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在小鼠中表达的人 STC1 或 -2 会减小骨大小,并严重抑制颅膜内骨生长。

Human stanniocalcin-1 or -2 expressed in mice reduces bone size and severely inhibits cranial intramembranous bone growth.

机构信息

Cancer Research Laboratory Program, London Regional Cancer Program (LRCP), 790 Commissioners Rd, Room A4-921, London, ON, N6A 4L6, Canada.

出版信息

Transgenic Res. 2010 Dec;19(6):1017-39. doi: 10.1007/s11248-010-9376-7. Epub 2010 Feb 20.

DOI:10.1007/s11248-010-9376-7
PMID:20174869
Abstract

Stanniocalcin-1 (STC1) and -2 (STC2) are highly related, secreted, homodimeric glycoproteins that are significantly upregulated by different forms of stress including high phosphate levels. Transgenic mice that constitutively express either human STC1 or STC2 exhibit intra-uterine growth restriction and permanent post-natal growth retardation. STC1 is expressed in chondrocytic and osteoblastic cells during murine development and can enhance differentiation of calvarial cells in culture. Therefore, there is mounting evidence that stanniocalcins (STCs) modulate bone development in vivo. To further define the effects of stanniocalcins on skeletal development, we performed a series of measurements on components of the axial, appendicular, and cranial skeleton in transgenic and wildtype mice. We show that skeletal growth is retarded and that the intramembranous bones of the cranium exhibit a particularly severe delay in suture closure. The posterior frontal suture remains patent throughout the lifetime of human STC1 and STC2 transgenic mice. We did not observe significant effects on chondrogenesis: however, calvarial cells exhibited reduced viability, proliferation and delayed differentiation, indicating that developing osteoblasts are particularly sensitive to the levels of STCs. Given the evidence linking STC1 to cellular phosphate homeostasis, we assessed the expression of a variety of phosphate regulators in transgenic and wildtype calvarial cells and found significantly lower levels of Mepe, Dmp1, Sfrp4 in transgenic cells without a change in Pit1 or Pit2. Collectively these data support a direct regulatory role for STCs in osteoblasts and suggest that overexposure to these factors inhibits normal skeletal development without significant changes in patterning.

摘要

Stanniocalcin-1 (STC1) 和 -2 (STC2) 是高度相关的分泌性同源二聚体糖蛋白,它们会被多种形式的应激显著上调,包括高磷酸盐水平。持续表达人 STC1 或 STC2 的转基因小鼠表现出宫内生长受限和永久性出生后生长迟缓。STC1 在鼠类发育过程中表达于软骨细胞和成骨细胞中,并能增强颅骨细胞在培养中的分化。因此,越来越多的证据表明,Stanniocalcins (STCs) 在体内调节骨发育。为了进一步确定 STCs 对骨骼发育的影响,我们在转基因和野生型小鼠中对轴骨、附肢骨和颅骨的成分进行了一系列测量。我们发现骨骼生长迟缓,颅骨的膜内骨在骨缝闭合方面表现出特别严重的延迟。人类 STC1 和 STC2 转基因小鼠的额骨后缝终生保持开放。我们没有观察到对软骨生成有显著影响:然而,颅骨细胞的活力、增殖和分化延迟减少,表明发育中的成骨细胞对 STCs 的水平特别敏感。鉴于 STC1 与细胞磷酸盐稳态有关的证据,我们评估了转基因和野生型颅骨细胞中多种磷酸盐调节剂的表达,发现转基因细胞中 Mepe、Dmp1、Sfrp4 的表达水平显著降低,而 Pit1 或 Pit2 没有变化。这些数据共同支持 STCs 在成骨细胞中的直接调节作用,并表明过度暴露于这些因子会抑制正常的骨骼发育,而不会导致模式发生显著变化。

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