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引用次数: 0
摘要
通过免疫组化鉴定 CD30 的表达对于使用 CD30 靶向抗体-药物共轭物治疗淋巴瘤至关重要。然而,目前还没有标准化的 CD30 染色方案。在这项研究中,我们比较了三种常见的自动免疫染色平台{Bond III (B III)、Dako Omnis (DO) 和 Ventana BenchMark ULTRA (VBMU)}。B III 和 DO 使用的是稀释 50-400 倍的 CD30 一抗(Ber-H2 克隆),VBMU 使用的是即用型抗体。所有方案中都引入了使用连接剂的增强步骤。首先,通过对六个病例进行染色,为每个平台挑选出几个候选稀释度。然后用 60 例各种类型的外周 T 细胞淋巴瘤(PTCL)来确认这些候选条件。除无性大细胞淋巴瘤外,不同平台的 CD30 表达一致性因截断值和抗体稀释度的不同而不同。如果在 B III 中使用 400 稀释的抗体,在 DO 中使用 100 稀释的抗体,那么当临界值分别为 1%和 10%时,三个平台评价 "阳性 "或 "阴性 "的一致率分别为 100%和 97%。该研究证明了通过调整方案在不同平台间实现 PTCL CD30 染色均等化的可行性。
Standardization of CD30 immunohistochemistry staining among three automated immunostaining platforms.
The identification of CD30 expression by immunohistochemistry is essential for the treatment of lymphomas using an antibody-drug conjugate targeting CD30. However, no standardized protocol for CD30 staining has been available. In this study, we compared three common automated immunostaining platforms {Bond III (B III), Dako Omnis (DO) and Ventana BenchMark ULTRA (VBMU)}. A primary antibody for CD30, the Ber-H2 clone, was diluted 50- to 400-fold for B III and DO, and ready-to-use antibody was used for VBMU. An enhancement step using a linker was introduced in all protocols. First, several candidate dilutions were selected for each platform by staining six cases. These candidate conditions were then confirmed with 60 cases of various types of peripheral T-cell lymphomas (PTCLs). The concordance rates of CD30 expression among platforms differed depending on cutoff values and antibody dilutions, except for anaplastic large cell lymphoma. The concordance rates among three platforms in the evaluation of "positive" or "negative" were 100% and 97% when the cutoff values were 1% and 10% respectively, if using 400-diluted antibody in B III and 100-diluted antibody in DO. This study demonstrated the feasibility of equalizing CD30 staining of PTCLs among different platforms by adjusting protocols.
期刊介绍:
Pathology International is the official English journal of the Japanese Society of Pathology, publishing articles of excellence in human and experimental pathology. The Journal focuses on the morphological study of the disease process and/or mechanisms. For human pathology, morphological investigation receives priority but manuscripts describing the result of any ancillary methods (cellular, chemical, immunological and molecular biological) that complement the morphology are accepted. Manuscript on experimental pathology that approach pathologenesis or mechanisms of disease processes are expected to report on the data obtained from models using cellular, biochemical, molecular biological, animal, immunological or other methods in conjunction with morphology. Manuscripts that report data on laboratory medicine (clinical pathology) without significant morphological contribution are not accepted.