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用于免疫组织化学解读与诊断的苏木精和伊红复染方案

Hematoxylin and Eosin Counterstaining Protocol for Immunohistochemistry Interpretation and Diagnosis.

作者信息

Grosset Andrée-Anne, Loayza-Vega Kevin, Adam-Granger Éloïse, Birlea Mirela, Gilks Blake, Nguyen Bich, Soucy Geneviève, Tran-Thanh Danh, Albadine Roula, Trudel Dominique

机构信息

Centre de recherche du Centre Hospitalier de l'Université de Montréal (CRCHUM).

Institut du cancer de Montréal.

出版信息

Appl Immunohistochem Mol Morphol. 2019 Aug;27(7):558-563. doi: 10.1097/PAI.0000000000000626.

Abstract

Hematoxylin and eosin (H&E) staining is a well-established technique in histopathology. However, immunohistochemistry (IHC) interpretation is done exclusively with hematoxylin counterstaining. Our goal was to investigate the potential of H&E as counterstaining (H&E-IHC) to allow for visualization of a marker while confirming the diagnosis on the same slide. The quality of immunostaining and the fast-technical performance were the main criteria to select the final protocol. We stained multiple diagnostic tissues with class I IHC tests with different subcellular localization markers (anti-CK7, CK20, synaptophysin, CD20, HMB45, and Ki-67) and with double-staining on prostate tissues with anti-high molecular weight keratins/p63 (DAB detection) and p504s (alkaline phosphatase detection). To validate the efficacy of the counterstaining, we stained tissue microarrays from the Canadian Immunohistochemistry Quality Control (cIQc) with class II IHC tests (ER, PR, HER2, and p53 markers). Interobserver and intraobserver concordance was assessed by κ statistics. Excellent agreement of H&E-IHC interpretation was observed in comparison with standard IHC from our laboratory (κ, 0.87 to 1.00), and with the cIQc reference values (κ, 0.81 to 1.00). Interobserver and intraobserver agreement was excellent (κ, 0.89 to 1.00 and 0.87 to 1.00, respectively). We therefore show for the first time the potential of using H&E counterstaining for IHC interpretation. We recommend the H&E-IHC protocol to enhance diagnostic precision for the clinical workflow and research studies.

摘要

苏木精和伊红(H&E)染色是组织病理学中一项成熟的技术。然而,免疫组织化学(IHC)解读仅采用苏木精复染。我们的目标是研究将H&E用作复染(H&E-IHC)的潜力,以便在同一张载玻片上确认诊断的同时使标志物可视化。免疫染色质量和快速技术性能是选择最终方案的主要标准。我们用具有不同亚细胞定位标志物的I类IHC检测(抗CK7、CK20、突触素、CD20、HMB45和Ki-67)对多个诊断组织进行染色,并在前列腺组织上用抗高分子量角蛋白/p63(DAB检测)和p504s(碱性磷酸酶检测)进行双重染色。为了验证复染的效果,我们用II类IHC检测(ER、PR、HER2和p53标志物)对来自加拿大免疫组织化学质量控制(cIQc)的组织微阵列进行染色。通过κ统计评估观察者间和观察者内的一致性。与我们实验室的标准IHC(κ值为0.87至1.00)以及cIQc参考值(κ值为0.81至1.00)相比,观察到H&E-IHC解读具有极好的一致性。观察者间和观察者内的一致性均极佳(分别为κ值0.89至1.00和0.87至1.00)。因此,我们首次展示了将H&E复染用于IHC解读的潜力。我们推荐H&E-IHC方案,以提高临床工作流程和研究的诊断准确性。

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