Comparative Analysis of Single-Cell RNA Sequencing Methods with and without Sample Multiplexing

Yi Xie; Huimei Chen; Vasuki Ranjani Chellamuthu; Ahmad bin Mohamed Lajam; Salvatore Albani; Andrea Hsiu Ling Low; Enrico Petretto; Jacques Behmoaras

doi:10.3390/ijms25073828

International Journal of Molecular Sciences (Mar 2024)

Comparative Analysis of Single-Cell RNA Sequencing Methods with and without Sample Multiplexing

Yi Xie,
Huimei Chen,
Vasuki Ranjani Chellamuthu,
Ahmad bin Mohamed Lajam,
Salvatore Albani,
Andrea Hsiu Ling Low,
Enrico Petretto,
Jacques Behmoaras

Affiliations

Yi Xie: Programme in Cardiovascular and Metabolic Disorders and Centre for Computational Biology, Duke-NUS Medical School, 8 College Road, Singapore 169857, Singapore
Huimei Chen: Programme in Cardiovascular and Metabolic Disorders and Centre for Computational Biology, Duke-NUS Medical School, 8 College Road, Singapore 169857, Singapore
Vasuki Ranjani Chellamuthu: Translational Immunology Institute, SingHealth/Duke-NUS Academic Medical Centre, Academia, Singapore 169856, Singapore
Ahmad bin Mohamed Lajam: Translational Immunology Institute, SingHealth/Duke-NUS Academic Medical Centre, Academia, Singapore 169856, Singapore
Salvatore Albani: Translational Immunology Institute, SingHealth/Duke-NUS Academic Medical Centre, Academia, Singapore 169856, Singapore
Andrea Hsiu Ling Low: Department of Rheumatology and Immunology, Singapore General Hospital, Academia, Singapore 169856, Singapore
Enrico Petretto: Programme in Cardiovascular and Metabolic Disorders and Centre for Computational Biology, Duke-NUS Medical School, 8 College Road, Singapore 169857, Singapore
Jacques Behmoaras: Programme in Cardiovascular and Metabolic Disorders and Centre for Computational Biology, Duke-NUS Medical School, 8 College Road, Singapore 169857, Singapore

DOI: https://doi.org/10.3390/ijms25073828
Journal volume & issue: Vol. 25, no. 7
p. 3828

Abstract

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Single-cell RNA sequencing (scRNA-seq) has emerged as a powerful technique for investigating biological heterogeneity at the single-cell level in human systems and model organisms. Recent advances in scRNA-seq have enabled the pooling of cells from multiple samples into single libraries, thereby increasing sample throughput while reducing technical batch effects, library preparation time, and the overall cost. However, a comparative analysis of scRNA-seq methods with and without sample multiplexing is lacking. In this study, we benchmarked methods from two representative platforms: Parse Biosciences (Parse; with sample multiplexing) and 10x Genomics (10x; without sample multiplexing). By using peripheral blood mononuclear cells (PBMCs) obtained from two healthy individuals, we demonstrate that demultiplexed scRNA-seq data obtained from Parse showed similar cell type frequencies compared to 10x data where samples were not multiplexed. Despite relatively lower cell capture affecting library preparation, Parse can detect rare cell types (e.g., plasmablasts and dendritic cells) which is likely due to its relatively higher sensitivity in gene detection. Moreover, a comparative analysis of transcript quantification between the two platforms revealed platform-specific distributions of gene length and GC content. These results offer guidance for researchers in designing high-throughput scRNA-seq studies.

Published in International Journal of Molecular Sciences

ISSN: 1661-6596 (Print); 1422-0067 (Online)
Publisher: MDPI AG
Country of publisher: Switzerland
LCC subjects: Science: Biology (General); Science: Chemistry
Website: http://www.mdpi.com/journal/ijms

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