关于牙本质屏障的修复。

Swedish dental journal. Supplement Pub Date : 2012-01-01
Helena Fransson
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引用次数: 0

摘要

本论文的总体目的是研究牙本质屏障修复的某些方面,特别是与牙髓盖合在一起。了解导致牙本质和牙髓愈合的事件,从而成功地保持牙齿的活力和功能,将为比进行根管治疗更具侵入性的牙髓暴露治疗提供科学依据。人体表面具有生理屏障功能,旨在保护身体免受外部有害物质的侵害。在牙齿中,排列在牙髓最外层的成牙细胞负责形成牙本质,在牙齿的屏障功能中起着核心作用,因此在牙齿的防御机制中起着重要作用。龋损内的微生物可经由牙本质小管到达牙髓。然而,屏障功能有助于防止微生物入侵,从而避免有害的炎症和随后的牙髓坏死。牙本质修复是牙本质屏障功能的重要组成部分。然而,对于这种修复是否也会导致功能的恢复以及长期抵抗细菌涌入的能力,人们仍有疑问。牙髓盖盖是一种在牙髓外露时使用的治疗方法,目的是刺激牙髓和牙本质愈合。对人类牙髓盖盖后牙本质修复的证据进行了系统的综述。文献检索的重点是在显微镜下研究人体硬组织形成的研究。基于现有的有限证据,我们得出结论,氢氧化钙基材料而不是结合剂促进硬组织桥的形成。在这方面,MTA是否优于氢氧化钙基材料缺乏科学证据。一种含有淀粉原蛋白的凝胶(Emdogain凝胶),已知与牙本质形成有关,在临床研究中对硬组织的形成进行了评估。与对照组相比,应用凝胶后形成了更多的硬组织。根据其1型胶原蛋白和牙本质唾液蛋白的含量,该组织的特征推断为牙本质,尽管它不是作为覆盖牙髓伤口的连续桥而形成的。在深龋损伤下,屏障功能的一个重要部分是成牙本质细胞对细菌的反应,形成新的牙本质。采用成牙细胞细胞模型研究了深部龋齿临床分离物对其生存能力和1型胶原生成的影响,1型胶原是牙本质形成早期的主要成分。有细菌对成牙细胞样细胞的活力产生负面影响,不同细菌对1型胶原蛋白产生的影响不同,这表明一些细菌可能直接影响成牙细胞形成牙本质的能力。在总结;Emdogain凝胶启动了牙本质的形成,尽管不是以一种可以构成屏障的形式,并且有迹象表明细菌可能会不同地影响成牙本质细胞修复牙本质屏障的能力。
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On the repair of the dentine barrier.

The overall aim of this thesis was to study some aspects of the repair of the dentine barrier, especially in conjunction with dental pulp capping. Understanding the events leading to the healing of the dentine and pulp, and hence successfully preserving the vitality and functions of the tooth, would lead to a scientific basis for a less invasive treatment of pulp exposures than performing root canal treatments. The surfaces of the body have physiological barrier functions aimed at protecting the body from external noxious agents. In the tooth, the odontoblasts, which line the outermost part of the pulp and are responsible for the formation of dentine, play a central role in the barrier function and thus in the defence mechanisms of the tooth. The micro-organisms in the caries lesion can reach the pulp via the dentinal tubules. However, the barrier function helps to prevent microbial invasion and thereby avoid deleterious inflammation and subsequent necrosis of the pulp. Dentine repair is an important part of the barrier function. There are however doubts as to whether the repair also leads to restitution of the function and the ability to withstand bacterial influx over the longer term. Pulp capping is a treatment method used when the pulp has been exposed in order to stimulate healing of the pulp and dentine. The evidence for repair of the dentine after pulp capping in humans has been studied by means of a systematic review. The focus of the literature search was studies performed in humans where hard tissue formation had been studied with the aid of a microscope. We concluded, based on the limited evidence available, that calcium hydroxide based materials but not bonding agents promote formation of a hard tissue bridge. Scientific evidence was lacking as to whether MTA was better than calcium hydroxide based materials in this regard. A gel (Emdogain Gel) containing amelogenin, known to be involved in dentinogenesis, was evaluated with regard to formation of hard tissue in a clinical study. A greater amount of hard tissue was formed after application of the gel compared to the control. Characterization of the tissue concluded it to be dentine, based on its content of type 1 collagen and dentine sialoprotein, although it was not formed as a continuous bridge covering the pulp wound. Beneath a deep caries lesion an important part of the barrier function is the odontoblasts' response to bacteria with the formation of new dentine. A cell model with odontoblasts was used to study the effects of clinical isolates from a deep carious lesion on their viability and production of type 1 collagen, the major component of the dentine in the early stages of its formation. There were bacteria that negatively affected the viability of the odontoblast-like cells and different bacteria varied in their effects on type 1 collagen production, suggesting that some bacteria may have a direct influence on the odontoblasts' ability to form dentine. In summary; Emdogain Gel initiated dentine formation, though not in a form that could constitute a barrier and there are indications that bacteria may differentially affect the odontoblasts' ability to repair the dentine barrier.

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