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Effects of monomeric acrylic embedding media on the antigenicity of two epitopes of the MIC2-encoded Ewing's sarcoma cell membrane antigen.

作者信息

Hamilton G, Hamilton B, Mallinger R

机构信息

I Surgical University Clinic, University of Vienna, Austria.

出版信息

Histochemistry. 1992;97(1):87-94. doi: 10.1007/BF00271286.

DOI:10.1007/BF00271286
PMID:1377663
Abstract

Comparative electron microscopic studies of pre- and postembedding immunolabeling experiments have shown that the antigenicity of some epitopes is lost during acrylic resin embedding of the respective tissues. In the present investigation we have tested the sensitivities of two embedding-labile epitopes (HBA-71 and HBA-45) of the Ewing's sarcoma-associated MIC2-encoded E2 antigen to the effects of the different treatment steps, which are necessary for the preparation of ultrathin sections. The extent of antigenic retention was quantitated using flow cytometry and enzyme-linked immunosorbent assays (ELISA) of tumor cell lines, thymocytes and cell membrane extracts. Fixation, dehydration and high temperature treatment of MIC2-positive cells showed only minor effects on the reactivity with the HBA-71 and HBA-45 antibodies. However, exposure of the cells to the monomeric acrylic resins LR White (LRW), LR Gold (LRG) and Lowicryl K4M at 4 degrees C for 2-18 h resulted in a significant reduction of the HBA-71 and HBA-45 reactivities. In contrast, the antigenicity of both epitopes was maintained during treatment with the apolar Lowicryl HM20 embedding medium under these non-polymerizing conditions. The resins have no direct effect on the HBA-71/HBA-45 antigen, since it could be extracted in intact form from membranes of native, but not of fixed, tumour cells using LRW for membrane solubilization. These data indicate that the HBA-71/HBA-45 antigen remains in the cell membrane and is indirectly influenced by the extraction/modification of adjacent membrane constituents. The adverse effects of the polymerization process, in the case of embedding at low temperature in Lowicryl HM20, destroyed MIC2-antigenicity.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

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2
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本文引用的文献

1
A simple post-embedding system for the rapid demonstration of tissue antigens under the electron microscope.一种用于在电子显微镜下快速显示组织抗原的简易包埋后系统。
Histochem J. 1983 Jun;15(6):543-55. doi: 10.1007/BF01954145.
2
Extraction of membrane lipids during fixation, dehydration and embedding of Acholeplasma laidlawii-cells for electron microscopy.在对莱氏无胆甾原体细胞进行电子显微镜观察的固定、脱水和包埋过程中膜脂的提取。
J Microsc. 1983 Feb;129(Pt 2):201-7. doi: 10.1111/j.1365-2818.1983.tb04174.x.
3
Dehydration and embedding temperatures affect the antigenic specificity of tubulin and immunolabeling by the protein A-colloidal gold technique.
脱水和包埋温度会影响微管蛋白的抗原特异性以及通过蛋白A-胶体金技术进行的免疫标记。
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Enhancement of structural preservation and immunocytochemical staining in low temperature embedded pancreatic tissue.低温包埋胰腺组织中结构保存和免疫细胞化学染色的增强
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Selective impairment of cell antigenicity by fixation.固定对细胞抗原性的选择性损伤。
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Use and abuse of LR White.LR White的使用与滥用。
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Post-embedding cytochemistry with gold-labelled reagents: a review.用金标试剂进行包埋后细胞化学:综述
J Microsc. 1986 Aug;143(Pt 2):125-37. doi: 10.1111/j.1365-2818.1986.tb02771.x.
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Fixation, processing, and immunochemical reagent effects on preservation of T-lymphocyte surface membrane antigens in paraffin-embedded tissue.固定、处理及免疫化学试剂对石蜡包埋组织中T淋巴细胞表面膜抗原保存的影响
J Histochem Cytochem. 1987 Nov;35(11):1329-38. doi: 10.1177/35.11.3309048.
10
Effect of tissue processing on colloidal gold cytochemistry.组织处理对胶体金细胞化学的影响。
J Histochem Cytochem. 1987 Sep;35(9):983-96. doi: 10.1177/35.9.3302022.