Project description:This SuperSeries is composed of the following subset Series: GSE33076: Linearity of amplification between gene expression values and the amounts of RNA in a retina cell group GSE33085: Transcriptome analysis of adult retina cell types GSE33088: Developmental time-course of adult cell-type-specific retina genes of amacrine cells Refer to individual Series

Project description:Brain circuits are assembled from a large variety of morphologically and functionally diverse cell types. It is not known how the intermingled cell types of individual brain regions differ in their expressed genomes. Here we describe an atlas of cell type transcriptomes of the adult retina. We found that each adult cell type expresses a specific set of genes, including a unique set of transcription factors, forming a “barcode” for cell identity. Cell type transcriptomes carry enough information to categorize cells into corresponding morphological classes and types. Surprisingly, several barcode genes are eye disease-associated genes that we demonstrate to be specifically expressed not only in photoreceptors but also in particular retinal circuit elements such as inhibitory neurons as well as in retinal microglia. Our data suggest that distinct cell types of individual brain regions are characterized by marked differences in their expressed genomes. To obtain insight into the developmental time course of adult cell type-specific gene expression, we followed gene expression in one amacrine cell group, Arc cells, for 20 postnatal days (P) starting at P1. Qualitative analysis of the expression time-course of cell type-specific genes revealed four patterns: increasing, decreasing or constant expression from P1 to P20, or a biphasic time-course (constant and increasing) with a switch at P9-P10. At this latter time point, bipolar cells begin to form synapses with amacrine and ganglion cells and the retina becomes light responsive. Pairwise correlations across the transcriptomes measured on each day exposed two major clusters, from P1 to P9 and from P10 to P20, which also suggested a transcriptional switch during the transition from P9 to P10. Thus, most adult cell type-specific genes are also expressed during development but at levels different to those in the adult. We performed gene expression analysis of one amacrine cell group, Arc, from P0 to P20 and for Starburst amacrine cells for the time point P3 and P18. All experiments were performed in biological triplicates. 1 retina was used for each time point and each sample of the biological triplicate.

Project description:Brain circuits are assembled from a large variety of morphologically and functionally diverse cell types. It is not known how the intermingled cell types of individual brain regions differ in their expressed genomes. Here we describe an atlas of cell type transcriptomes of the adult retina. We found that each adult cell type expresses a specific set of genes, including a unique set of transcription factors, forming a “barcode” for cell identity. Cell type transcriptomes carry enough information to categorize cells into corresponding morphological classes and types. Surprisingly, several barcode genes are eye disease-associated genes that we demonstrate to be specifically expressed not only in photoreceptors but also in particular retinal circuit elements such as inhibitory neurons as well as in retinal microglia. Our data suggest that distinct cell types of individual brain regions are characterized by marked differences in their expressed genomes. To test whether amplifications were linear, we examined the relationship between gene expression values and the amounts of RNA in a cell group. We pooled together two retinas from the Chrnb4-GFP (cone) and six retinas from the ChAT-Cre × Rosa26-LSL-RFP (starburst amacrine cell) mouse lines. Five mixtures of GFP:RFP cells (“titration mixtures”) were then FACS-sorted with the following cone-starburst compositions: 0:200, 50:150, 100:100, 150:50 and 200:0. The total number of cells in each mixture was 200. Five mixtures from different mice were sorted 3 times to give biological triplicates. Next 20 genes with the highest specificity ratio for cones and another 20 for starburst cells were chosen and linear curves were fitted to the data pairs of expression value:cone number or expression value:starburst cell number. For both cone- and starburst-enriched genes, gene expression values increased linearly with an increase in the number of cones or starburst cells in the mixtures. The linear correlation coefficients were independent of the extent to which genes were expressed in the pure cone and starburst cell groups. This suggests that A practical use of the finding that amplification is linear is to separate the transcriptome of a cell group that contains cells from different types into its cell-type components. Assuming, for example, a cell group (Group A) containing a mixture of two cell types, Type 1 and Type 2, as well as a futher cell group (Group B) containing only Type 1 (Supplementary Figure 10). We wish to determine the transcriptome of Type 2 but we have no cell group (Group C) that contains Type 2 only. Or more generally, assume a cell group (Group A) containing a mixture of cell types, Type 1, Type 2…Type N, as well as a further cell group (Group B) containing only Type 1. We wish to determine the mixed transcriptome of Group C that contains Type 2….Type N, without Type 1. This separation of cell-type transcriptomes is useful for two reasons. First, ~80% of mouse retinal cells are rods30 and it is expected that transcripts from rods will be present in the solution after retina dissociation, leading to rod contamination of the transcriptome of each cell group. We wished to eliminate rod contamination. Second, we found that cones in some mouse lines are labeled together with a type of amacrine cell and we needed to determine the amacrine cell transcriptome alone. Due to linearity, the following procedure can be used to separate Type 1 from the rest of the cell types in a mixture (Group A). A set of cell type-specific genes for Type 1 is determined. This may be known a priori or from the dataset itself. The ratio of the expression value in Group A to the expression value in Group B is calculated for each Type 1-specific gene. The mean ratio is the estimate of the number of Type 1 cells in Group A. Next, the transcriptome (the expression values of all genes, which we treat as a vector) of Group B is multiplied by the mean ratio and the result is subtracted from the transcriptome of Group A. All negative numbers are then removed from this “unmixed” transcriptome by setting them to zero followed by normalization with the Group B (Type 1) transcriptome using quantile normalization. The quantile normalized “unmixed” transcriptome forms the prediction of the transcriptome of Group C. Note that if Group A contains only two cell types, Type 1 and Type 2, then the transcriptome of Group C is the transcriptome of Type 2 cells. We have demonstrated and quantitatively evaluated this procedure for the cone:starburst mixtures described above. In addition to the titration mixtures, we also made three “test mixtures” consisting the following cone:starburst cell numbers: 157:43, 75:125 and 183:17. Cones served as the Type 1 cells and starburst cells as Type 2. In our experiment, we had one pure cone group (200:0) and one pure starburst cell group (0:200) as well as six mixtures (50:150, 100:100, 150:50, 157:43, 75:125 and 183:17. First, we predicted the mixture composition using different numbers of cone-specific genes. Since we chose 20 cone-specific genes, the use of single genes presents 20 possible ways of predicting the number of cones in the mixture. Using two genes for the prediction provides 190 possible ways of predicting the number of cones in the mixture. The number of possible predictions when using k genes is: 20!/((20-k)! k!). When more than one gene is used for the prediction, the prediction is the mean of the individual gene-based predictions. Error was calculated as the mean of the absolute values of the deviation from the cone cell numbers in the mixtures. The mean and standard deviation of the prediction error decrease with the use of increasing number of genes. With 10 genes used for the prediction, for example, the prediction error will be approximately 12±3% (s.d.), regardless of which 10 genes are chosen, as long as they are cell type-specific. We pooled together two adult retinas from the Chrnb4-GFP (cone) and six adult retinas from the ChAT-Cre × Rosa26-LSL-RFP (starburst amacrine cell) mouse lines. Five mixtures of GFP:RFP cells (“titration mixtures”) were then FACS-sorted with the following cone-starburst compositions: ChAT.200: cone 0, ChAT.150: cone 50, ChAT.100: cone 100, ChAT.50 : cone 150, ChAT.0: cone 200. The total number of cells in each mixture was 200. Five mixtures from different mice were sorted 3 times to give biological triplicates (indicated by _1, _2, _3). X1, X2 and X3 stand for the following ratios: X1: ChAT.43 : cone 157, ChAT.125 : cone 75, ChAT.17 : cone 183. Arc represents as internal batch control to compare with other gene arrays within our dataset.

Project description:To comprehensively profile cell types in the human retina, we performed single cell RNA-sequencing on 20,009 cells obtained post-mortem from three donors and compiled a reference transcriptome atlas. Using unsupervised clustering analysis, we identified 18 transcriptionally distinct clusters representing all known retinal cells: rod photoreceptors, cone photoreceptors, Müller glia cells, bipolar cells, amacrine cells, retinal ganglion cells, horizontal cells, retinal astrocytes and microglia.

Project description:In order to provide multi-omic resolution to human retinal organoid developmental dynamics, we performed scRNA-seq and scATAC-seq from the same cell suspension across a time course (6-46 weeks) of human retinal organoid development. This data set covers all the retinal organoid scRNA-seq data generated from IMR90 and409B2-iCas9 cell lines.

Project description:To begin to understand how TFs regulate retinal cell type identity in human tissues, we established a pooled loss of function (LOF) experiment based on the CROP-seq protocol in developed retinal organoids. We targeted five TFs (OTX2, NRL, CRX, VSX2, and PAX6) that are important for retinal development and expressed dynamically over the organoid developmental time course.

Project description:The human brain has changed dramatically since humans diverged from our closest living relatives, chimpanzees and the other great apes. However, the genetic and developmental programs underlying this divergence are not fully understood. Here, we generate single-nucleus RNA-seq data of human, chimpanzee and macaque adult prefrontal cortex. Spatial information is obtained by isolating nuclei from sequential sections sliced from basal to apical positions. By comparing transcriptome of different cell types in the three species, we map human-specific expression in adult prefrontal cortex. By comparing to single cell RNA-seq data of cerebral organoids of the same species, we find developmental differences that persist into adulthood, as well as cell state-specific changes that occur exclusively in the adult brain.

Project description:Studies correlating genetic variation to gene expression facilitate the interpretation of common human phenotypes and disease. As functional variants may be operating in a tissue-dependent manner, we performed gene expression profiling and association with genetic variants (SNPs) on three cell types of 85 individuals. After excluding 10 outlier individuals detected through principal component analysis, we detected cell type-specific genetic effects, with 69 - 80% of regulatory variants operating in a cell type-specific manner and identified multiple eQTLs per gene, unique or shared among cell types and positively correlated with the number of transcripts per gene. Cell type specific eQTLs were found at larger distances from genes and lower effect size similar to known enhancers. These data suggest that the complete regulatory variant repertoire can only be uncovered in the context of cell type specificity. Total RNA was extracted from fibroblasts, LCLs, and T-cells of the 85 unrelated individuals of the GenCord. Two one-quarter scale Message Amp II reactions (Ambion, Foster City, CA) were performed for each RNA extraction with 200 ng of total RNA. 1.5 μg of cRNA was hybridized to a commercial whole-genome expression array (WG-6 v3 Expression BeadChip, Illumina) to quantify transcript abundance. In total there were two technical replicates (labeling and hybridization) for each RNA sample.

Project description:Retinal organoids samples that derived from human embryonic stem cells were analyzed by single-cell RNA sequencing. Two samples at different differentiation stages (day57 and day 171) were included in this study for cell type comparison.

Project description:Long non-coding (lnc)RNAs play key roles in many biological processes. Elucidating the function of lncRNAs in cell type specification during organ development requires knowledge about their expression in individual progenitor types rather than in whole tissues. To achieve this during cortical development, we used a dual-reporter mouse line to isolate coexisting proliferating neural stem cells, differentiating neurogenic progenitors and newborn neurons and assessed the expression of lncRNAs by paired-end, high-throughput sequencing. We identified 379 genomic loci encoding novel lncRNAs and performed a comprehensive assessment of cell-specific expression patterns for all, annotated and novel, lncRNAs described to date. Our study provides a powerful new resource for studying these elusive transcripts during stem cell commitment and neurogenesis. mRNA profiles of Proliferating Progenitors, Differentiating Progenitors and Neurons from lateral cortex of E14.5 mouse embryos. Each cell type in three biological replicates.