Massively parallel digital transcriptional profiling of single cells

doi:10.1038/ncomms14049

. 2017 Jan 16:8:14049.

doi: 10.1038/ncomms14049.

Massively parallel digital transcriptional profiling of single cells

Grace X Y Zheng¹, Jessica M Terry¹, Phillip Belgrader¹, Paul Ryvkin¹, Zachary W Bent¹, Ryan Wilson¹, Solongo B Ziraldo¹, Tobias D Wheeler¹, Geoff P McDermott¹, Junjie Zhu¹, Mark T Gregory², Joe Shuga¹, Luz Montesclaros¹, Jason G Underwood^{1

3}, Donald A Masquelier¹, Stefanie Y Nishimura¹, Michael Schnall-Levin¹, Paul W Wyatt¹, Christopher M Hindson¹, Rajiv Bharadwaj¹, Alexander Wong¹, Kevin D Ness¹, Lan W Beppu⁴, H Joachim Deeg⁴, Christopher McFarland⁵, Keith R Loeb^{4

6}, William J Valente^{2

7

8}, Nolan G Ericson², Emily A Stevens⁴, Jerald P Radich⁴, Tarjei S Mikkelsen¹, Benjamin J Hindson¹, Jason H Bielas^{2

6

8

9}

Affiliations

¹ 10x Genomics Inc., Pleasanton, California, 94566, USA.
² Translational Research Program, Public Health Sciences Division, Fred Hutchinson Cancer Research Center, Seattle, Washington 98109, USA.
³ Department of Genome Sciences, University of Washington, Seattle, Washington 98195, USA.
⁴ Clinical Research Division, Fred Hutchinson Cancer Research Center, Seattle, Washington 98109, USA.
⁵ Seattle Cancer Care Alliance Clinical Immunogenetics Laboratory, Seattle, Washington 98109, USA.
⁶ Department of Pathology, University of Washington, Seattle, Washington 98195, USA.
⁷ Medical Scientist Training Program, University of Washington School of Medicine, Seattle, Washington 98195, USA.
⁸ Molecular and Cellular Biology Graduate Program, University of Washington, Seattle, Washington 98195, USA.
⁹ Human Biology Division, Fred Hutchinson Cancer Research Center, Seattle, Washington 98109, USA.

PMID: 28091601
PMCID: PMC5241818
DOI: 10.1038/ncomms14049

Massively parallel digital transcriptional profiling of single cells

Grace X Y Zheng et al. Nat Commun. 2017.

. 2017 Jan 16:8:14049.

doi: 10.1038/ncomms14049.

Authors

Affiliations

¹ 10x Genomics Inc., Pleasanton, California, 94566, USA.
² Translational Research Program, Public Health Sciences Division, Fred Hutchinson Cancer Research Center, Seattle, Washington 98109, USA.
³ Department of Genome Sciences, University of Washington, Seattle, Washington 98195, USA.
⁴ Clinical Research Division, Fred Hutchinson Cancer Research Center, Seattle, Washington 98109, USA.
⁵ Seattle Cancer Care Alliance Clinical Immunogenetics Laboratory, Seattle, Washington 98109, USA.
⁶ Department of Pathology, University of Washington, Seattle, Washington 98195, USA.
⁷ Medical Scientist Training Program, University of Washington School of Medicine, Seattle, Washington 98195, USA.
⁸ Molecular and Cellular Biology Graduate Program, University of Washington, Seattle, Washington 98195, USA.
⁹ Human Biology Division, Fred Hutchinson Cancer Research Center, Seattle, Washington 98109, USA.

PMID: 28091601
PMCID: PMC5241818
DOI: 10.1038/ncomms14049

Abstract

Characterizing the transcriptome of individual cells is fundamental to understanding complex biological systems. We describe a droplet-based system that enables 3' mRNA counting of tens of thousands of single cells per sample. Cell encapsulation, of up to 8 samples at a time, takes place in ∼6 min, with ∼50% cell capture efficiency. To demonstrate the system's technical performance, we collected transcriptome data from ∼250k single cells across 29 samples. We validated the sensitivity of the system and its ability to detect rare populations using cell lines and synthetic RNAs. We profiled 68k peripheral blood mononuclear cells to demonstrate the system's ability to characterize large immune populations. Finally, we used sequence variation in the transcriptome data to determine host and donor chimerism at single-cell resolution from bone marrow mononuclear cells isolated from transplant patients.

PubMed Disclaimer

Conflict of interest statement

G.X.Y.Z., J.M.T., P.B., P.R., Z.W.B., R.W., S.B.Z., T.D.W., J.J.Z., G.P.M., J.S., L.M., D.A.M., S.Y.N., M.S.L., P.W.W., C.M.H., R.B., A.W., K.D.N., T.S.M. and B.J.H. are employees of 10x Genomics.

Figures

**Figure 1. GemCode single-cell technology enables 3′ profiling of RNAs from thousands of single cells simultaneously.**
(a) scRNA-seq workflow on GemCode technology platform. Cells were combined with reagents in one channel of a microfluidic chip, and gel beads from another channel to form GEMs. RT takes place inside each GEM, after which cDNAs are pooled for amplification and library construction in bulk. (b) Gel beads loaded with primers and barcoded oligonucleotides are first mixed with cells and reagents, and subsequently mixed with oil-surfactant solution at a microfluidic junction. Single-cell GEMs are collected in the GEM outlet. (c) Percentage of GEMs containing 0 gel bead (N=0), 1 gel bead (N=1) and >1 gel bead (N>1). Data include five independent runs from multiple chip and gel bead lots over >70k GEMs for each run, n=5, mean±s.e.m. (d) Gel beads contain barcoded oligonucleotides consisting of Illumina adapters, 10x barcodes, UMIs and oligo dTs, which prime RT of polyadenylated RNAs. (e) Finished library molecules consist of Illumina adapters and sample indices, allowing pooling and sequencing of multiple libraries on a next-generation short read sequencer. (f) CellRanger pipeline workflow. Gene-barcode matrix (highlighted in green) is an output of the pipeline.

**Figure 2. Demonstration of technical performance of GemCode single-cell technology with cell lines and ERCC.**
(a) Scatter plot of human and mouse UMI counts detected in a mixture of 293T and 3T3 cells. Cell barcodes containing primarily mouse reads are colored in cyan and termed ‘Mouse only'; cell barcodes with primarily human reads are colored in red and termed ‘Human only'; and cell barcodes with significant mouse and human reads are coloured in grey and termed ‘Human:Mouse'. A multiplet rate of 1.6% was inferred. Median number of genes (b) and UMI counts (c) detected per cell in a mixture of 293T (red) and 3T3 (cyan) cells at different raw reads per cell. Data from three independent experiments were included, mean±s.e.m. (d) Mean observed UMI counts for each ERCC molecule is compared with expected number of ERCC molecules per GEM. A straight line was fitted to summarize the relationship. (e) Principal component analysis was performed on normalized scRNA-seq data of Jurkat and 293T cells mixed at four different ratios (100% 293T, 100% Jurkat, 50:50 293T:Jurkat and 1:99 293T and Jurkat). PC1 and PC3 are plotted, and each cell is colored by the normalized expression of *CD3D*. (f) SNV analysis was performed, and 293T- and Jurkat-enriched SNVs were plotted for each sample. A 3.1% multiplet rate was inferred from the 50:50 293T: Jurkat sample.

**Figure 3. Distinct populations can be detected in fresh 68k PBMCs.**
(a) Distribution of number of genes (left) and UMI counts (right) detected per 68k PBMCs. (b) tSNE projection of 68k PBMCs, where each cell is grouped into one of the 10 clusters (distinguished by their colours). Cluster number is indicated, with the percentage of cells in each cluster noted within parentheses. (c) Normalized expression (centred) of the top variable genes (rows) from each of 10 clusters (columns) is shown in a heatmap. Numbers at the top indicate cluster number in (b), with connecting lines indicating the hierarchical relationship between clusters. Representative markers from each cluster are shown on the right, and an inferred cluster assignment is shown on the left. (d–i) tSNE projection of 68k PBMCs, with each cell coloured based on their normalized expression of *CD3D*, *CD8A*, *NKG7*, *FCER1A*, *CD16* and *S100A8*. UMI normalization was performed by first dividing UMI counts by the total UMI counts in each cell, followed by multiplication with the median of the total UMI counts across cells. Then, we took the natural log of the UMI counts. Finally, each gene was normalized such that the mean signal for each gene is 0, and standard deviation is 1. (j) tSNE projection of 68k PBMCs, with each cell coloured based on their correlation-based assignment to a purified subpopulation of PBMCs. Subclusters within T cells are marked by dashed polygons. NK, natural killer cells; reg T, regulatory T cells.

**Figure 4. Genotype analysis of *in silico* and *in vitro* mixing of PBMCs.**
(a) Sensitivity versus percentage of minor population, where sensitivity is evaluated against the true labelling of *in silico* mixed PBMCs from Donors B and C. Red line indicates that the major population comes from Donor B PBMCs. Blue line indicates that the major population comes from Donor C PBMCs. (b) Positive predictive value (PPV) versus percentage of minor population, where PPV is evaluated against the true labelling of *in silico* mixed PBMCs from Donors B and C. Red line indicates that the major population comes from Donor B cells. Blue line indicates that the major population comes from Donor C cells. (c) Called mix fraction versus actual mix fraction in *in silico* mixing of PBMCs from Donors B and C. Fifty per cent actual mix fraction is correctly called, but omitted from the plot so that the rest of the ratios can be clearly displayed.

**Figure 5. Genotype and single-cell expression analysis of transplant BMMCs.**
(a) tSNE projection of scRNA-seq data from a healthy control, AML027 pre- and post-transplant samples (post-transplant sample is separated into host and donor) and AML035 pre- and post-transplant samples. tSNE projection was also performed on a second healthy control, but the plot is not included here as it is very similar to that of the first healthy control. Each cell is coloured by their classification, which is labelled next to the cell clusters. (b) Proportion of subpopulations in each sample.

See this image and copyright information in PMC

Cited by

Scalable, multimodal profiling of chromatin accessibility, gene expression and protein levels in single cells.
Mimitou EP, Lareau CA, Chen KY, Zorzetto-Fernandes AL, Hao Y, Takeshima Y, Luo W, Huang TS, Yeung BZ, Papalexi E, Thakore PI, Kibayashi T, Wing JB, Hata M, Satija R, Nazor KL, Sakaguchi S, Ludwig LS, Sankaran VG, Regev A, Smibert P. Mimitou EP, et al. Nat Biotechnol. 2021 Oct;39(10):1246-1258. doi: 10.1038/s41587-021-00927-2. Epub 2021 Jun 3. Nat Biotechnol. 2021. PMID: 34083792 Free PMC article.
The molecular landscape of neural differentiation in the developing Drosophila brain revealed by targeted scRNA-seq and multi-informatic analysis.
Michki NS, Li Y, Sanjasaz K, Zhao Y, Shen FY, Walker LA, Cao W, Lee CY, Cai D. Michki NS, et al. Cell Rep. 2021 Apr 27;35(4):109039. doi: 10.1016/j.celrep.2021.109039. Cell Rep. 2021. PMID: 33909998 Free PMC article.
Protocol to dissociate, process, and analyze the human lung tissue using single-cell RNA-seq.
Quintanal-Villalonga Á, Chan JM, Masilionis I, Gao VR, Xie Y, Allaj V, Chow A, Poirier JT, Pe'er D, Rudin CM, Mazutis L. Quintanal-Villalonga Á, et al. STAR Protoc. 2022 Oct 21;3(4):101776. doi: 10.1016/j.xpro.2022.101776. eCollection 2022 Dec 16. STAR Protoc. 2022. PMID: 36313536 Free PMC article.
Microglia Gravitate toward Amyloid Plaques Surrounded by Externalized Phosphatidylserine via TREM2.
Park JC, Han JW, Lee W, Kim J, Lee SE, Lee D, Choi H, Han J, Kang YJ, Diep YN, Cho H, Kang R, Yu WJ, Lee J, Choi M, Im SW, Kim JI, Mook-Jung I. Park JC, et al. Adv Sci (Weinh). 2024 Sep;11(34):e2400064. doi: 10.1002/advs.202400064. Epub 2024 Jul 9. Adv Sci (Weinh). 2024. PMID: 38981007 Free PMC article.
Analysis of alternative polyadenylation from single-cell RNA-seq using scDaPars reveals cell subpopulations invisible to gene expression.
Gao Y, Li L, Amos CI, Li W. Gao Y, et al. Genome Res. 2021 Oct;31(10):1856-1866. doi: 10.1101/gr.271346.120. Epub 2021 May 25. Genome Res. 2021. PMID: 34035046 Free PMC article.

See all "Cited by" articles

References

1. Shalek A. K. et al.. Single-cell transcriptomics reveals bimodality in expression and splicing in immune cells. Nature 498, 236–240 (2013). - PMC - PubMed
1. Wills Q. F. et al.. Single-cell gene expression analysis reveals genetic associations masked in whole-tissue experiments. Nat. Biotechnol. 31, 748–752 (2013). - PubMed
1. Liu S. & Trapnell C. Single-Cell Transcriptome Sequencing: Recent Advances and Remaining Challenges Vol. 5 F1000 Research (2016). - PMC - PubMed
1. Jaitin D. A. et al.. Massively parallel single-cell RNA-seq for marker-free decomposition of tissues into cell types. Science 343, 776–779 (2014). - PMC - PubMed
1. Pollen A. A. et al.. Low-coverage single-cell mRNA sequencing reveals cellular heterogeneity and activated signaling pathways in developing cerebral cortex. Nat. Biotechnol. 32, 1053–1058 (2014). - PMC - PubMed

Publication types

Actions

MeSH terms

Actions
Actions
Actions
Actions
Actions
Actions
Actions
Actions
Actions
Actions

Substances

Actions

Grants and funding

U10 CA180861/CA/NCI NIH HHS/United States

LinkOut - more resources

Full Text Sources
Other Literature Sources
Molecular Biology Databases
- Mouse Genome Informatics (MGI)
- NIAID Data Ecosystem - Find datasets on Infectious and Immune-mediated Diseases

[1] Shalek A. K. et al.. Single-cell transcriptomics reveals bimodality in expression and splicing in immune cells. Nature 498, 236–240 (2013). - PMC - PubMed

[2] Shalek A. K. et al.. Single-cell transcriptomics reveals bimodality in expression and splicing in immune cells. Nature 498, 236–240 (2013). - PMC - PubMed

[3] Wills Q. F. et al.. Single-cell gene expression analysis reveals genetic associations masked in whole-tissue experiments. Nat. Biotechnol. 31, 748–752 (2013). - PubMed

[4] Wills Q. F. et al.. Single-cell gene expression analysis reveals genetic associations masked in whole-tissue experiments. Nat. Biotechnol. 31, 748–752 (2013). - PubMed

[5] Liu S. & Trapnell C. Single-Cell Transcriptome Sequencing: Recent Advances and Remaining Challenges Vol. 5 F1000 Research (2016). - PMC - PubMed

[6] Liu S. & Trapnell C. Single-Cell Transcriptome Sequencing: Recent Advances and Remaining Challenges Vol. 5 F1000 Research (2016). - PMC - PubMed

[7] Jaitin D. A. et al.. Massively parallel single-cell RNA-seq for marker-free decomposition of tissues into cell types. Science 343, 776–779 (2014). - PMC - PubMed

[8] Jaitin D. A. et al.. Massively parallel single-cell RNA-seq for marker-free decomposition of tissues into cell types. Science 343, 776–779 (2014). - PMC - PubMed

[9] Pollen A. A. et al.. Low-coverage single-cell mRNA sequencing reveals cellular heterogeneity and activated signaling pathways in developing cerebral cortex. Nat. Biotechnol. 32, 1053–1058 (2014). - PMC - PubMed

[10] Pollen A. A. et al.. Low-coverage single-cell mRNA sequencing reveals cellular heterogeneity and activated signaling pathways in developing cerebral cortex. Nat. Biotechnol. 32, 1053–1058 (2014). - PMC - PubMed

Save citation to file

Email citation

Add to Collections

Add to My Bibliography

Your saved search

Create a file for external citation management software

Your RSS Feed

Massively parallel digital transcriptional profiling of single cells

Affiliations

Massively parallel digital transcriptional profiling of single cells

Authors

Affiliations

Abstract

Conflict of interest statement

Figures

Similar articles

Cited by

References

Publication types

MeSH terms

Substances

Grants and funding

LinkOut - more resources

Full Text Sources

Other Literature Sources

Molecular Biology Databases

Abstract

Conflict of interest statement

Figures

Similar articles

Cited by

References

Publication types

MeSH terms

Substances

Related information

Grants and funding

LinkOut - more resources

Full Text Sources

Other Literature Sources

Molecular Biology Databases