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釉原蛋白与釉蛋白的定位和定量共定位。

Localization and quantitative co-localization of enamelin with amelogenin.

机构信息

Center for Craniofacial Molecular Biology, University of Southern California, Herman Ostrow School of Dentistry, Los Angeles, CA 90033, USA.

出版信息

J Struct Biol. 2013 Aug;183(2):239-49. doi: 10.1016/j.jsb.2013.03.014. Epub 2013 Apr 4.

Abstract

Enamelin and amelogenin are vital proteins in enamel formation. The cooperative function of these two proteins controls crystal nucleation and morphology in vitro. We quantitatively analyzed the co-localization between enamelin and amelogenin by confocal microscopy and using two antibodies, one raised against a sequence in the porcine 32 kDa enamelin region and the other raised against full-length recombinant mouse amelogenin. We further investigated the interaction of the porcine 32 kDa enamelin and recombinant amelogenin using immuno-gold labeling. This study reports the quantitative co-localization results for postnatal days 1-8 mandibular mouse molars. We show that amelogenin and enamelin are secreted into the extracellular matrix on the cuspal slopes of the molars at day 1 and that secretion continues to at least day 8. Quantitative co-localization analysis (QCA) was performed in several different configurations using large (45 μm height, 33 μm width) and small (7 μm diameter) regions of interest to elucidate any patterns. Co-localization patterns in day 8 samples revealed that enamelin and amelogenin co-localize near the secretory face of the ameloblasts and appear to be secreted approximately in a 1:1 ratio. The degree of co-localization decreases as the enamel matures, both along the secretory face of ameloblasts and throughout the entire thickness of the enamel. Immuno-reactivity against enamelin is concentrated along the secretory face of ameloblasts, supporting the theory that this protein together with amelogenin is intimately involved in mineral induction at the beginning of enamel formation.

摘要

釉原蛋白和釉基质蛋白是釉质形成的重要蛋白。这两种蛋白的协同功能控制着体外晶体的成核和形态。我们通过共聚焦显微镜和使用两种抗体(一种针对猪 32kDa 釉原蛋白区域的序列,另一种针对全长重组鼠釉基质蛋白)对釉原蛋白和釉基质蛋白的共定位进行了定量分析。我们进一步使用免疫金标记法研究了猪 32kDa 釉原蛋白和重组釉基质蛋白的相互作用。本研究报告了下颌磨牙出生后第 1-8 天的定量共定位结果。我们发现釉基质蛋白和釉原蛋白在第 1 天分泌到磨牙牙尖的细胞外基质中,并持续分泌到至少第 8 天。使用大(45μm 高,33μm 宽)和小(7μm 直径)感兴趣区域进行了几种不同配置的定量共定位分析(QCA),以阐明任何模式。第 8 天样本的共定位模式表明,釉原蛋白和釉基质蛋白在釉质细胞的分泌面附近共定位,并似乎以大约 1:1 的比例分泌。随着釉质的成熟,共定位程度在釉质细胞的分泌面以及整个釉质厚度上都降低。针对釉原蛋白的免疫反应性集中在釉质细胞的分泌面,支持了这样一种理论,即这种蛋白与釉基质蛋白一起,在釉质形成的早期密切参与了矿化诱导。

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