3-Layer Immunoperoxidase Protocol Reaction, Endomucin, and Alpha-smooth Muscle Actin Detection

Rukaia Sheneeb, Fawzia Takala
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Abstract

Background and objectives. Immunohistochemistry (IHC) is the detection of antigens in tissue sections by specific antibodies. It has the unique advantage over other methods for detection proteins like α-Smooth Muscle Actin and endomucin, enabling the correlation of antigens with their location within a tissue. The aim of the study was to identify α-SMA and endomucin in cardiac muscle tissue and arterial blood vessels which have important diagnostic purposes. Methods. Three Specimens (aSMA, Endomucin and control) of formalin-fixed paraffin embedded mouse embryo tissue sections have been de-waxed, rehydrated. Then they were covered with accurate primary antibody: αSMA slide in dilute mouse monoclonal anti-smooth muscle actin, Endomucin slide in dilute rat monoclonal anti-endomucin and the control slide gets just PBS (no-primary control). Then the sections were covered with the right secondary antibody: αSMA slide with biotinylated rabbit anti-mouse IgGIgG diluted and Endomucin slide with biotinylated rabbit anti-rat IgG, control slide with either antibody. Next color reagent was applied; it contains 3,3′-Diaminobenzidine and 0.3% hydrogen peroxide. Finally examine slides using a microscope. Results. The results showed that there was different brown 3,3′-Diaminobenzidine staining patterns in the two test slides for the individual primary antibodies. The 3,3′-Diaminobenzidine Staining was highly expressed in the external part of the section as a result of the presence of α-Smooth Muscle Actin. Whereas, in case of Endomucin, the stain is expressed in the central part of specimens due to presence of the endothelial tissue. and no staining in the primary control sections. Conclusion. As a result of the presence of α-Smooth Muscle Actin in the muscular tissue,3,3′-Diaminobenzidine Staining was highly expressed in the external part of the section. However, in case of Endomucin the stain is expressed in the central part of specimens due to presence of the endothelial tissue.
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三层免疫过氧化物酶方案反应,内啡肽和α -平滑肌肌动蛋白检测
背景和目标。免疫组织化学(IHC)是通过特异性抗体检测组织切片中的抗原。与其他检测蛋白质的方法相比,它具有独特的优势,如α-平滑肌肌动蛋白和内啡肽,可以将抗原与其在组织中的位置联系起来。本研究的目的是鉴定心肌组织和动脉血管中的α-SMA和内啡肽,这两种蛋白具有重要的诊断意义。方法。对福尔马林固定石蜡包埋的小鼠胚胎组织切片进行脱蜡、复水处理,分别为aSMA、Endomucin和对照。然后涂上精确的一抗:稀释小鼠单克隆抗平滑肌肌动蛋白αSMA玻片,稀释大鼠单克隆抗内啡肽Endomucin玻片,对照玻片只涂PBS(无一抗)。然后涂上正确的二抗:αSMA玻片加生物素化兔抗小鼠IgGIgG稀释,Endomucin玻片加生物素化兔抗大鼠IgG稀释,对照玻片加任意一种抗体。下一道显色剂;它含有3,3 ' -二氨基联苯胺和0.3%的过氧化氢。最后用显微镜检查载玻片。结果。结果显示,两种载玻片中,单个一抗存在不同的棕色3,3 ' -二氨基苯胺染色模式。由于α-平滑肌肌动蛋白的存在,3,3′-二氨基苯胺染色在切片的外部高度表达。然而,在Endomucin的情况下,由于内皮组织的存在,染色在标本的中心部分表达。主对照切片未见染色。结论。由于肌肉组织中α-平滑肌肌动蛋白的存在,3,3 ' -二氨基苯丙胺染色在切片外侧高度表达。然而,在Endomucin的情况下,由于内皮组织的存在,染色在标本的中心部分表达。
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