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The spatial landscape of gene expression isoforms in tissue sections

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ABSTRACTIn situcapturing technologies add tissue context to gene expression data, with the potential of providing a greater understanding of complex biological systems. However, splicing variants and fulllength sequence heterogeneity cannot be characterized at spatial resolution with current transcriptome profiling methods. To that end, we introduce Spatial Isoform Transcriptomics (SiT), an explorative method for characterizing spatial isoform variation and sequence heterogeneity. We show in mouse brain how SIT can be used to profile isoform expression and sequence heterogeneity in different areas of the tissue. SiT reveals regional isoform switching ofPlp1gene between different layers of the olfactory bulb, and use of external single cell data allowed to nominate cell types expressing each isoform. Furthermore, SiT identifies differential isoform usage for several major genes implicated in brain function (Snap25, Bin1, Gnas) that we independently validated byin situsequencing. SiT also provides for the first time an in-depth A-to-I RNA editing map of the adult mouse brain. Data exploration can be performed through an online resource (https://www.isomics.eu), where isoform expression and RNA editing can be visualized in a spatial context.
Title: The spatial landscape of gene expression isoforms in tissue sections
Description:
ABSTRACTIn situcapturing technologies add tissue context to gene expression data, with the potential of providing a greater understanding of complex biological systems.
However, splicing variants and fulllength sequence heterogeneity cannot be characterized at spatial resolution with current transcriptome profiling methods.
To that end, we introduce Spatial Isoform Transcriptomics (SiT), an explorative method for characterizing spatial isoform variation and sequence heterogeneity.
We show in mouse brain how SIT can be used to profile isoform expression and sequence heterogeneity in different areas of the tissue.
SiT reveals regional isoform switching ofPlp1gene between different layers of the olfactory bulb, and use of external single cell data allowed to nominate cell types expressing each isoform.
Furthermore, SiT identifies differential isoform usage for several major genes implicated in brain function (Snap25, Bin1, Gnas) that we independently validated byin situsequencing.
SiT also provides for the first time an in-depth A-to-I RNA editing map of the adult mouse brain.
Data exploration can be performed through an online resource (https://www.
isomics.
eu), where isoform expression and RNA editing can be visualized in a spatial context.

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