Histological preparation of implanted biomaterials for light microscopic evaluation of the implant-tissue interaction.

E Murice-Lambert, A B Banford, R L Folger
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引用次数: 28

Abstract

A technique is presented for processing implanted biomaterials with surrounding soft tissue for histological assessment of the implant-tissue interaction. Specimens are removed with the implant-tissue interface intact, fixed in formalin, dehydrated in a graded series of ethanol followed by a graded series of acetone in ethanol, and embedded in Spurr's low viscosity epoxy resin. Sections 0.5-1.0 mm thick are cut from the cured blocks using a metallurigical saw with a diamond wafer blade. After being glued to glass microscope slides, they are ground and polished to approximately 75 microns in thickness. The polished sections are treated with 95% ethanol saturated with sodium hydroxide, stained with Gill's hematoxylin and counterstained in eosin Y-phloxine B. The sodium hydroxide solution degrades the resin, allowing the stain to penetrate the tissue. By limiting the time in sodium hydroxide, the depth of staining is controlled and one is able to simulate a thin paraffin section with high resolution of the implant-soft tissue interface.

植入生物材料的组织学准备,用于植入物与组织相互作用的光镜评估。
提出了一种处理植入生物材料与周围软组织的技术,用于植入物与组织相互作用的组织学评估。标本在植入物-组织界面完整的情况下取出,在福尔马林中固定,在分级系列乙醇中脱水,然后在乙醇中分级系列丙酮中脱水,然后嵌入spr的低粘度环氧树脂中。用带金刚石片刀片的冶金锯从固化块上切下0.5-1.0毫米厚的部分。在被粘到玻璃显微镜载玻片上后,它们被研磨和抛光到大约75微米的厚度。抛光后的切片用饱和氢氧化钠的95%乙醇处理,用吉尔苏木精染色,并用伊红y -苯氧辛b反染色。氢氧化钠溶液降解树脂,使染色渗入组织。通过限制在氢氧化钠中的时间,可以控制染色深度,并且可以模拟具有高分辨率的种植体-软组织界面的薄石蜡切片。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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