Yiqiang Song scite author profile

The short stature homeobox gene SHOX is associated with idiopathic short stature in humans, as seen in Turner syndrome and Leri-Weill dyschondrosteosis, while little is known about its close relative SHOX2. We report the restricted expression of Shox2 in the anterior domain of the secondary palate in mice and humans. Shox2-/- mice develop an incomplete cleft that is confined to the anterior region of the palate, an extremely rare type of clefting in humans. The Shox2-/- palatal shelves initiate, grow and elevate normally, but the anterior region fails to contact and fuse at the midline, owing to altered cell proliferation and apoptosis, leading to incomplete clefting within the presumptive hard palate. Accompanied with these cellular alterations is an ectopic expression of Fgf10 and Fgfr2c in the anterior palatal mesenchyme of the mutants. Tissue recombination and bead implantation experiments revealed that signals from the anterior palatal epithelium are responsible for the restricted mesenchymal Shox2 expression. BMP activity is necessary but not sufficient for the induction of palatal Shox2 expression. Our results demonstrate an intrinsic requirement for Shox2 in palatogenesis, and support the idea that palatogenesis is differentially regulated along the anteroposterior axis. Furthermore, our results demonstrate that fusion of the posterior palate can occur independently of fusion in the anterior palate.

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An incoherent regulatory network architecture that orchestrates B cell diversification in response to antigen signaling

Sciammas

Liu

Warmflash

et al. 2011

Molecular Systems Biology

116

145

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Transgenically ectopic expression of Bmp4 to the Msx1 mutant dental mesenchyme restores downstream gene expression but represses Shh and Bmp2 in the enamel knot of wild type tooth germ

Zhao

Zhang

Song

et al. 2000

Mechanisms of Development

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Bmp4 is a downstream gene of Msx1 in early mouse tooth development. In this study, we introduced the Msx1-Bmp4 transgenic allele to the Msx1 mutants in which tooth development is arrested at the bud stage in an effort of rescuing Msx1 mutant tooth phenotype in vivo. Ectopic expression of a Bmp4 transgene driven by the mouse Msx1promoter in the dental mesenchyme restored the expression of Lef-1 and Dlx2 but neither Fgf3 nor syndecan-1 in the Msx1 mutant molar tooth germ. The mutant phenotype of molar but not incisor could be partially rescued to progress to the cap stage. The Msx1-Bmp4 transgene was also able to rescue the alveolar processes and the neonatal lethality of the Msx1 mutants. In contrast, overexpression of Bmp4 in the wild type molar mesenchyme down-regulated Shh and Bmp2 expression in the enamel knot, the putative signaling center for tooth patterning, but did not produce a tooth phenotype. These results indicate that Bmp4 can bypass Msx1 function to partially rescue molar tooth development in vivo, and to support alveolar process formation. Expression of Shh and Bmp2 in the enamel knot may not represent critical signals for tooth patterning.

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Calcium-mediated Stress Kinase Activation by DMP1 Promotes Osteoblast Differentiation

Eapen

Sundivakkam

Song

et al. 2010

Journal of Biological Chemistry

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Calcium signaling and calcium transport play a key role during osteoblast differentiation and bone formation. Here, we demonstrate that DMP1 mediated calcium signaling, and its downstream effectors play an essential role in the differentiation of preosteoblasts to fully functional osteoblasts. DMP1, a key regulatory bone matrix protein, can be endocytosed by preosteoblasts, triggering a rise in cytosolic levels of calcium that initiates a series of downstream events leading to cellular stress. These events include release of store-operated calcium that facilitates the activation of stress-induced p38 MAPK leading to osteoblast differentiation. However, chelation of intracellular calcium and inhibition of the p38 signaling pathway by specific pharmacological inhibitors and dominant negative plasmid suppressed this activation. Interestingly, activated p38 MAPK can translocate to the nucleus to phosphorylate transcription factors that coordinate the expression of downstream target genes such as Runx 2, a key modulator of osteoblast differentiation. These studies suggest a novel paradigm by which DMP1-mediated release of intracellular calcium activates p38 MAPK signaling cascade to regulate gene expression and osteoblast differentiation.Osteoblasts can react to a variety of biological signals. Among these, calcium signaling is essential for the proliferation and differentiation of osteoblasts. Earlier studies have shown that treating osteoblasts with parathyroid hormone or vitamin D 3 induces an increase in intracellular calcium ([Ca 2ϩ ] i ) by increasing the release of Ca 2ϩ from the intracellular stores (1-5). Store-operated Ca 2ϩ channels, which are activated in response to Ca 2ϩ store depletion, control homeostasis between the extracellular Ca 2ϩ reservoir and intracellular Ca 2ϩ storage and control a wide range of cellular functions.Dentin matrix protein 1 (DMP1) initially identified and localized in the mineralized dentin and bone matrix (6) is thought to play a regulatory role only in the calcification of the extracellular matrix. Apart from its role in mineralization, one of the putative functions of DMP1 is its involvement during differentiation of osteoblasts and odontoblasts (7-9). DMP1-null mice displayed severe defects in bone formation (10). We had shown earlier that DMP1 is specifically localized in the nucleus of differentiating osteoblasts and odontoblasts, and this translocation from the extracellular matrix is facilitated by the endocytic receptor GRP78 (11). The 78-kDa glucose-regulated protein (GRP78) is a calcium-binding molecular chaperone expressed in the endoplasmic reticulum of eukaryotic cells. Identification of GRP78 as a cell surface receptor for DMP1 is particularly interesting as its induction is a protective response against several kinds of stress, including ER 2 Ca 2ϩ depletion and accumulation of unglycosylated proteins (12, 13). However, the specific signaling pathways activated following DMP1 stimulus and osteoblast differentiation are not delineated yet.p38 MAPKs are widely e...

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Application of lentivirus‐mediated RNAi in studying gene function in mammalian tooth development

Song

Zhang

et al. 2006

Developmental Dynamics

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RNA interference (RNAi) has recently become a powerful tool to silence gene expression in mammalian cells, but its application in assessing gene function in mammalian developing organs remains highly limited. Here we describe several unique developmental properties of the mouse molar germ. Embryonic molar mesenchyme, but not the incisor mesenchyme, once dissociated into single cell suspension and re-aggregated, retains its odontogenic potential, the capability of a tissue to instruct an adjacent tissue to initiate tooth formation. Dissociated molar mesenchymal cells, even after being plated in cell culture, retain odontogenic competence, the capability of a tissue to respond to odontogenic signals and to support tooth formation. Most interestingly, while dissociated epithelial and mesenchymal cells of molar tooth germ are mixed and re-aggregated, the epithelial cells are able to sort out from the mesenchymal cells and organize into a well-defined dental epithelial structure, leading to the formation of a well-differentiated tooth organ after sub-renal culture. These unique molar developmental properties allow us to develop a strategy using a lentivirus-mediated RNAi approach to silence gene expression in dental mesenchymal cells and assess gene function in tooth development. We show that knockdown of Msx1 or Dlx2 expression in the dental mesenchyme faithfully recapitulates the tooth phenotype of their targeted mutant mice. Silencing of Barx1 expression in the dental mesenchyme causes an arrest of tooth development at the bud stage, demonstrating a crucial role for Barx1 in tooth formation. Our studies have established a reliable and rapid assay that would permit large-scale analysis of gene function in mammalian tooth development.

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Yiqiang Song

Shox2-deficient mice exhibit a rare type of incomplete clefting of the secondary palate

An incoherent regulatory network architecture that orchestrates B cell diversification in response to antigen signaling

Transgenically ectopic expression of Bmp4 to the Msx1 mutant dental mesenchyme restores downstream gene expression but represses Shh and Bmp2 in the enamel knot of wild type tooth germ

Calcium-mediated Stress Kinase Activation by DMP1 Promotes Osteoblast Differentiation

Application of lentivirus‐mediated RNAi in studying gene function in mammalian tooth development

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