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The Utah Protocol for Postmortem Eye Phenotyping and Molecular Biochemical Analysis.犹他州死后眼部表型分析和分子生化分析协议
Invest Ophthalmol Vis Sci. 2019 Mar 1;60(4):1204-1212. doi: 10.1167/iovs.18-24254.
2
Molecular Classification and Comparative Taxonomics of Foveal and Peripheral Cells in Primate Retina.灵长类动物视网膜中央凹和周边细胞的分子分类和比较分类学。
Cell. 2019 Feb 21;176(5):1222-1237.e22. doi: 10.1016/j.cell.2019.01.004. Epub 2019 Jan 31.
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Reproducibility and staging of 3D human retinal organoids across multiple pluripotent stem cell lines.在多个多能干细胞系中重现和分期 3D 人视网膜类器官。
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Deconstructing Retinal Organoids: Single Cell RNA-Seq Reveals the Cellular Components of Human Pluripotent Stem Cell-Derived Retina.解析视网膜类器官:单细胞 RNA 测序揭示人多能干细胞源性视网膜的细胞成分。
Stem Cells. 2019 May;37(5):593-598. doi: 10.1002/stem.2963. Epub 2019 Jan 12.
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Thyroid hormone signaling specifies cone subtypes in human retinal organoids.甲状腺激素信号指定人类视网膜类器官中的锥形细胞亚型。
Science. 2018 Oct 12;362(6411). doi: 10.1126/science.aau6348.
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Generation of Retinal Organoids with Mature Rods and Cones from Urine-Derived Human Induced Pluripotent Stem Cells.从尿液来源的人类诱导多能干细胞生成具有成熟视杆细胞和视锥细胞的视网膜类器官。
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Human-Induced Pluripotent Stem Cells Generate Light Responsive Retinal Organoids with Variable and Nutrient-Dependent Efficiency.人诱导多能干细胞产生具有可变和营养依赖性效率的光响应视网膜类器官。
Stem Cells. 2018 Oct;36(10):1535-1551. doi: 10.1002/stem.2883. Epub 2018 Aug 13.
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Regenerating Eye Tissues to Preserve and Restore Vision.再生眼部组织以保存和恢复视力。
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RNA Biology in Retinal Development and Disease.视网膜发育与疾病中的 RNA 生物学。
Trends Genet. 2018 May;34(5):341-351. doi: 10.1016/j.tig.2018.01.002. Epub 2018 Jan 31.
10
Molecular Anatomy of the Developing Human Retina.发育中的人类视网膜的分子解剖学
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生成富含视锥细胞的人视网膜类器官及其转录组特征分析和功能验证。

Generation, transcriptome profiling, and functional validation of cone-rich human retinal organoids.

机构信息

Human Genome Sequencing Center, Department of Molecular and Human Genetics, Baylor College of Medicine, Houston, TX 77030.

Department of Ophthalmology and Visual Sciences, Albert Einstein College of Medicine, Bronx, NY 10461.

出版信息

Proc Natl Acad Sci U S A. 2019 May 28;116(22):10824-10833. doi: 10.1073/pnas.1901572116. Epub 2019 May 9.

DOI:10.1073/pnas.1901572116
PMID:31072937
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC6561190/
Abstract

Rod and cone photoreceptors are light-sensing cells in the human retina. Rods are dominant in the peripheral retina, whereas cones are enriched in the macula, which is responsible for central vision and visual acuity. Macular degenerations affect vision the most and are currently incurable. Here we report the generation, transcriptome profiling, and functional validation of cone-rich human retinal organoids differentiated from hESCs using an improved retinal differentiation system. Induced by extracellular matrix, aggregates of hESCs formed single-lumen cysts composed of epithelial cells with anterior neuroectodermal/ectodermal fates, including retinal cell fate. Then, the cysts were -passaged, attached to culture surface, and grew, forming colonies in which retinal progenitor cell patches were found. Following gentle cell detachment, retinal progenitor cells self-assembled into retinal epithelium-retinal organoid-that differentiated into stratified cone-rich retinal tissue in agitated cultures. Electron microscopy revealed differentiating outer segments of photoreceptor cells. Bulk RNA-sequencing profiling of time-course retinal organoids demonstrated that retinal differentiation in vitro recapitulated in vivo retinogenesis in temporal expression of cell differentiation markers and retinal disease genes, as well as in mRNA alternative splicing. Single-cell RNA-sequencing profiling of 8-mo retinal organoids identified cone and rod cell clusters and confirmed the cone enrichment initially revealed by quantitative microscopy. Notably, cones from retinal organoids and human macula had similar single-cell transcriptomes, and so did rods. Cones in retinal organoids exhibited electrophysiological functions. Collectively, we have established cone-rich retinal organoids and a reference of transcriptomes that are valuable resources for retinal studies.

摘要

杆状和锥状光感受器是人类视网膜中的光感受器细胞。杆状细胞在周边视网膜中占优势,而锥状细胞在黄斑中丰富,黄斑负责中央视觉和视力敏锐度。黄斑变性对视力的影响最大,目前无法治愈。在这里,我们报告了使用改进的视网膜分化系统,从 hESC 分化出富含锥体细胞的人视网膜类器官的生成、转录组分析和功能验证。在细胞外基质的诱导下,hESC 聚集形成由具有前神经外胚层/外胚层命运的上皮细胞组成的单腔囊泡,包括视网膜细胞命运。然后,将囊泡传代、附着在培养表面上并生长,形成含有视网膜祖细胞斑的集落。在温和的细胞分离后,视网膜祖细胞自我组装成视网膜上皮细胞-视网膜类器官,在搅动培养中分化为分层的富含锥体细胞的视网膜组织。电子显微镜显示了正在分化的光感受器细胞的外节。对时间过程视网膜类器官的批量 RNA 测序分析表明,体外视网膜分化在细胞分化标志物和视网膜疾病基因的时空表达以及 mRNA 选择性剪接方面再现了体内视网膜发生。对 8 个月龄的视网膜类器官的单细胞 RNA 测序分析鉴定了锥状细胞和杆状细胞簇,并证实了定量显微镜最初揭示的锥状细胞富集。来自视网膜类器官和人黄斑的锥体具有相似的单细胞转录组,杆状细胞也是如此。视网膜类器官中的锥体表现出电生理功能。总之,我们已经建立了富含锥体的视网膜类器官和转录组参考资源,这对于视网膜研究具有重要价值。