Nebel Daniel
Department of Periodontology, Faculty of Odontology, Malmö University, Sweden.
Swed Dent J Suppl. 2012(221):11-66.
The main functions of estrogen are associated with reproduction. However, estrogen has been shown to be of functional importance also in non-classic target organs. Previous studies, especially epidemiologic and clinical ones, have addressed estrogen's influence on periodontitis, suggesting that estrogen has a beneficial effect, but the biological mechanisms have not been identified. Estrogen exerts genomic effects in the target cells by binding to the nuclear receptors, estrogen receptor (ERs), ERalpha and ERbeta. The expression of the two subtypes of ERs varies depending on the tissue. The overall objectives of this thesis were to study the functional importance of estrogen receptors in the periodontium with special focus on inflammation, and stimulators of inflammation and their signaling pathways. The thesis is based on the following five papers. In Paper I, effects of estrogen on E. coli LPS-induced PDL cell production of interleukin-6 (IL-6), monocyte chemoattractant protein-1 (MCP-1) and C-reactive protein (CRP) are assessed, by using ELISA. Furthermore, effects of LPS and estrogen on the normal characteristics of the PDL cell such as collagen synthesis and cell proliferation is determined by using L-[3H]proline incorporation and measurement of DNA synthesis, respectively.
E. coli LPS stimulates PDL cell IL-6 and MCP-1 production but has no effect on the normal physiological properties of PDL cells. LPS-induced IL-6 and MCP-1 is not reversed by estrogen suggesting that estrogen has no anti-inflammatory effect in these experiments. In Paper II, we investigate the effects of ovariectomy and aging on tooth attachment in female mice by using morphometric analysis.
Withdrawal of female sex hormone production by ovariectomy has no effect on alveolar bone height and apical termination of the junctional epithelium. In a second series of experiments these parameters are similar in mice sacrificed at 8-26 weeks of age, suggesting that tooth attachment is preserved with age in mice within a period of six months. In Paper III, the objective is to investigate the regulation of CCL2/MCP-1, CCL3/MIP-1alpha, and CCL5/RANTES chemokines by estrogen in human PDL cells by determining mRNA transcript levels (using quantitative real-time PCR) and protein levels (using ELISA).
A physiological concentration of estrogen reduces the expression of CCL3 mRNA by about 40% compared to PDL cells treated with LPS alone. In contrast, inter-individual differences in the effects of estrogen on CCL5 mRNA expression are observed. These findings indicate that estrogen affects chemokine expression in PDL cells showing a complex pattern involving down-regulation as well as up-regulation of chemokines. Estrogen exerts both anti-inflammatory and pro-inflammatory effects through these mechanisms. In Paper IV, ER expression in human gingival biopsies, and effects of estrogen on cultured gingival epithelial cell (HGEP) proliferation, are investigated. Expression of ERalpha and ERbeta is determined by immunohistochemistry and effects of estrogen on HGEP proliferation monitored by measuring DNA synthesis.
HGEP cells show strong ERbeta immunoreactivity but low ERalpha immunoreactivity both in vivo and in culture, suggesting that ERbeta is the predominant ER subtype in HGEP. High, but not low, concentrations of estrogen attenuates proliferation of gingival epithelial cells, indicating a concentration-dependent mechanism. In Paper V, the objective is to investigate the effects of LPS from Escherichia coli and Porphyromonas gingivalis on IL-6 production in human PDL cells and endothelial cells, and the signaling mechanisms involved. Quantitative real-time PCR is used to determine IL-6 mRNA levels and ELISA to determine IL-6 protein.
E. coli LPS (but not P. gingivalis LPS) stimulates IL-6 production in PDL cells. Treatment with the non-selective nitric oxide synthase inhibitor L-NAME reduces IL-6 by 30%, while aminoguanidine, an inhibitor of inducible nitric oxide synthase, does not affect IL-6 levels, showing a mechanism probably involving nitric oxide formation via endothelial nitric oxide synthase. Treatment with the glucocorticoid steroid dexamethasone totally prevents-E. coli LPS-induced IL-6 in PDL cells.
雌激素的主要功能与生殖相关。然而,雌激素在非经典靶器官中也具有重要功能。以往的研究,尤其是流行病学和临床研究,探讨了雌激素对牙周炎的影响,表明雌激素具有有益作用,但尚未确定其生物学机制。雌激素通过与核受体雌激素受体(ERs)、雌激素受体α(ERα)和雌激素受体β(ERβ)结合,在靶细胞中发挥基因组效应。两种ER亚型的表达因组织而异。本论文的总体目标是研究雌激素受体在牙周组织中的功能重要性,特别关注炎症、炎症刺激物及其信号通路。本论文基于以下五篇论文。在论文I中,通过酶联免疫吸附测定法(ELISA)评估雌激素对大肠杆菌脂多糖(LPS)诱导的牙周膜细胞产生白细胞介素-6(IL-6)、单核细胞趋化蛋白-1(MCP-1)和C反应蛋白(CRP)的影响。此外,分别通过L-[3H]脯氨酸掺入法和DNA合成测量法,确定LPS和雌激素对牙周膜细胞正常特性(如胶原蛋白合成和细胞增殖)的影响。
大肠杆菌LPS刺激牙周膜细胞产生IL-6和MCP-1,但对牙周膜细胞的正常生理特性无影响。雌激素不能逆转LPS诱导的IL-6和MCP-1,表明在这些实验中雌激素没有抗炎作用。在论文II中,我们通过形态计量分析研究卵巢切除和衰老对雌性小鼠牙齿附着的影响。
卵巢切除导致雌性性激素分泌减少,对牙槽骨高度和结合上皮根尖终止无影响。在第二系列实验中,8 - 26周龄处死的小鼠的这些参数相似,表明在六个月的时间段内,小鼠的牙齿附着随年龄增长得以保留。在论文III中,目的是通过测定mRNA转录水平(使用定量实时聚合酶链反应)和蛋白质水平(使用ELISA),研究雌激素对人牙周膜细胞中CCL2/MCP-1、CCL3/MIP-1α和CCL5/RANTES趋化因子的调节作用。
与单独用LPS处理的牙周膜细胞相比,生理浓度的雌激素使CCL3 mRNA表达降低约40%。相反,观察到雌激素对CCL5 mRNA表达的影响存在个体差异。这些发现表明雌激素影响牙周膜细胞中趋化因子的表达,呈现出涉及趋化因子下调和上调的复杂模式。雌激素通过这些机制发挥抗炎和促炎作用。在论文IV中,研究人牙龈活检组织中ER的表达以及雌激素对培养的牙龈上皮细胞(HGEP)增殖的影响。通过免疫组织化学法确定ERα和ERβ的表达,并通过测量DNA合成监测雌激素对HGEP增殖的影响。
HGEP细胞在体内和体外培养中均显示出强ERβ免疫反应性,但ERα免疫反应性低,表明ERβ是HGEP中主要的ER亚型。高浓度而非低浓度的雌激素减弱牙龈上皮细胞的增殖,表明存在浓度依赖性机制。在论文V中,目的是研究大肠杆菌和牙龈卟啉单胞菌的LPS对人牙周膜细胞和内皮细胞中IL-6产生的影响以及涉及的信号机制。使用定量实时聚合酶链反应确定IL-6 mRNA水平,使用ELISA确定IL-6蛋白水平。
大肠杆菌LPS(而非牙龈卟啉单胞菌LPS)刺激牙周膜细胞产生IL-6。用非选择性一氧化氮合酶抑制剂L-NAME处理可使IL-6降低30%,而诱导型一氧化氮合酶抑制剂氨基胍不影响IL-6水平,表明可能涉及通过内皮型一氧化氮合酶形成一氧化氮的机制。用糖皮质激素地塞米松处理可完全阻止大肠杆菌LPS诱导的牙周膜细胞产生IL-6。
