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氟化物通过雄激素和孕激素受体信号通路改变成釉细胞成熟期的激肽释放酶4表达。

Fluoride Alters Klk4 Expression in Maturation Ameloblasts through Androgen and Progesterone Receptor Signaling.

作者信息

Le Michael H, Nakano Yukiko, Abduweli Uyghurturk Dawud, Zhu Li, Den Besten Pamela K

机构信息

Department of Orofacial Sciences, School of Dentistry, University of California, San Francisco, San Francisco, CA, United States.

Center for Children's Oral Health Research, School of Dentistry, University of California, San Francisco, San Francisco, CA, United States.

出版信息

Front Physiol. 2017 Nov 14;8:925. doi: 10.3389/fphys.2017.00925. eCollection 2017.

Abstract

Fluorosed maturation stage enamel is hypomineralized in part due to a delay in the removal of matrix proteins to inhibit final crystal growth. The delay in protein removal is likely related to reduced expression of kallikrein-related peptidase 4 (KLK4), resulting in a reduced matrix proteinase activity that found in fluorosed enamel. transcription is known to be regulated in other cell types by androgen receptor (AR) and progesterone receptors (PR). In this study, we determined the possible role of fluoride in down-regulation of KLK4 expression through changes in AR and PR. Immunohistochemical localization showed that both AR and PR nuclear translocation was suppressed in fluoride exposed mice. However, when AR signaling was silenced in mouse ameloblast-lineage cells (ALCs), expression of both and were increased. Similar to the effect from AR silencing, fluoride also upregulated in ALCs, but downregulated . This finding suggests that though suppression of AR transactivation by fluoride increases expression, inhibition of PR transactivation by fluoride has a much greater effect, ultimately resulting in downregulation of expression. These findings indicate that in ameloblasts, PR has a dominant role in regulating expression. We found that when AR was retained in the cytoplasm in the presence of fluoride, that co-localized with heat shock protein 90 (HSP90), a well-known chaperone for steroid hormone receptors. HSP90 also known to regulate TGF-β signaling. Consistent with the effect of fluoride on AR and HSP90, we found evidence of reduced TGF-β signaling activity in fluorosed ameloblasts as reduced immunolocalization of TGFB1 and TGFBR-2 and a significant increase in Cyclin D1 mRNA expression, which also possibly contributes to the reduced AR signaling activity. , when serum was removed from the media, aluminum was required for fluoride to inhibit the dissociation of HSP90 from AR. In conclusion, fluoride related downregulation of is associated with reduced nuclear translocation of AR and PR, and also reduced TGF-β signaling activity, all of which are regulated by HSP90. We suggest that a common mechanism by which fluoride affects AR, PR, and TGF-β signaling is through inhibiting ATP-dependent conformational cycling of HSP90.

摘要

氟斑牙成熟阶段的牙釉质存在矿化不足的情况,部分原因是基质蛋白去除延迟,从而抑制了晶体的最终生长。蛋白去除延迟可能与激肽释放酶相关肽酶4(KLK4)表达降低有关,导致氟斑牙釉质中基质蛋白酶活性降低。已知转录在其他细胞类型中受雄激素受体(AR)和孕激素受体(PR)调控。在本研究中,我们通过AR和PR的变化确定了氟化物在下调KLK4表达中的可能作用。免疫组织化学定位显示,在氟暴露小鼠中,AR和PR的核转位均受到抑制。然而,当在小鼠成釉细胞系细胞(ALCs)中沉默AR信号时,KLK4和PR的表达均增加。与AR沉默的效果相似,氟化物也上调了ALCs中KLK4的表达,但下调了PR的表达。这一发现表明,尽管氟化物抑制AR反式激活会增加KLK4表达,但氟化物抑制PR反式激活的作用更大,最终导致KLK4表达下调。这些发现表明,在成釉细胞中,PR在调节KLK4表达中起主导作用。我们发现,当在氟化物存在的情况下AR保留在细胞质中时,它与热休克蛋白90(HSP90)共定位,HSP90是类固醇激素受体的著名伴侣蛋白。HSP90也已知调节TGF-β信号通路。与氟化物对AR和HSP90的作用一致,我们发现氟斑牙成釉细胞中TGF-β信号活性降低的证据,表现为TGFB1和TGFBR-2免疫定位减少以及细胞周期蛋白D1 mRNA表达显著增加,这也可能导致AR信号活性降低。此外,当从培养基中去除血清时,氟化物需要铝来抑制HSP90与AR的解离。总之,氟化物相关的KLK4下调与AR和PR的核转位减少以及TGF-β信号活性降低有关,所有这些都受HSP90调控。我们认为氟化物影响AR、PR和TGF-β信号通路的共同机制是通过抑制HSP90依赖ATP 的构象循环。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f001/5715335/78ddcc73b791/fphys-08-00925-g0001.jpg

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