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      The Mouse Retinal Organoid Trisection Recipe: Efficient Generation of 3D Retinal Tissue from Mouse Embryonic Stem Cells.

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          Abstract

          The introduction of stem cell-based technologies for the derivation of three-dimensional retinal tissues, the so-called retinal organoids, offers many new possibilities for vision research: Organoids facilitate studies on retinal development and in vitro retinal disease modeling, as well as being valuable for drug testing. Further, retinal organoids also provide an unlimited cell source for cell replacement therapies. Here, we describe our protocol for efficiently differentiating large, stratified retinal organoids from mouse embryonic stem cells: unbiased manual dissection of the developing retinal organoid at an early stage into three evenly sized neuroepithelial portions (trisection step) doubles the yield of high-quality organoids. We also describe some useful applications of the protocol, e.g., generation of rod- or cone-enriched retinal organoids, AAV transfection, and cell birth dating. In addition, we provide details of how to process retinal organoids for single organoid gene expression analysis, immunohistochemistry, and electron microscopy.

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          Author and article information

          Journal
          Methods Mol. Biol.
          Methods in molecular biology (Clifton, N.J.)
          Springer Science and Business Media LLC
          1940-6029
          1064-3745
          2019
          : 1834
          Affiliations
          [1 ] German Center for Neurodegenerative Diseases Dresden (DZNE), Dresden, Germany.
          [2 ] Technische Universität Dresden, Center for Molecular and Cellular Bioengineering (CMCB), Center for Regenerative Therapies Dresden (CRTD), Dresden, Germany.
          [3 ] German Center for Neurodegenerative Diseases Dresden (DZNE), Dresden, Germany. mike.karl@dzne.de.
          [4 ] Technische Universität Dresden, Center for Molecular and Cellular Bioengineering (CMCB), Center for Regenerative Therapies Dresden (CRTD), Dresden, Germany. mike.karl@dzne.de.
          Article
          10.1007/978-1-4939-8669-9_9
          30324441
          bf6368f6-164a-446c-8c3d-d32b023ce948
          History

          DAPT,Cone photoreceptors,(Single) Organoid QPCR studies,Mouse retinal organoids (MRO),Electron microscopy,Photoreceptor-enriched organoids,Immunohistochemistry,AAV infection,Cell birth dating,RNA isolation,Mouse embryonic stem cell (mESC)

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