北京大学学报(医学版) ›› 2018, Vol. 50 ›› Issue (3): 521-526. doi: 10.3969/j.issn.1671-167X.2018.03.021
杨柳,楚小玉,赵奇△
YANG Liu,CHU Xiao-yu,ZHAO Qi△
摘要: Objective: To investigate the regulation mechanism of RhoA signaling pathway during the enamel formation by using the EGFPRhoA Dominant Negative (EGFPRhoADN)transgenic mice model, from the aspect of adherens junctions, and to provide a theory basis for mechanism of enamel development defects. Methods: The enamel thickness of mandibular first molars of EGFPRhoADN transgenic mice and wild type (WT) mice were observed by scanning electronic microscopy at 20 kV, and the enamel thickness of the distal face of the central cusp was measured at 10 locations via analysis by ImageJ (Rasband, 1997-2009). The enamel organs from mandibular first molars from postnatal4day (P4) EGFPRhoADN mice and wild type mice were isolated, and the total RNA and protein were extracted from the epithelium of the enamel organs. The expression level of the adherens junctions components in ameloblasts layer of the postnatal4day EGFPRhoADN transgenic mice and wild type mice mandibular first molars were detected by realtime PCR and Western blot assay. Results: The EGFPRhoADN transgenic mice had decreased enamel thickness in their bilateral mandibular first molars versus those of control group (n=20), and enamel thickness was (84.60±0.20) μm vs. (106.24±0.24) μm, P<0.05 .The protein expressions of Ecadherin, αEcatenin and pancadherin in ameloblasts layer of postnatal4day EGFPRhoADN transgenic mice molars were downregulated, and the protein level of βcatenin in ameloblasts layer of P4 EGFPRhoADN transgenic mice molars was upregulated. The mRNA level of Ecadherin in ameloblasts layer of P4 EGFPRhoADN transgenic mice molars was downregulated versus that of WT mice, and the gene expression of Ecadherin was 0.93±0.01 vs. 1.00±0.02, P<0.05. The mRNA level of βcatenin in ameloblasts layer of P4 EGFPRhoADN transgenic mice molars was upregulated versus that of WT mice, and the gene expression of βcatenin was 1.23±0.03 vs. 1.00±0.05, P<0.05. Conclusion: In the mandibular first molars of EGFPRhoADN transgenic mice, the enamel formation was disrupted and the adherens junctions of EGFPRhoADN transgenic mice ameloblasts were implicated during amelogenesis. RhoA signaling pathway may play a critical role in enamel development by altering the adherens junctions in ameloblasts.
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