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荧光显微镜原位观察初始生物黏附过程中非细胞成分的可视化。

Fluorescence microscopic visualization of non cellular components during initial bioadhesion in situ.

机构信息

Clinic of Operative Dentistry, Medical Faculty Carl Gustav Carus, TU Dresden, Fetscherstr. 74, D-01307 Dresden, Germany.

出版信息

Arch Oral Biol. 2013 Oct;58(10):1271-81. doi: 10.1016/j.archoralbio.2013.07.006. Epub 2013 Aug 23.

DOI:10.1016/j.archoralbio.2013.07.006
PMID:24011302
Abstract

OBJECTIVE

The formation of an intraoral biofilm is primarily determined by initial bioadhesion processes, including molecular interactions. Therefore, this study aimed to establish fluorescent labelling protocols to enable the simultaneous visualization of different pellicle enzymes, extracellular glucans and adherent bacteria throughout the initial phase of biofilm formation.

DESIGN

In situ formed biofilm samples were collected on enamel and dentine slabs that were fixed on buccal sites of individual splints, being worn by 5 subjects. After an intraoral slab exposure from 30min to 8h, the following specially adapted fluorescent labelling assays were performed and analyzed by epifluorescent microscopy: pellicle-amylase, -lysozyme, -peroxidase and -glycosyltransferases B, C and D were marked with specific primary antibodies and then visualized by the aid of different fluorescently labelled secondary antibodies (Texas Red, DyLight 488, FITC). Afterwards the same samples were subjected to a combined DAPI-/Concanavalin A-staining to determine adherent bacteria and glucans.

RESULTS

All fluorescence labelling assays were successfully established to visualize pellicle enzymes, glucans and adherent bacteria at different times of biofilm formation. The combination of the labelling protocols showed a characteristic agglomeration of glucans and bacteria as well as an increased concentration of the pellicle enzymes in the initial phase of bioadhesion.

CONCLUSION

Fluorescent labelling techniques are a valuable supplement of dental research as they provide an insight into the mutual interactions of different biofilm determinants in situ. Based hereon, information could also be deduced about the influence of oral therapeutics on individual caries susceptibility.

摘要

目的

口腔生物膜的形成主要取决于初始生物附着过程,包括分子相互作用。因此,本研究旨在建立荧光标记方案,以实现不同菌膜酶、细胞外葡聚糖和附着细菌在生物膜形成初始阶段的同时可视化。

设计

在釉质和牙本质平板上收集原位形成的生物膜样本,将平板固定在个别夹板的颊侧部位,由 5 名受试者佩戴。在口腔平板暴露 30 分钟至 8 小时后,进行以下特别适应的荧光标记测定,并通过荧光显微镜分析:用特异性的一抗标记菌膜 -淀粉酶、-溶菌酶、-过氧化物酶和 -糖基转移酶 B、C 和 D,然后借助不同的荧光标记二抗(Texas Red、DyLight 488、FITC)进行可视化。之后,对相同的样本进行 DAPI-/伴刀豆球蛋白 A 染色,以确定附着的细菌和葡聚糖。

结果

所有荧光标记测定均成功建立,以在生物膜形成的不同时间可视化菌膜酶、葡聚糖和附着的细菌。标记方案的组合显示了葡聚糖和细菌的特征聚集,以及初始生物附着阶段菌膜酶浓度的增加。

结论

荧光标记技术是牙科研究的有价值的补充,因为它们提供了对不同生物膜决定因素在原位相互作用的深入了解。在此基础上,还可以推断口腔治疗对个体龋易感性的影响。

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