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Truncated amelogenin and LRAP transgenes improve Amelx null mouse enamel

机译:截短的釉原蛋白和LRAP转基因可改善Amelx无小鼠釉质

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摘要

Amelogenin is the most abundant enamel protein involved in enamel mineralization. Our goal was to determine whether all three regions of amelogenin (N-terminus, C-terminus, central core) are required for enamel formation. Amelogenin RNA is alternatively spliced, resulting in at least 16 different amelogenin isoforms in mice, with M180 and LRAP expressed most abundantly. Soon after secretion by ameloblasts, M180 is cleaved by MMP20 resulting in C-terminal truncated (CTRNC) amelogenin. We aimed to determine whether the 2 transgenes (Tg), LRAP and CTRNC together, can improve LRAPTg/Amelx−/− and CTRNCTg/Amelx−/− enamel thickness and prism organization, which were not rescued in Amelx−/− enamel. We generated CTRNCTg/LRAPTg/Amelx−/− mice and analyzed developing and mature incisor and molar enamel histologically, by microCT, SEM and microhardness testing. CTRNCTg and LRAPTg overexpression together significantly improved the enamel phenotype of LRAPTg/Amelx−/− and CTRNCTg/Amelx−/− mouse enamel, however enamel microhardness was recovered only when M180Tg was expressed, alone or with LRAPTg. We determined that both LRAP and CTRNC, which together express all three regions of the amelogenin protein (N-terminus, C-terminus and hydrophobic core) contribute to the final enamel thickness and prism organization in mice.
机译:釉釉蛋白是参与釉质矿化的最丰富的釉质蛋白。我们的目标是确定牙釉蛋白的三个区域(N端,C端,中央核心)是否都需要形成牙釉质。剪接Amelogenin RNA,在小鼠中产生至少16种不同的Amelogenin亚型,其中M180和LRAP表达最丰富。成釉细胞分泌后不久,MMP20裂解M180,导致C端截短(CTRNC)牙釉蛋白。我们旨在确定LRAP和CTRNC这两个转基因(Tg)是否可以共同改善LRAPTg / Amelx-/-和CTRNCTg / Amelx-/-釉质的厚度和棱柱组织,而这在Amelx-/-釉质中无法挽救。我们生成了CTRNCTg / LRAPTg / Amelx-/-小鼠,并通过microCT,SEM和显微硬度测试从组织学上分析了发育成熟的门牙和磨牙珐琅质。 CTRNCTg和LRAPTg的过表达共同显着改善了LRAPTg / Amelx-/-和CTRNCTg / Amelx-/-小鼠牙釉质的牙釉质表型,但是仅当表达M180Tg或单独使用LRAPTg时,牙釉质的显微硬度才能恢复。我们确定,LRAP和CTRNC共同表达釉蛋白原蛋白的所有三个区域(N端,C端和疏水核)共同促进了小鼠的最终釉质厚度和棱柱组织。

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