| Literature DB >> 33469025 |
Anoushka Joglekar1, Andrey Prjibelski2, Ahmed Mahfouz3,4,5, Paul Collier1, Susan Lin6,7, Anna Katharina Schlusche1, Jordan Marrocco8, Stephen R Williams9, Bettina Haase10, Ashley Hayes9, Jennifer G Chew9, Neil I Weisenfeld9, Man Ying Wong11, Alexander N Stein12, Simon A Hardwick1,13, Toby Hunt14, Qi Wang15, Christoph Dieterich15, Zachary Bent9, Olivier Fedrigo10, Steven A Sloan16, Davide Risso17, Erich D Jarvis10,18, Paul Flicek14, Wenjie Luo11, Geoffrey S Pitt6,7, Adam Frankish14, August B Smit19, M Elizabeth Ross1, Hagen U Tilgner20.
Abstract
Splicing varies across brain regions, but the single-cell resolution of regional variation is unclear. We present a single-cell investigation of differential isoform expression (DIE) between brain regions using single-cell long-read sequencing in mouse hippocampus and prefrontal cortex in 45 cell types at postnatal day 7 ( www.isoformAtlas.com ). Isoform tests for DIE show better performance than exon tests. We detect hundreds of DIE events traceable to cell types, often corresponding to functionally distinct protein isoforms. Mostly, one cell type is responsible for brain-region specific DIE. However, for fewer genes, multiple cell types influence DIE. Thus, regional identity can, although rarely, override cell-type specificity. Cell types indigenous to one anatomic structure display distinctive DIE, e.g. the choroid plexus epithelium manifests distinct transcription-start-site usage. Spatial transcriptomics and long-read sequencing yield a spatially resolved splicing map. Our methods quantify isoform expression with cell-type and spatial resolution and it contributes to further our understanding of how the brain integrates molecular and cellular complexity.Entities:
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Year: 2021 PMID: 33469025 PMCID: PMC7815907 DOI: 10.1038/s41467-020-20343-5
Source DB: PubMed Journal: Nat Commun ISSN: 2041-1723 Impact factor: 14.919