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与新鲜混合的牙髓材料接触培养的细胞中前列腺素E的产生及细胞活力

Prostaglandin E production and viability of cells cultured in contact with freshly mixed endodontic materials.

作者信息

Melegari K K, Botero T M, Holland G R

机构信息

Department of Cariology, Restorative Sciences, and Endodontics, University of Michigan, School of Dentistry, Ann Arbor, MI 48109-1078, USA.

出版信息

Int Endod J. 2006 May;39(5):357-62. doi: 10.1111/j.1365-2591.2006.01070.x.

DOI:10.1111/j.1365-2591.2006.01070.x
PMID:16640633
Abstract

AIM

To determine whether commonly used endodontic sealers could either induce or increase the release of prostaglandin E2 (PGE2) when in contact with cell types found in the periapical tissues.

METHODOLOGY

Freshly mixed samples of Roth 801 sealer, Sealapex and ProRoot mineral trioxide aggregate (MTA) were placed in contact with cultured macrophages and fibroblasts for 24 h. The supernatant from the cultures was assayed for PGE2 using enzyme-linked immunosorbent assay. Cell viability counts were made. As a positive control, similar cultures were also exposed to lipopolysaccharide and the supernatant analysed for PGE2. Data were compared by anova.

RESULTS

The three materials examined in these experiments did not stimulate increased PGE2 release from either of the cell lines. In control cultures, lipopolysaccharide increased PGE2 release from macrophages but not from fibroblasts. Viability counts revealed that, whilst Roth 801 sealer caused some cell death in both fibroblasts and macrophages, Sealapex led to cell death only in the macrophage cultures. ProRoot MTA did not lead to statistically significant cell death in either culture.

CONCLUSIONS

Under 24-h culture conditions, the three freshly mixed test materials did not increase directly either production or release of PGE2 from either macrophages or gingival fibroblasts. Roth 801 decreased cell viability counts for both fibroblasts and macrophages. Sealapex decreases macrophage viability. ProRoot MTA did not affect viability in either cell line.

摘要

目的

确定常用的根管封闭剂在与根尖周组织中发现的细胞类型接触时,是否会诱导或增加前列腺素E2(PGE2)的释放。

方法

将新鲜混合的Roth 801封闭剂、Sealapex和ProRoot三氧化矿物凝聚体(MTA)样本与培养的巨噬细胞和成纤维细胞接触24小时。使用酶联免疫吸附测定法检测培养物上清液中的PGE2。进行细胞活力计数。作为阳性对照,类似的培养物也暴露于脂多糖,并分析上清液中的PGE2。数据通过方差分析进行比较。

结果

在这些实验中检测的三种材料均未刺激两种细胞系中PGE2释放增加。在对照培养物中,脂多糖增加了巨噬细胞中PGE2的释放,但未增加成纤维细胞中PGE2的释放。活力计数显示,虽然Roth 801封闭剂在成纤维细胞和巨噬细胞中均导致了一些细胞死亡,但Sealapex仅在巨噬细胞培养物中导致细胞死亡。ProRoot MTA在两种培养物中均未导致具有统计学意义的细胞死亡。

结论

在24小时培养条件下,三种新鲜混合的测试材料均未直接增加巨噬细胞或牙龈成纤维细胞中PGE2的产生或释放。Roth 801降低了成纤维细胞和巨噬细胞的活力计数。Sealapex降低了巨噬细胞的活力。ProRoot MTA对两种细胞系的活力均无影响。

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