槟榔生物碱对人牙龈、正常颊黏膜和口腔黏膜下纤维化成纤维细胞体外产生白细胞介素-6的研究

C C Chen, J F Huang, C C Tsai
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引用次数: 0

摘要

本研究旨在探讨槟榔碱和槟榔碱对体外培养的人正常牙龈、口腔黏膜和口腔粘膜下纤维化(OSF)成纤维细胞增殖和白细胞介素-6 (IL-6)产生的直接影响。将成纤维细胞融合单层在含有或不含生物碱的情况下,在含有10%胎牛血清的条件下,于37℃、5% CO2和空气中孵育48小时。在培养期结束时,收集上清液,检测IL-6水平。通过测定细胞DNA中5-溴-2′-脱氧尿苷(BrdU)的掺入量来监测细胞增殖。除槟榔碱在100微克/毫升时抑制细胞生长外,槟榔碱和槟榔碱对三组成纤维细胞的增殖具有相似的剂量依赖性刺激作用。对照培养上清液中IL-6的浓度在健康牙龈成纤维细胞中最高,其次是正常颊黏膜和OSF。此外,胎牛血清的存在可以刺激IL-6的释放。除槟榔碱浓度为100微克/毫克外,同一组中处理组与对照培养组之间IL-6水平以平均+/- sd表达时无显著差异。然而,6名个体中有2名正常颊黏膜成纤维细胞释放的IL-6明显减少,而一些OSF病例和健康牙龈在培养细胞暴露于槟榔碱或槟榔碱时,IL-6水平略高。提示槟榔碱和槟榔碱能促进细胞增殖,影响成纤维细胞合成IL-6。此外,IL-6可能是OSF病理特征的一个分子因素。
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In vitro production of interleukin-6 by human gingival, normal buccal mucosa, and oral submucous fibrosis fibroblasts treated with betel-nut alkaloids.

This study aimed to assess the possibility of a direct effect of betel-nut alkaloids arecoline and arecaidine on cell proliferation and interleukin-6 (IL-6) production by cultured fibroblasts from human normal gingiva, buccal mucosa and oral submucous fibrosis (OSF) buccal mucosa in vitro. Confluent monolayers of fibroblasts were incubated with or without alkaloids in the presence of 10% fetal calf serum for 48 h at 37 degree C in 5% CO2 and air. At the end of the culture period, supernatants were collected and assayed for IL-6 level. The cell proliferation was monitored by determining 5-bromo-2'-deoxy-uridine (BrdU) incorporated into cellular DNA. Except for the fact that arecoline inhibited cell growth at 100 micrograms/ml, arecoline and arecaidine had similar dose-dependent stimulant effects on the proliferation of these three groups fibroblasts. Concentrations of IL-6 in the control culture supernatants were greatest in healthy gingival fibroblasts, followed by normal buccal mucosa and OSF. Also, the presence of fetal calf serum could stimulate IL-6 release. Except for arecoline at the 100 microgram/mg, there were no significant differences in IL-6 levels between treated and control cultures of the same group when the data were expressed with mean +/- S.D.. However, two of six individuals' normal buccal mucosa fibroblasts significantly released less IL-6, and some cases of OSF and healthy gingiva exhibited slightly higher levels of IL-6 when cells were exposed to arecoline or arecaidine in cultures. Such findings suggests that arecoline and arecaidine can enhance cell proliferation and affect fibroblasts to synthesize IL-6. Furthermore, IL-6 may be a contributing molecular factor in the pathological features noted in OSF.

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