SNX10 regulates osteoclastogenic cell fusion and osteoclast size in mice.
Maayan Barnea-ZoharMerle SteinNina ReuvenSabina Winograd-KatzSooyeon LeeYoseph AddadiEsther ArmanJan TuckermannBenjamin GeigerAri ElsonPublished in: Journal of bone and mineral research : the official journal of the American Society for Bone and Mineral Research (2024)
Bone-resorbing osteoclasts (OCLs) are formed by differentiation and fusion of monocyte precursor cells, generating large multi-nucleated cells. Tightly-regulated cell fusion during osteoclastogenesis leads to formation of resorption-competent OCLs, whose sizes fall within a predictable physiological range. The molecular mechanisms that regulate the onset of OCL fusion and its subsequent arrest are, however, largely unknown. We have previously shown that OCLs cultured from mice homozygous for the R51Q mutation in the vesicle trafficking-associated protein sorting nexin 10, a mutation that induces autosomal recessive osteopetrosis in humans and in mice, display deregulated and continuous fusion that generates gigantic, inactive OCLs. Fusion of mature OCLs is therefore arrested by an active, genetically-encoded, cell-autonomous, and SNX10-dependent mechanism. In order to directly examine whether SNX10 performs a similar role in vivo, we generated SNX10-deficient (SKO) mice and demonstrated that they display massive osteopetrosis and that their OCLs fuse uncontrollably in culture, as do homozygous R51Q SNX10 (RQ/RQ) mice. OCLs that lack SNX10 exhibit persistent presence of DC-STAMP protein at their periphery, which may contribute to their uncontrolled fusion. In order to visualize endogenous SNX10-mutant OCLs in their native bone environment we genetically labelled the OCLs of wild-type, SKO and RQ/RQ mice with EGFP, and then visualized the three-dimensional organization of resident OCLs and the pericellular bone matrix by two-photon, confocal, and second harmonics generation microscopy. We show that the volumes, surface areas and, in particular, the numbers of nuclei in the OCLs of both mutant strains were on average 2-6 fold larger than those of OCLs from wild-type mice, indicating that deregulated, excessive fusion occurs in the mutant mice. We conclude that the fusion of OCLs, and consequently their size, are regulated in vivo by SNX10-dependent arrest of fusion of mature OCLs.
Keyphrases
- wild type
- high fat diet induced
- induced apoptosis
- escherichia coli
- cell therapy
- insulin resistance
- stem cells
- single cell
- mesenchymal stem cells
- high resolution
- type diabetes
- protein protein
- cell death
- body mass index
- immune response
- high speed
- small molecule
- cell cycle
- optical coherence tomography
- mass spectrometry
- physical activity
- quality improvement
- body composition
- metabolic syndrome
- postmenopausal women
- living cells
- cord blood
- binding protein