Zhijia Tan, Hiu Tung Shek, Zeluan Li, Linjian Xia, Yanni He, Peikai Chen, Janus Siu Him Wong, Bo Gao, Danny Chan, Michael Kai Tsun To
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The mutant Ifitm5 allele could be regulated by the endogenous regulatory elements after Cre recombination, maintaining its spatiotemporal expression pattern and physiological level. Specifically, Prx1-Cre; Ifitm5flox c.-14C>T mutant mice were born with fractures in all limbs, showing impaired ossification and enhanced chondrogenesis associated with increased SOX9 abundance. Analyses of single-cell RNA sequencing data revealed arrested osteogenesis in Prx1-Cre; Ifitm5flox c.-14C>T mouse. A major population of cells expressing both osteogenic and chondrogenic signature genes was identified in the mutant mouse. Reduced expression of SP7 and SOST in the cortical regions of mutant mice confirmed delayed osteocyte maturation and compromised osteogenesis. Elevated bone marrow adipocytes were found in the adult mutant mice. Ectopic chondrogenesis and SOX9 expression were also observed in the perichondrium regions of Col1a1-Cre; Ifitm5flox c.-14C>T and Ocn-Cre; Ifitm5flox c.-14C>T mutant mice. 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引用次数: 0
摘要
成骨不全(OI) V型的典型特征是桡骨头脱位、骨间膜钙化和骨痂增生。它是由IFITM5基因5' UTR的c - 14c > T突变引起的,在IFITM5蛋白的n端增加了5个氨基酸(MALEP)。先前的研究表明MALEP-IFITM5蛋白具有新形态功能。然而,由于先前小鼠模型的胚胎致死性,其潜在机制尚不清楚。因此,我们建立了可被不同发育阶段表达的Cre诱导的诱导小鼠模型(Ifitm5flox c - 14c > T),以探索新形态MALEP-IFITM5的致病作用。突变体Ifitm5等位基因在Cre重组后可受到内源调控元件的调控,维持其时空表达模式和生理水平。具体来说,Prx1-Cre;Ifitm5flox c - 14c >t突变小鼠出生时四肢骨折,骨化受损,软骨形成增强,SOX9丰度增加。单细胞RNA测序数据分析显示Prx1-Cre成骨阻滞;Ifitm5flox c - 14c > T鼠标。在突变小鼠中发现了表达成骨和软骨特征基因的主要细胞群。突变小鼠皮质区SP7和SOST的表达降低证实了骨细胞成熟延迟和成骨功能受损。在成年突变小鼠中发现骨髓脂肪细胞升高。Col1a1-Cre的软骨膜区也观察到异位软骨形成和SOX9的表达;Ifitm5flox c - 14c > T和Ocn-Cre;Ifitm5flox c - 14c > T突变小鼠。诱导型Ifitm5flox c - 14c > T小鼠模型和单细胞转录组学综合分析表明,SOX9的异位表达和成骨、软骨和脂肪生成之间的稳态平衡被破坏可能参与了MALEP-IFITM5引起的发病机制,有助于深入了解V型OI的分子机制。
An inducible mouse model of osteogenesis imperfecta type V reveals aberrant osteogenesis caused by Ifitm5 c.-14C>T mutation.
Osteogenesis imperfecta (OI) type V is typically characterized by radial head dislocation, calcification of interosseous membrane, and hyperplastic callus. It is caused by the c.-14C>T mutation in the 5' UTR of IFITM5 gene, adding 5 amino acids (MALEP) to the N-terminal of IFITM5 protein. Previous studies have suggested a neomorphic function of the MALEP-IFITM5 protein. However, the underlying mechanisms remain unclear due to embryonic lethality in previous mouse models. Therefore, we developed an inducible mouse model (Ifitm5flox c.-14C>T) that could be induced by Cre expressed at different developmental stages to explore the pathogenic effects of the neomorphic MALEP-IFITM5. The mutant Ifitm5 allele could be regulated by the endogenous regulatory elements after Cre recombination, maintaining its spatiotemporal expression pattern and physiological level. Specifically, Prx1-Cre; Ifitm5flox c.-14C>T mutant mice were born with fractures in all limbs, showing impaired ossification and enhanced chondrogenesis associated with increased SOX9 abundance. Analyses of single-cell RNA sequencing data revealed arrested osteogenesis in Prx1-Cre; Ifitm5flox c.-14C>T mouse. A major population of cells expressing both osteogenic and chondrogenic signature genes was identified in the mutant mouse. Reduced expression of SP7 and SOST in the cortical regions of mutant mice confirmed delayed osteocyte maturation and compromised osteogenesis. Elevated bone marrow adipocytes were found in the adult mutant mice. Ectopic chondrogenesis and SOX9 expression were also observed in the perichondrium regions of Col1a1-Cre; Ifitm5flox c.-14C>T and Ocn-Cre; Ifitm5flox c.-14C>T mutant mice. The inducible Ifitm5flox c.-14C>T mouse model and integrated single-cell transcriptomic analyses elucidated that ectopic expression of SOX9 and disrupted homeostatic balance among osteogenesis, chondrogenesis, and adipogenesis may contribute to the pathogenesis caused by MALEP-IFITM5, helping to gain deeper insights into the molecular mechanisms of type V OI.
期刊介绍:
The Journal of Bone and Mineral Research (JBMR) publishes highly impactful original manuscripts, reviews, and special articles on basic, translational and clinical investigations relevant to the musculoskeletal system and mineral metabolism. Specifically, the journal is interested in original research on the biology and physiology of skeletal tissues, interdisciplinary research spanning the musculoskeletal and other systems, including but not limited to immunology, hematology, energy metabolism, cancer biology, and neurology, and systems biology topics using large scale “-omics” approaches. The journal welcomes clinical research on the pathophysiology, treatment and prevention of osteoporosis and fractures, as well as sarcopenia, disorders of bone and mineral metabolism, and rare or genetically determined bone diseases.
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