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大鼠切牙釉质器分泌区中辣根过氧化物酶的命运

Fate of horseradish peroxidase in the secretion zone of the rat incisor enamel organ.

作者信息

Kallenbach E

出版信息

Tissue Cell. 1980;12(3):491-501. doi: 10.1016/0040-8166(80)90038-5.

Abstract

Adult CDF albino rats were killed from 10 min to 6 hr after a single intravenous dose of HRP. Experimental and control tissues were reacted for peroxidase activity and processed for light and electron microscopy. At 10 min, all extracellular spaces of the secretion zone showed reaction product. A reaction was also seen around Tomes' processes and in a layer of enamel spaces in the region of thin enamel. At later times intervals, reactions around Tomes' processes were also seen in regions of thicker enamel. Tracer was located preferentially at the growth fronts of rod and interrod enamel, and also diffused for some distance into enamel. From 2 to 6 hr, the enamel over the transition zone became heavily labeled. The tracer penetrated for more than 90 micrometer into the enamel and was localized mainly in the interrod enamel. Droplets of dense stippled material in the extracellular spaces between Tomes' processes did not mix with tracer, but sites which contain a light stippled material in the controls (extracellular spaces, vesicles within ameloblasts) showed a reaction. It is concluded that (1) the basal terminal bars of secretory ameloblasts do not impede the flow of large molecules, (2) the apical terminal bars are permeable in early secretion, become increasingly tight as secretion progresses, and are again permeable in the transition zone, (3) ameloblasts can shuttle large extracellular molecules towards the enamel growth fronts, (4) large molecules can diffuse into enamel; rod and interrod enamel differ with regard to the diffusion of large molecules, (5) ameloblasts phagocytose significant amounts of light stippled material. The possibility is considered that extracellular enamel precursor molecules move preferentially towards the enamel growth fronts, perhaps by a mechanism involving membrane flow, and diffuse through enamel in similar fashion as HRP.

摘要

成年CDF白化大鼠在单次静脉注射辣根过氧化物酶(HRP)后10分钟至6小时内处死。对实验组织和对照组织进行过氧化物酶活性反应,并进行光镜和电镜处理。10分钟时,分泌区的所有细胞外间隙均显示出反应产物。在托姆斯突周围以及薄釉质区域的一层釉质间隙中也可见反应。在随后的时间间隔内,在较厚釉质区域的托姆斯突周围也可见反应。示踪剂优先位于釉柱和柱间质釉质的生长前沿,并且也扩散到釉质中一段距离。从2小时到6小时,过渡区上方的釉质被大量标记。示踪剂穿透釉质超过90微米,主要定位于柱间质釉质中。托姆斯突之间细胞外间隙中的密集点状物质小滴不与示踪剂混合,但对照中含有轻度点状物质的部位(细胞外间隙、成釉细胞内的小泡)显示出反应。得出以下结论:(1)分泌期成釉细胞的基底终末杆不阻碍大分子的流动;(2)顶端终末杆在早期分泌时是可渗透的,随着分泌的进行变得越来越紧密,在过渡区再次变得可渗透;(3)成釉细胞可以将大的细胞外分子向釉质生长前沿运输;(4)大分子可以扩散到釉质中;釉柱和柱间质釉质在大分子扩散方面存在差异;(5)成釉细胞吞噬大量轻度点状物质。考虑到细胞外釉质前体分子可能优先向釉质生长前沿移动,也许是通过一种涉及膜流动的机制,并以与HRP相似的方式扩散通过釉质。

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