实体肿瘤中FGFR2b蛋白表达的精确检测：通过自动化免疫组织化学对染色参数的综合评估

Archives of pathology & laboratory medicine Pub Date : 2025-05-06 DOI:10.5858/arpa.2024-0497-OA

Autumn Sky Watson, Catherine Le, Anne Wertheimer, Spencer Escobedo, Lisa So, Bhavani Bagevalu Siddegowda, John Palting, Susan Marion, Steven P Stratton, Birte Aggeler

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引用次数: 0

摘要

上下文。-：免疫组织化学有效地揭示了成纤维细胞生长因子受体2b （FGFR2b）在不同肿瘤组织类型中的表达和抗原可及性的异质性，这种差异性受到组织类型和固定质量的显著影响，这两者都深刻影响了福尔马林固定石蜡包埋（FFPE）组织标本中靶抗原的可及性。自动染色平台上的检索参数会影响染色结果和测定灵敏度。对染色程序进行了全面优化，包括抗原提取、蛋白水解酶消化、一抗孵育和检测选择，产生了针对特定肿瘤类型设计的两种不同方案。两种方案均针对各自的肿瘤类型进行了优化，其中一种方案针对胃和胃食管交界（G/GEJ）腺癌进行了优化，另一种方案针对非小细胞肺癌（NSCLC）和更广泛的实体肿瘤进行了微调。-：通过修改已建立的VENTANA FGFR2b （FPR2-D）小鼠单克隆抗体检测，优化用于非小细胞肺癌和更广泛实体肿瘤的FGFR2b （FPR2-D）检测，该检测最初用于G/GEJ腺癌。-：多种FGFR2b检测方案用于对10种肿瘤类型的商业采购标本的FFPE组织切片进行染色。对每个标本进行评估，以选择在最小背景下实现强特异性染色的首选方案参数。然后评估该分析的敏感性、特异性和可重复性。-：参考VENTANA FGFR2b （FPR2-D）小鼠单克隆抗体的最佳胃癌组织染色方案，建立其他实体瘤类型的检测方法。-：这项研究表明，在免疫组织化学中评估不同肿瘤类型的FGFR2b时，参数筛选方法对于确保最佳染色性能的重要性。

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Precision Detection of FGFR2b Protein Expression in Solid Tumors: A Comprehensive Assessment of Staining Parameters via Automated Immunohistochemistry.

Context.—: Immunohistochemistry effectively reveals the heterogeneous nature of fibroblast growth factor receptor 2b (FGFR2b) expression and antigen accessibility across diverse tumor histologic types, a variability significantly influenced by tissue type and fixation quality, both of which profoundly impact target antigen accessibility within formalin-fixed, paraffin-embedded (FFPE) tissue specimens. Retrieval parameters on automated staining platforms can impact staining outcomes and assay sensitivity. A comprehensive optimization of staining procedures, encompassing antigen retrieval, proteolytic enzyme digestion, primary antibody incubation, and detection selections, yielded 2 distinct protocols designed for specific tumor types. The protocols were tailored to maximize performance on their respective tumor types, with one protocol optimized for gastric and gastroesophageal junction (G/GEJ) adenocarcinoma, and the other fine-tuned for non-small cell lung cancer (NSCLC) and a broader spectrum of solid tumors.

Objective.—: To optimize an FGFR2b (FPR2-D) assay for NSCLC and a broader spectrum of solid tumors through modification of the established VENTANA FGFR2b (FPR2-D) Mouse Monoclonal Antibody assay, originally validated for G/GEJ adenocarcinoma.

Design.—: Multiple FGFR2b assay protocols were used to stain sections of FFPE tissue from commercially procured specimens spanning 10 tumor types. Each specimen was evaluated to select the preferred protocol parameters that achieved strong specific staining with minimal background. The assay was then assessed for sensitivity, specificity, and repeatability.

Results.—: The optimal gastric cancer tissue staining protocol for the VENTANA FGFR2b (FPR2-D) Mouse Monoclonal Antibody was referenced to develop an assay for other solid tumor types.

Conclusions.—: This investigation shows the importance of parameter screening approaches when evaluating FGFR2b across tumor types in immunohistochemistry to ensure optimal staining performance.

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Archives of pathology & laboratory medicine

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