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孕激素受体免疫组化定量与胞浆检测法的比较:与乳腺癌预后的相关性

Progesterone receptor immunohistochemical quantitation compared with cytosolic assay: correlation with prognosis in breast cancer.

作者信息

Lohmann C, Gibney E, Cotsonis G, Lawson D, Cohen C

机构信息

Department of Pathology and Laboratory Medicine, Emory University School of Medicine, Atlanta, Georgia, USA.

出版信息

Appl Immunohistochem Mol Morphol. 2001 Mar;9(1):49-53.

Abstract

Quantitation of estrogen and progesterone receptors (PR) represents the standard of care in the treatment of patients with breast cancer. Historically this was performed by cytosolic assay; current methods utilize immunohistochemical staining, which may be quantitated visually or by image cytometry. Formalin-fixed paraffin embedded sections from 95 breast carcinomas were immunostained with an avidin-biotin complex technique. steam antigen retrieval, and a monoclonal PR antibody (1/40 Biogenex). Nuclear immunostain was quantitated visually as the percentage of immunopositive nuclei, scored as 0 to 4. By image cytometry, the percentage of positively staining nuclear area (PPNA) was determined in 15 hpf using the CAS 200 Image Analyzer. Dextran-coated charcoal (DCC) ligand binding assay data were divided into negative (<10 fmol), low positive (10-50), or positive (>50). A statistically significant correlation was found between stage (P = 0.0001), the presence of nodal metastases (P = 0.0001), cytosolic assay (P = 0.036), image cytometry (P = 0.01), and disease-free survival. Only stage (P = 0.0001) and PR quantitation per cytosolic assay (P = 0.0001) correlated with overall survival. The method of choice for the assessment of PR hormone status in breast carcinomas is the DCC ligand binding assay. This method correlates with both survival and disease-free survival. Image cytometric quantitation of PR immunohistochemical staining correlates only with disease-free survival. The commonly used method of visual quantitation of PR immunostaining fails to relate either to survival or disease-free survival.

摘要

雌激素和孕激素受体(PR)定量是乳腺癌患者治疗中的标准操作。历史上这是通过胞质测定法进行的;目前的方法采用免疫组织化学染色,可通过视觉或图像细胞术进行定量。对95例乳腺癌的福尔马林固定石蜡包埋切片采用抗生物素蛋白-生物素复合物技术进行免疫染色、蒸汽抗原修复,并使用单克隆PR抗体(1/40,Biogenex)。核免疫染色通过视觉定量为免疫阳性细胞核的百分比,评分为0至4分。通过图像细胞术,使用CAS 200图像分析仪在15个高倍视野中确定阳性染色核面积百分比(PPNA)。葡聚糖包被活性炭(DCC)配体结合测定数据分为阴性(<10 fmol)、低阳性(10 - 50)或阳性(>50)。发现分期(P = 0.0001)、淋巴结转移情况(P = 0.0001)、胞质测定(P = 0.036)、图像细胞术(P = 0.01)与无病生存期之间存在统计学显著相关性。只有分期(P = 0.0001)和每次胞质测定的PR定量(P = 0.0001)与总生存期相关。评估乳腺癌中PR激素状态的首选方法是DCC配体结合测定。该方法与生存期和无病生存期均相关。PR免疫组织化学染色的图像细胞术定量仅与无病生存期相关。PR免疫染色常用的视觉定量方法与生存期或无病生存期均无关。

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