Methylation of the mouse DIx5 and Osx gene promoters regulates cell type-specific gene expression

Dlx5 and Osx are master regulatory proteins essential for initiating the cascade leading to osteoblast differentiation in mammals, but the mechanism of osteoblast-specific expression is not fully understood. DNA methylation at CpG sequences is involved in tissue and cell type-specific gene expression. We investigated the methylation status of Dlx5 and Osx in osteogenic and nonosteogenic cell lines by methylation-specific PCR (MSP). The CpG dinucleotides of the Dlx5 and Osx promoter regions were unmethylated in osteogenic cell lines transcribing these genes but methylated in nonosteogenic cell lines. Treatment of C2C12 cells with 5-AzadC induced dose- and time-dependent expression of Dlx5 and Osx mRNA by demethylating the corresponding promoters. Furthermore the mRNAs for the osteoblast markers ALP and OC, which were undetectable in untreated cells, gradually increased after 5-AzadC treatment. In addition, BMP-2 stimulation induced Dlx5 expression by hypomethylating its promoter. These findings suggest that DNA methylation plays an important role in cell type-specific expression of Dlx5 and Osx.     

转录因子Osterix对成骨细胞Col1a1基因的反式激活作用

Osterix（Osx）是一种具有锌指结构的转录因子,对骨形成十分重要. 但到目前为止,直接接受Osterix调控的靶基因尚不清楚.用骨形态发生蛋白2（bone morphogenetic protein 2,BMP2）诱导原代培养小鼠成骨细胞的骨分化,定量RT PCR检测Ⅰ型胶原蛋白(collagen Ⅰ a 1, Col1a1)与Osx的转录水平.结果发现,二者的转录时相具有相同的变化模式.为了确定二者之间的关系,采用腺病毒表达系统在原代成骨细胞中过表达Osx. 数据表明,Osx能够明显上调Col1a1的转录水平.用EMSA（electromobility shift assay）检测这些过表达Osx基因的成骨细胞核抽提物,迁移条带的出现表明,Osx能够直接与Col1a1的启动子相结合.结果提示,在原代培养的成骨细胞中,Osterix通过直接与启动子相结合,调控Col1a1基因的转录.     

Distinct roles for Hedgehog and canonical Wnt signaling in specification, differentiation and maintenance of osteoblast progenitors

Hedgehog and canonical Wnt/beta-catenin signaling are implicated in development of the osteoblast, the bone matrix-secreting cell of the vertebrate skeleton. We have used genetic approaches to dissect the roles of these pathways in specification of the osteoblast lineage. Previous studies indicate that Ihh signaling in the long bones is essential for initial specification of an osteoblast progenitor to a Runx2+ osteoblast precursor. We show here that this is a transient requirement, as removal of Hh responsiveness in later Runx2+, Osx1+ osteoblast precursors does not disrupt the formation of mature osteoblasts. By contrast, the removal of canonical Wnt signaling by conditional removal of the beta-catenin gene in early osteoblast progenitors or in Runx2+, Osx1+ osteoblast precursors results in a similar phenotype: osteoblasts fail to progress to a terminal osteocalcin+ fate and instead convert to a chondrocyte fate. By contrast, stabilization of beta-catenin signaling in Runx2+, Osx1+ osteoblast precursors leads to the premature differentiation of bone matrix secreting osteoblasts. These data demonstrate that commitment within the osteoblast lineage requires sequential, stage-specific, Ihh and canonical Wnt/beta-catenin signaling to promote osteogenic, and block chondrogenic, programs of cell fate specification.     

重组Osx腺病毒载体的构建及其调控成骨细胞增殖与分化的作用

构建表达成骨相关转录因子Osx的腺病毒,观察Osx对原代培养的小鼠成骨细胞增殖与分化的调控作用。将Osx编码基因克隆入腺病毒载体pAdEasy中,经293A包装后得到重组腺病毒,感染原代培养的小鼠颅骨细胞,茜素红染色观察矿化程度,实时定量RT-PCR检测成骨相关标志基因的转录水平,流式细胞检测细胞周期的改变。结果发现,①得到的病毒滴度为2×109PFU/ml,最佳感染复数为50;②表达Osx并不能够促进成骨细胞的矿化;③定量RT-PCR表明表达Osx 1d、3d、6d后成骨分化标志骨钙素、骨涎蛋白、Ⅰ型胶原蛋白的表达量明显上调(p<0.01);④流式细胞仪的结果表明Osx能够促进成骨细胞的增殖(p<0.01)。通过腺病毒在原代培养的成骨细胞中表达Osx能够促进成骨细胞的增殖,并对其分化具有一定的调控作用,为Osx在各种骨损伤的基因治疗应用方面提供了基础。