Store-operated Ca2+ entry controls ameloblast cell function and enamel development
Miriam Eckstein, Martin Vaeth, Cinzia Fornai, Manikandan Vinu, Timothy G. Bromage, Meerim K. Nurbaeva, Jessica L. Sorge, Paulo G. Coelho, Youssef Idaghdour, Stefan Feske, Rodrigo S. Lacruz
Miriam Eckstein, Martin Vaeth, Cinzia Fornai, Manikandan Vinu, Timothy G. Bromage, Meerim K. Nurbaeva, Jessica L. Sorge, Paulo G. Coelho, Youssef Idaghdour, Stefan Feske, Rodrigo S. Lacruz
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Research Article Bone biology Cell biology

Store-operated Ca2+ entry controls ameloblast cell function and enamel development

Abstract

Loss-of-function mutations in stromal interaction molecule 1 (STIM1) impair the activation of Ca2+ release–activated Ca2+ (CRAC) channels and store-operated Ca2+ entry (SOCE), resulting in a disease syndrome called CRAC channelopathy that is characterized by severe dental enamel defects. The cause of these enamel defects has remained unclear given a lack of animal models. We generated Stim1/2K14cre mice to delete STIM1 and its homolog STIM2 in enamel cells. These mice showed impaired SOCE in enamel cells. Enamel in Stim1/2K14cre mice was hypomineralized with decreased Ca content, mechanically weak, and thinner. The morphology of SOCE-deficient ameloblasts was altered, showing loss of the typical ruffled border, resulting in mislocalized mitochondria. Global gene expression analysis of SOCE-deficient ameloblasts revealed strong dysregulation of several pathways. ER stress genes associated with the unfolded protein response were increased in Stim1/2-deficient cells, whereas the expression of components of the glutathione system were decreased. Consistent with increased oxidative stress, we found increased ROS production, decreased mitochondrial function, and abnormal mitochondrial morphology in ameloblasts of Stim1/2K14cre mice. Collectively, these data show that loss of SOCE in enamel cells has substantial detrimental effects on gene expression, cell function, and the mineralization of dental enamel.

Authors

Miriam Eckstein, Martin Vaeth, Cinzia Fornai, Manikandan Vinu, Timothy G. Bromage, Meerim K. Nurbaeva, Jessica L. Sorge, Paulo G. Coelho, Youssef Idaghdour, Stefan Feske, Rodrigo S. Lacruz

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Figure 3

Stim1/2K14cre mice show hypomineralized enamel.

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Stim1/2K14cre mice show hypomineralized enamel. (A and B) Backscattered...
(A and B) Backscattered scanning electron microscopy (BSE) analyses of incisor cross-sections isolated from WT (A) and Stim1/2K14cre mice (B) sampled just below the anterior first lower molar (M1) (see also Supplemental Figure 1) showing diminished BSE signals in the enamel in Stim1/2K14cre mice, consistent with severe hypomineralization (n = 3 mice per group). (C and D) Representative scanning electron microscopy (SEM) micrographs in secondary electron mode of the same mice showing normal rod-interrod microstructure in the WT (C) and Stim1/2K14cre mouse enamel (D). (E and F) Molar rows in WT (E) and Stim1/2K14cre mice (F) showing increased wear in the latter. All Stim1/2K14cre mice analyzed in this study showed increased tooth wear. (G and H) Close up of the boxed areas in E and F showing severely cracked outer enamel in Stim1/2K14cre mouse molars. Scale bar: 10 μm (A–D); 100 μm (E and F). E, enamel; D, dentine. The asterisk in D might be an artefact during processing of sample for SEM.