Multi-omics profiling of mouse gastrulation at single-cell resolution

Argelaguet, Ricard; Clark, Stephen J.; Mohammed, Hisham; Stapel, L. Carine; Krueger, Christel; Kapourani, Chantriolnt-Andreas; Imaz-Rosshandler, Iván; Lohoff, Tim; Xiang, Yunlong; Hanna, Courtney W.; Smallwood, Sébastien A.; Ibarra-Soria, Ximena; Buettner, Florian; Sanguinetti, Guido; Xie, Wei; Krueger, Felix; Göttgens, Berthold; Rugg‐Gunn, Peter J.; Kelsey, Gavin; Dean, Wendy; Nichols, Jennifer; Stegle, Oliver; Marioni, John C.; Reik, Wolf

doi:10.1038/s41586-019-1825-8

Cited by 356 publications

(460 citation statements)

References 57 publications

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“…One module covered only DNA methylation. This module comprised cells from different cell types at E7.5, again highlighting that while the transcriptional signatures of different cell types differ at that stage, the promoter methylation profile of the different germ layers is still quite similar 27 . Overall, these results demonstrate that Monet can be applied and lead to insights in diverse biological scenarios.…”

Section: Simulated Datasetsmentioning

confidence: 92%

“…Finally, we applied Monet to single-cell data. Argelaguet et al recently developed scNMT, a method that measured gene expression, DNA methylation and DNA accessibility at single cell resolution, and applied it to mouse embryos at embryonic days 4.5-7.5 27 . We applied Monet to the gene expression and promoter methylation data of 619 single cells (Fig 5b, 5c).…”

Section: Simulated Datasetsmentioning

confidence: 99%

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MONET: Multi-omic patient module detection by omic selection

Rappoport

Safra

Shamir

2020

Preprint

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Recent advances in experimental biology allow creation of datasets where several genome-wide data types (called omics) are measured per sample. Integrative analysis of multi-omic datasets in general, and clustering of samples in such datasets specifically, can improve our understanding of biological processes and discover different disease subtypes. In this work we present Monet (Multi Omic clustering by Non-Exhaustive Types), which presents a unique approach to multi-omic clustering. Monet discovers modules of similar samples, such that each module is allowed to have a clustering structure for only a subset of the omics. This approach differs from most extant multi-omic clustering algorithms, which assume a common structure across all omics, and from several recent algorithms that model distinct cluster structures using Bayesian statistics. We tested Monet extensively on simulated data, on an image dataset, and on ten multi-omic cancer datasets from TCGA. Our analysis shows that Monet compares favorably with other multi-omic clustering methods. We demonstrate Monet's biological and clinical relevance by analyzing its results for Ovarian Serous Cystadenocarcinoma. We also show that Monet is robust to missing data, can cluster genes in multi-omic dataset, and reveal modules of cell types in single-cell multi-omic data. Our work shows that Monet is a valuable tool that can provide complementary results to those provided by extant algorithms for multi-omic analysis.

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Section: Simulated Datasetsmentioning

confidence: 92%

Section: Simulated Datasetsmentioning

confidence: 99%

MONET: Multi-omic patient module detection by omic selection

Rappoport

Safra

Shamir

2020

Preprint

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“…7). Although part of the populations from E6.5 and E7.5 has some overlap in the integrated data based on MAPLE input, this outcome is due to the biological nature of the data, as it is observed in all data modalities including gene expression (Argelaguet et al 2019) .…”

Section: Predicted Gene Activity Enhances Integration With Scrna-seq mentioning

confidence: 99%

“…Single-cell multi-omics studies suggest significant correlation (both positive and negative) between expression and gene body methylation for only a limited number of genes Angermueller, Clark, et al 2016) . As a repressive marker, mean promoter methylation is significantly negatively correlated with gene expression only in a fraction of promoters (Angermueller, Clark, et al 2016;Clark et al 2018;Argelaguet et al 2019) in individual cells. As a result, there is not a straightforward approach for inferring gene activity levels using single-cell DNA methylation datasets.…”

Section: Introductionmentioning

confidence: 99%

Predictive modeling of single-cell DNA methylome data enhances integration with transcriptome data

Tan

2020

Preprint

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Despite rapid advances in single-cell DNA methylation profiling methods, computational tools for data analysis are lagging far behind. A number of tasks, including cell type calling and integration with transcriptome data, requires the construction of a robust gene activity matrix as the prerequisite but challenging task. The advent of multi-omics data enables measurement of both DNA methylation and gene expression for the same single cells. Although such data is rather sparse, they are sufficient to train supervised models that capture the complex relationship between DNA methylation and gene expression and predict gene activities at single-cell level. Here, we present MAPLE (Methylome Association by Predictive Linkage to Expression), a computational framework that learns the association between DNA methylation and expression using both gene-and cell-dependent statistical features. Using multiple datasets generated with different experimental protocols, we show that using predicted gene activity values significantly improves several analysis tasks, including clustering, cell type identification and integration with transcriptome data. With the rapid accumulation of single-cell epigenomics data, MAPLE provides a general framework for integrating such data with transcriptome data.

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“…The transition from HSC to frank lineages is multi-faceted, and therefore reliance on a single set of features is unlikely to reveal the full extent of molecular changes. We anticipate that future single cell multi-omics approaches extracting several epigenomic features such as DNA methylation, and chromatin accessibility (Argelaguet et al 2019) while simultaneously coupled to lineage tracing might yield molecular signatures that more accurately correspond to, temporally precede and hence empower the transition in potency. The scATAC-seq itself provides an elegant solution by utilizing reads mapped to the mitochondrial genome to clonally track the lineages while simultaneously reading out the chromatin features within the same cell (Ludwig et al 2019;Xu et al 2019).…”

Section: Intriguingly Concurrent Accessibility Of Binding Motifs Of mentioning

confidence: 99%

Concurrent stem- and lineage-affiliated chromatin programs precede hematopoietic lineage restriction

Safi

Dhapola

Warsi

et al. 2020

Preprint

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word count: 150 Manuscript word count: 6952 Nr of references: 61 SUMMARY The emerging notion of hematopoietic stem-and progenitor cells (HSPCs) as a low-primed cloud without sharply demarcated gene expression programs raises the question on how cellular fate options emerge, and at which stem-like stage lineage priming is initiated. Here we investigated single-cell chromatin accessibility of Lineage -, cKit + , Sca1 + (LSK) HSPCs spanning the early differentiation landscape. Application of a signal-processing algorithm to detect transition points corresponding to massive alterations in accessibility of 571 transcription factor-motifs revealed a population of LSK FMS-like tyrosine kinase 3(Flt3) int CD9 high cells that concurrently display stemlike and lineage-affiliated chromatin signatures pointing to a simultaneous gain of both Lympho-Myeloid and Megakaryocyte-Erythroid programs. Molecularly and functionally, these cells position between stem cells and committed progenitors, display multi-lineage capacity in vitro and in vivo, but lack self-renewal activity. This integrative molecular analysis resolves the heterogeneity of cells along hematopoietic differentiation and permits investigation of chromatin-mediated transition between multipotency and lineage restriction.

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Multi-omics profiling of mouse gastrulation at single-cell resolution

Cited by 356 publications

References 57 publications

MONET: Multi-omic patient module detection by omic selection

MONET: Multi-omic patient module detection by omic selection

Predictive modeling of single-cell DNA methylome data enhances integration with transcriptome data

Concurrent stem- and lineage-affiliated chromatin programs precede hematopoietic lineage restriction

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