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Chondrocyte-specific regulatory activity of runx2 is essential for survival and skeletal development.

机译:runx2的软骨细胞特异性调节活性对于生存和骨骼发育至关重要。

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Coordinated activities of multiple mesenchymal cell types contribute to the development of the mammalian skeleton formed through endochondral ossification. Synthesis of a cartilage template by chondrocytes is an obligatory step for the generation of skeletal elements during endochondral ossification. Gene ablation studies have established that Runx2 is an essential transcription factor for bone formation and the differentiation of skeletal cells. However, global gene deletion has failed to discern the tissue- and cell type-specific roles of Runx2. We generated floxed mice to elucidate the Runx2 regulatory control distinctive to cartilage tissue during bone development. Exon 8 of the Runx2 gene was selectively deleted in developing chondrocytes by utilizing Col2a-Cre mice. Cell- and tissue-specific gene recombination was confirmed by beta-gal activity in R26R mice. The chondrocyte-specific loss of Runx2 caused failure of endochondral ossification, impaired craniofacial development, dwarfism, and perinatal lethality. Radiographic imaging and histochemical approaches were used to characterize the skeletal phenotype. We conclude that regulatory control of Runx2 in chondrocytes is essential for endochondral ossification, and it is independent of the role of Runx2 in osteoblasts.
机译:多种间充质细胞类型的协调活动有助于通过软骨内骨化形成的哺乳动物骨骼的发展。软骨细胞合成软骨模板是在软骨内骨化过程中生成骨骼元素的必不可少的步骤。基因消融研究已确定Runx2是骨骼形成和骨骼细胞分化的重要转录因子。但是,全局基因删除未能识别Runx2的组织和细胞类型特定的作用。我们生成了疏松的小鼠,以阐明在骨骼发育过程中软骨组织所特有的Runx2调节控制。通过使用Col2a-Cre小鼠,在发育中的软骨细胞中选择性删除了Runx2基因的外显子8。 R26R小鼠的β-gal活性证实了细胞和组织特异性基因重组。 Runx2的软骨细胞特异性丢失导致软骨内骨化失败,颅面发育受损,侏儒症和围生期致死率降低。放射成像和组织化学方法被用来表征骨骼表型。我们得出结论,软骨细胞中Runx2的调节控制对于软骨内骨化至关重要,并且它独立于Runx2在成骨细胞中的作用。

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