Transcriptome-scale super-resolved imaging in tissues by RNA seqFISH+

Creators: Eng, Chee-Huat Linus; Lawson, Michael; Zhu, Qian; Dries, Ruben; Koulena, Noushin; Takei, Yodai; Yun, Jina; Cronin, Christopher; Karp, Christoph; Yuan, Guo-Cheng; Cai, Long

Abstract

Imaging the transcriptome in situ with high accuracy has been a major challenge in single-cell biology, which is particularly hindered by the limits of optical resolution and the density of transcripts in single cells. Here we demonstrate an evolution of sequential fluorescence in situ hybridization (seqFISH+). We show that seqFISH+ can image mRNAs for 10,000 genes in single cells—with high accuracy and sub-diffraction-limit resolution—in the cortex, subventricular zone and olfactory bulb of mouse brain, using a standard confocal microscope. The transcriptome-level profiling of seqFISH+ allows unbiased identification of cell classes and their spatial organization in tissues. In addition, seqFISH+ reveals subcellular mRNA localization patterns in cells and ligand–receptor pairs across neighbouring cells. This technology demonstrates the ability to generate spatial cell atlases and to perform discovery-driven studies of biological processes in situ.

Additional Information

© 2019 Springer Nature Publishing AG. Received 05 November 2018; Accepted 27 February 2019; Published 25 March 2019. Code availability: The custom written scripts used in this study are available at https://github.com/CaiGroup/seqFISH-PLUS. Data availability: RNA-seq data were obtained from GEO accession number GSE98674. RNA SPOTs data were obtained from a previous study. Source data from this study are available at https://github.com/CaiGroup/seqFISH-PLUS. All data obtained during this study are available from the corresponding author upon reasonable request. We thank L. Sanchez-Guardado from the Lois laboratory and the Thanos laboratory for providing mouse samples; S. Schindler for sectioning the tissue slices; J. Thomassie for help with data analysis; S. Shah for help with image analysis and input on the manuscript; K. Frieda for advice on the manuscript and help with making figures; and M. Thomsons, S. Chen and C. Lois for discussions. This project is funded by NIH TR01 OD024686, NIH HubMAP UG3HL145609, Paul G. Allen Frontiers Foundation Discovery Center and a Chan-Zuckerberg Initiative pilot grant. Author Contributions: C.-H.L.E. and L.C. conceived the idea and designed experiments. C.-H.L.E. performed all the experiments. M.L. performed image analysis. C.-H.L.E., M.L., Q.Z., R.D. and L.C. performed data analysis. L.C. and G.-C.Y. supervised the analysis process. C.-H.L.E. and N.K. performed cell segmentation and generated the primary probes. Y.T. designed the readout probes. C.-H.L.E., Y.T. and J.Y. validated the readout probes. C.C. and C.K. built the automated fluidic delivery system. C.-H.L.E., M.L, Q.Z., R.D. and Y.T. provided input for L.C. when writing the manuscript. L.C. supervised all aspects of the project. Competing interests: C.-H.L.E and L.C. filed a patent on the pseudocolour-encoding scheme in seqFISH+.

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Resource type: Journal Article
Publisher: Nature Publishing Group
Published in: Nature, 568(7751), 235-239, ISSN: 0028-0836.