Integration of Single-Cell Transcriptomics With a High Throughput Functional Screening Assay to Resolve Cell Type, Growth Kinetics, and Stemness Heterogeneity Within the Comma-1D Cell Line

Arpit Dave; Erin Nekritz; Daniel Charytonowicz; Michael Beaumont; Melissa Smith; Kristin Beaumont; Jose Silva; Robert Sebra

doi:10.3389/fgene.2022.894597

Integration of Single-Cell Transcriptomics With a High Throughput Functional Screening Assay to Resolve Cell Type, Growth Kinetics, and Stemness Heterogeneity Within the Comma-1D Cell Line

Front Genet. 2022 Jun 14:13:894597. doi: 10.3389/fgene.2022.894597. eCollection 2022.

Authors

Arpit Dave¹, Erin Nekritz², Daniel Charytonowicz¹, Michael Beaumont^{1

3}, Melissa Smith⁴, Kristin Beaumont^{1

3}, Jose Silva², Robert Sebra^{1

3

5

6

7}

Affiliations

¹ Department of Genetics and Genomic Sciences, Icahn School of Medicine at Mount Sinai, New York, NY, United States.
² Department of Pathology, Icahn School of Medicine at Mount Sinai Hospital, New York, NY, United States.
³ Icahn Genomics Institute, Icahn School of Medicine at Mount Sinai, New York, NY, United States.
⁴ Department of Biochemistry and Molecular Genetics, University of Louisville, Louisville, KY, United States.
⁵ Black Family Stem Cell Institute, Icahn School of Medicine at Mount Sinai, New York, NY, United States.
⁶ Center for Advanced Genomics Technology, Icahn School of Medicine at Mount Sinai, New York, NY, United States.
⁷ Sema4, A Mount Sinai Venture, Stamford, CT, United States.

Abstract

Cell lines are one of the most frequently implemented model systems in life sciences research as they provide reproducible high throughput testing. Differentiation of cell cultures varies by line and, in some cases, can result in functional modifications within a population. Although research is increasingly dependent on these in vitro model systems, the heterogeneity within cell lines has not been thoroughly investigated. Here, we have leveraged high throughput single-cell assays to investigate the Comma-1D mouse cell line that is known to differentiate in culture. Using scRNASeq and custom single-cell phenotype assays, we resolve the clonal heterogeneity within the referenced cell line on the genomic and functional level. We performed a cohesive analysis of the transcriptome of 5,195 sequenced cells, of which 85.3% of the total reads successfully mapped to the mm10-3.0.0 reference genome. Across multiple gene expression analysis pipelines, both luminal and myoepithelial lineages were observed. Deep differential gene expression analysis revealed eight subclusters identified as luminal progenitor, luminal differentiated, myoepithelial differentiated, and fibroblast subpopulations-suggesting functional clustering within each lineage. Gene expression of published mammary stem cell (MaSC) markers Epcam, Cd49f, and Sca-1 was detected across the population, with 116 (2.23%) sequenced cells expressing all three markers. To gain insight into functional heterogeneity, cells with patterned MaSC marker expression were isolated and phenotypically investigated through a custom single-cell high throughput assay. The comparison of growth kinetics demonstrates functional heterogeneity within each cell cluster while also illustrating significant limitations in current cell isolation methods. We outlined the upstream use of our novel automated cell identification platform-to be used prior to single-cell culture-for reduced cell stress and improved rare cell identification and capture. Through compounding single-cell pipelines, we better reveal the heterogeneity within Comma-1D to identify subpopulations with specific functional characteristics.

Keywords: Comma-1D; Functional Assay; High throughput; Mammary Development; Mouse Cell Line; scRNASeq.

Grants and funding

P30 AR079200/AR/NIAMS NIH HHS/United States