Sun Zewen, Yan Mingyue, Wang Junjie, Zhang Haoyun, Ji Xiaobin, Xiao Yujing, Wang Tianrui, Yu Tengbo
Qingdao Medical College, Qingdao University, Qingdao, Shandong, China.
Department of Orthopedics, The Affiliated Hospital of Qingdao University, Qingdao, Shandong, China.
Front Immunol. 2024 May 29;15:1407679. doi: 10.3389/fimmu.2024.1407679. eCollection 2024.
Cartilage injury is the main pathological manifestation of osteoarthritis (OA). Healthy chondrocyte is a prerequisite for cartilage regeneration and repair. Differences between healthy and OA chondrocyte types and the role these types play in cartilage regeneration and OA progression are unclear.
This study conducted single-cell RNA sequencing (scRNA-seq) on the cartilage from normal distal femur of the knee (NC group) and OA femur (OA group) cartilage, the chondrocyte atlas was constructed, and the differences of cell subtypes between the two groups were compared. Pseudo-time and RNA velocity analysis were both performed to verify the possible differentiation sequence of cell subtypes. GO and KEGG pathway enrichment analysis were used to explore the potential functional characteristics of each cell subtype, and to predict the functional changes during cell differentiation. Differences in transcriptional regulation in subtypes were explored by single-cell regulatory network inference and clustering (SCENIC). The distribution of each cell subtype in cartilage tissue was identified by immunohistochemical staining (IHC).
A total of 75,104 cells were included, they were divided into 19 clusters and annotated as 11 chondrocyte subtypes, including two new chondrocyte subtypes: METRNL+ and PRG4+ subtype. METRNL+ is in an early stage during chondrocyte differentiation, and RegC-B is in an intermediate state before chondrocyte dedifferentiation. With cell differentiation, cell subtypes shift from genetic expression to extracellular matrix adhesion and collagen remodeling, and signal pathways shift from HIF-1 to Hippo. The 11 subtypes were finally classified as intrinsic chondrocytes, effector chondrocytes, abnormally differentiated chondrocytes and dedifferentiated chondrocytes. IHC was used to verify the presence and distribution of each chondrocyte subtype.
This study screened two new chondrocyte subtypes, and a novel classification of each subtype was proposed. METRNL+ subtype is in an early stage during chondrocyte differentiation, and its transcriptomic characteristics and specific pathways provide a foundation for cartilage regeneration. EC-B, PRG4+ RegC-B, and FC are typical subtypes in the OA group, and the HippO-Taz pathway enriched by these cell subtypes may play a role in cartilage repair and OA progression. RegC-B is in the intermediate state before chondrocyte dedifferentiation, and its transcriptomic characteristics may provide a theoretical basis for intervening chondrocyte dedifferentiation.
软骨损伤是骨关节炎(OA)的主要病理表现。健康的软骨细胞是软骨再生和修复的前提条件。健康软骨细胞与骨关节炎软骨细胞类型之间的差异以及这些类型在软骨再生和骨关节炎进展中所起的作用尚不清楚。
本研究对膝关节正常股骨远端软骨(NC组)和骨关节炎股骨软骨(OA组)进行单细胞RNA测序(scRNA-seq),构建软骨细胞图谱,并比较两组细胞亚型的差异。进行了伪时间和RNA速度分析以验证细胞亚型可能的分化顺序。使用GO和KEGG通路富集分析来探索每个细胞亚型的潜在功能特征,并预测细胞分化过程中的功能变化。通过单细胞调控网络推断和聚类(SCENIC)探索亚型中转录调控的差异。通过免疫组织化学染色(IHC)确定每种细胞亚型在软骨组织中的分布。
共纳入75104个细胞,它们被分为19个簇,并注释为11种软骨细胞亚型,包括两种新的软骨细胞亚型:METRNL+和PRG4+亚型。METRNL+处于软骨细胞分化的早期阶段,而RegC-B处于软骨细胞去分化前的中间状态。随着细胞分化,细胞亚型从基因表达转变为细胞外基质粘附和胶原蛋白重塑,信号通路从HIF-1转变为Hippo。这11种亚型最终被分类为固有软骨细胞、效应软骨细胞、异常分化软骨细胞和去分化软骨细胞。使用IHC验证每种软骨细胞亚型的存在和分布。
本研究筛选出两种新的软骨细胞亚型,并提出了每种亚型的新分类。METRNL+亚型处于软骨细胞分化早期,其转录组特征和特定途径为软骨再生提供了基础。EC-B、PRG4+ RegC-B和FC是OA组中的典型亚型,这些细胞亚型富集的HippO-Taz通路可能在软骨修复和OA进展中起作用。RegC-B处于软骨细胞去分化前的中间状态,其转录组特征可能为干预软骨细胞去分化提供理论依据。
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