

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