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Transcriptional control of chondrocyte fate and differentiation.软骨细胞命运与分化的转录调控。
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转录因子ERG与小鼠肢体和脊柱骨骼形成过程中的关节及关节软骨形成

Transcription factor ERG and joint and articular cartilage formation during mouse limb and spine skeletogenesis.

作者信息

Iwamoto Masahiro, Tamamura Yoshihiro, Koyama Eiki, Komori Toshihisa, Takeshita Nobuo, Williams Julie A, Nakamura Takashi, Enomoto-Iwamoto Motomi, Pacifici Maurizio

机构信息

Department of Orthopaedic Surgery, Thomas Jefferson University College of Medicine, Philadelphia, PA 19107, USA.

出版信息

Dev Biol. 2007 May 1;305(1):40-51. doi: 10.1016/j.ydbio.2007.01.037. Epub 2007 Feb 7.

DOI:10.1016/j.ydbio.2007.01.037
PMID:17336282
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2104487/
Abstract

Articular cartilage and synovial joints are critical for skeletal function, but the mechanisms regulating their development are largely unknown. In previous studies we found that the ets transcription factor ERG and its alternatively-spliced variant C-1-1 have roles in joint formation in chick. Here, we extended our studies to mouse. We found that ERG is also expressed in developing mouse limb joints. To test regulation of ERG expression, beads coated with the joint master regulator protein GDF-5 were implanted close to incipient joints in mouse limb explants; this led to rapid and strong ectopic ERG expression. We cloned and characterized several mammalian ERG variants and expressed a human C-1-1 counterpart (hERG3Delta81) throughout the cartilaginous skeleton of transgenic mice, using Col2a1 gene promoter/enhancer sequences. The skeletal phenotype was severe and neonatal lethal, and the transgenic mice were smaller than wild type littermates and their skeletons were largely cartilaginous. Limb long bone anlagen were entirely composed of chondrocytes actively expressing collagen IX and aggrecan as well as articular markers such as tenascin-C. Typical growth plates were absent and there was very low expression of maturation and hypertrophy markers, including Indian hedgehog, collagen X and MMP-13. The results suggest that ERG is part of molecular mechanisms leading chondrocytes into a permanent developmental path and become joint forming cells, and may do so by acting downstream of GDF-5.

摘要

关节软骨和滑膜关节对骨骼功能至关重要,但其发育调控机制在很大程度上尚不清楚。在先前的研究中,我们发现ets转录因子ERG及其可变剪接变体C-1-1在鸡的关节形成中发挥作用。在此,我们将研究扩展至小鼠。我们发现ERG也在发育中的小鼠肢体关节中表达。为了测试ERG表达的调控,将包被有关节主调节蛋白GDF-5的珠子植入小鼠肢体外植体中接近初始关节的位置;这导致了快速且强烈的异位ERG表达。我们克隆并鉴定了几种哺乳动物ERG变体,并使用Col2a1基因启动子/增强子序列在转基因小鼠的整个软骨骨骼中表达了人类C-1-1对应物(hERG3Delta81)。骨骼表型严重且新生致死,转基因小鼠比野生型同窝小鼠体型小,其骨骼主要为软骨。肢体长骨原基完全由活跃表达胶原蛋白IX和聚集蛋白聚糖以及诸如肌腱蛋白-C等关节标志物的软骨细胞组成。典型的生长板缺失,包括印度刺猬蛋白、胶原蛋白X和基质金属蛋白酶-13在内的成熟和肥大标志物的表达非常低。结果表明,ERG是导致软骨细胞进入永久性发育路径并成为关节形成细胞的分子机制的一部分,并且可能是通过在GDF-5下游发挥作用来实现的。