Single-cell RNA Sequencing Reveals Heterogeneity of Cultured Bovine Satellite Cells

Pengcheng Lyu; Yumin Qi; Zhijian J Tu; Honglin Jiang

doi:10.3389/fgene.2021.742077

Single-cell RNA Sequencing Reveals Heterogeneity of Cultured Bovine Satellite Cells

Front Genet. 2021 Oct 28:12:742077. doi: 10.3389/fgene.2021.742077. eCollection 2021.

Authors

Pengcheng Lyu¹, Yumin Qi², Zhijian J Tu², Honglin Jiang¹

Affiliations

¹ Department of Animal and Poultry Sciences, Virginia Tech, Blacksburg, VA, United States.
² Department of Biochemistry, Virginia Tech, Blacksburg, VA, United States.

Abstract

Skeletal muscle from meat-producing livestock such as cattle is a major source of food for humans. To improve skeletal muscle growth efficiency or quality in cattle, it is necessary to understand the genetic and physiological mechanisms that govern skeletal muscle composition, development, and growth. Satellite cells are the myogenic progenitor cells in postnatal skeletal muscle. In this study we analyzed the composition of bovine satellite cells with single-cell RNA sequencing (scRNA-seq). We isolated satellite cells from a 2-week-old male calf, cultured them in growth medium for a week, and performed scRNA-seq using the 10x Genomics platform. Deep sequencing of two scRNA-seq libraries constructed from cultured bovine satellite cells yielded 860 million reads. Cell calling analyses revealed that these reads were sequenced from 19,096 individual cells. Clustering analyses indicated that these reads represented 15 cell clusters that differed in gene expression profile. Based on the enriched expression of markers of satellite cells (PAX7 and PAX3), markers of myoblasts (MYOD1, MYF5), and markers of differentiated myoblasts or myocytes (MYOG), three clusters were determined to be satellite cells, two clusters myoblasts, and two clusters myocytes. Gene ontology and trajectory inference analyses indicated that cells in these myogenic clusters differed in proliferation rate and differentiation stage. Two of the remaining clusters were enriched with PDGFRA, a marker of fibro-adipogenic (FAP) cells, the progenitor cells for intramuscular fat, and are therefore considered to be FAP cells. Gene ontology analyses indicated active lipogenesis in one of these two clusters. The identity of the remaining six clusters could not be defined. Overall, the results of this study support the hypothesis that bovine satellite cells are composed of subpopulations that differ in transcriptional and myogenic state. The results of this study also support the hypothesis that intramuscular fat in cattle originates from fibro-adipogenic cells.

Keywords: FAP; ScRNA-seq; cattle; fibro-adipogenic progenitors; myoblast; skeletal muscle.