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长期氟暴露对定义大鼠切牙釉质形成阶段和成釉细胞调节的形态计量学参数的影响。

Effects of chronic fluoride exposure on morphometric parameters defining the stages of amelogenesis and ameloblast modulation in rat incisors.

作者信息

Smith C E, Nanci A, Denbesten P K

机构信息

Department of Anatomy and Cell Biology, McGill University, Montreal, Canada.

出版信息

Anat Rec. 1993 Oct;237(2):243-58. doi: 10.1002/ar.1092370212.

Abstract

The response of ameloblasts to long-term (6 weeks) exposure to 100 ppm fluoride was examined in continuously erupting mandibular incisors of female Sprague-Dawley rats as compared to control rats receiving a similar diet (Teklad L-356) but no sodium fluoride in their drinking water. After treatment, animals from both groups were perfused intravascularly with glutaraldehyde, and the incisors were removed and processed for light microscope morphometric analyses directly from 1 microns thick Epon sections. Other animals were injected intravenously with calcein (green fluorescence) followed 4 hours later by xylenol orange (red fluorescence) in order to reveal smooth-ended ameloblast modulation bands and thereby allow quantification of parameters related to the creation and movement of modulation waves within the maturation zone of these teeth. The results indicated that rat incisors expressed four major changes in normal amelogenesis which could be attributed to the chronic fluoride treatment. First, ameloblasts produced a thinner than normal enamel layer by the time they completed the secretory stage and entered the maturation stage of amelogenesis. Second, enamel organ cells within the maturation zone, especially those from the papillary layer, were shorter in height than normal. Third, ameloblasts related to maturing enamel in areas where it was partially soluble and/or fully soluble in EDTA modulated at a rate that was much slower than normal. In some locations ameloblasts remained ruffle-ended for as much as 30% longer than normal per cycle. This upset the usual pattern such that fewer total modulation cycles were completed per unit time by these ameloblasts. Fourth, enamel proteins were lost from the maturing enamel layer at a rate that was about 40% slower than normal. The data suggested that ameloblasts detected the delay in the extracellular breakdown and/or loss of enamel proteins and they responded by remaining ruffle-ended for longer intervals than usual (positive feedback).

摘要

在雌性斯普拉格-道利大鼠持续萌出的下颌切牙中,研究了成釉细胞对长期(6周)暴露于100 ppm氟的反应,并与接受相似饮食(Teklad L-356)但饮用水中不添加氟化钠的对照大鼠进行比较。处理后,两组动物均通过血管内灌注戊二醛,然后取出切牙,直接从1微米厚的环氧树脂切片进行光镜形态计量分析。其他动物静脉注射钙黄绿素(绿色荧光),4小时后再注射二甲酚橙(红色荧光),以显示平滑末端的成釉细胞调制带,从而能够对与这些牙齿成熟区内调制波的产生和移动相关的参数进行量化。结果表明,大鼠切牙在正常釉质形成过程中表现出四种主要变化,这可归因于慢性氟处理。第一,成釉细胞在完成分泌阶段并进入釉质形成的成熟阶段时,产生的釉质层比正常的薄。第二,成熟区内的釉器细胞,尤其是来自乳头层的细胞,高度比正常的短。第三,在部分可溶于乙二胺四乙酸(EDTA)和/或完全可溶于EDTA的成熟釉质区域,与之相关的成釉细胞调制速度比正常慢得多。在某些位置,成釉细胞每个周期保持皱折末端的时间比正常情况长多达30%。这扰乱了通常的模式,使得这些成釉细胞每单位时间完成的总调制周期减少。第四,成熟釉质层中釉质蛋白的流失速度比正常情况慢约40%。数据表明,成釉细胞检测到细胞外釉质蛋白分解和/或流失的延迟,并通过比正常情况更长时间地保持皱折末端做出反应(正反馈)。

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