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Introducing a Rapid and Safe Method for Myeloperoxidase Staining

机译:介绍一种快速安全的髓过氧化物酶染色方法

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Background: Myeloperoxidase staining is used to differentiate leukemias since several decades. Despite implementation of flow cytometric, cytogenetic and molecular techniques for identification of leukemic blasts, histochemical stains such as myeloperoxidase stain are persistently used for better classification of leukemias. The myeloperoxidase staining is a time consuming and hazardous procedure. The present report describes a sensitive, rapid and easy method for assessment of peroxidase activity. Materials and Methods: Bone marrow aspiration slides were stained with Dako product: Code number: K3467 containing DAB chromogen (3,3-diaminobenzidine in chromogen solution) and substrate buffer (Imidasole-HCL buffer, PH 7.5 containing hydrogen peroxide and an anti microbial agent) in a rapid procedure taking only ten minutes time. The staining needs no material preparation steps. Neutrophils in the slide are taken as positive control or another normal smear was costained to be used as control. All cases were followed up with flow cytometry and cytogenetic studies. Result: The reaction product of this stain is brown and granular. Promyelocytes and myelocytes are the most strongly staining cells with positive (primary) granules. Lymphoblasts are negative. The result of classification of leukemias with this technique was in concordance with flow cytometric immunophenotyping. Discussion: Many practical techniques have been described using benzidine as an indicator for myeloperoxidase staining. Benzidine is a carcinogenic material and its usage is severely restricted in laboratory. Formerly we prepared requisite materials for myeloperoxidase staining by hazardous ways (boiling), but we decided to apply ready to use 3,3-diaminobenzidine (DAB), which is used in final step of immunohistochemistry stains. Conclusion: Use of 3,3-diaminobenzidine (DAB) is highly recommended for myeloperoxidase staining, while the result is extraordinary and fully compatible with flow cytometry and the method is safe and rapid.
机译:背景:髓过氧化物酶染色自几十年来一直用于区分白血病。尽管实施了流式细胞术,细胞遗传学和分子技术来鉴定白血病母细胞,但仍坚持使用组织化学染色剂如髓过氧化物酶染色剂来更好地分类白血病。髓过氧化物酶染色是耗时且危险的过程。本报告介绍了一种评估过氧化物酶活性的灵敏,快速,简便的方法。材料和方法:用Dako产品对骨髓吸出玻片进行染色:货号:K3467,其中含有DAB色原(在色原溶液中的3,3-二氨基联苯胺)和底物缓冲液(咪达唑-HCL缓冲液,PH 7.5包含过氧化氢和抗微生物剂) ),只需十分钟即可完成。染色不需要材料准备步骤。将载玻片中的嗜中性粒细胞作为阳性对照,或将另一正常涂片染色作为对照。所有病例均进行了流式细胞术和细胞遗传学研究。结果:该污渍的反应产物为褐色和颗粒状。早幼粒细胞和骨髓细胞是染色最强的阳性(初级)颗粒细胞。淋巴母细胞是阴性的。用这种技术对白血病进行分类的结果与流式细胞仪免疫表型一致。讨论:已经描述了许多使用联苯胺作为髓过氧化物酶染色指示剂的实用技术。联苯胺是一种致癌物质,在实验室中其使用受到严格限制。以前,我们通过危险方式(沸腾)为髓过氧化物酶染色准备了必要的材料,但我们决定立即使用3,3-二氨基联苯胺(DAB),将其用于免疫组化染色的最后一步。结论:强烈建议使用3,3-二氨基联苯胺(DAB)进行髓过氧化物酶染色,其结果非同凡响,与流式细胞仪完全兼容,该方法安全,快速。

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