Ambn 基因敲除小鼠牙釉质表型的转基因挽救。
Transgenic rescue of enamel phenotype in Ambn null mice.
机构信息
Department of Biologic and Materials Sciences, University of Michigan, School of Dentistry, 1011 North University, Ann Arbor, MI 48109-1078, USA.
出版信息
J Dent Res. 2010 Dec;89(12):1414-20. doi: 10.1177/0022034510379223. Epub 2010 Oct 12.
Abstract
Ameloblastin null mice fail to make an enamel layer, but the defects could be due to an absence of functional ameloblastin or to the secretion of a potentially toxic mutant ameloblastin. We hypothesized that the enamel phenotype could be rescued by the transgenic expression of normal ameloblastin in Ambn mutant mice. We established and analyzed 5 transgenic lines that expressed ameloblastin from the amelogenin (AmelX) promoter and identified transgenic lines that express virtually no transgene, slightly less than normal (Tg+), somewhat higher than normal (Tg++), and much higher than normal (Tg+++) levels of ameloblastin. All lines expressing detectable levels of ameloblastin at least partially recovered the enamel phenotype. When ameloblastin expression was only somewhat higher than normal, the enamel covering the molars and incisors was of normal thickness, had clearly defined rod and interrod enamel, and held up well in function. We conclude that ameloblastin is essential for dental enamel formation.
摘要
成釉蛋白基因敲除小鼠无法形成釉质层,但这种缺陷可能是由于功能性成釉蛋白的缺失,也可能是由于分泌潜在毒性的突变体成釉蛋白。我们假设在 Ambn 突变小鼠中转基因表达正常的成釉蛋白可以挽救釉质表型。我们建立并分析了 5 条表达釉原蛋白(AmelX)启动子的成釉蛋白的转基因系,并鉴定出表达几乎没有转基因(Tg+)、略低于正常(Tg++)、略高于正常(Tg+++)和成釉蛋白水平的转基因系。所有表达可检测水平成釉蛋白的转基因系至少部分恢复了釉质表型。当成釉蛋白的表达略高于正常时,磨牙和切牙的釉质覆盖层厚度正常,具有清晰定义的杆状和杆间釉质,在功能上表现良好。我们的结论是,成釉蛋白对于牙釉质的形成是必不可少的。
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