Arihiro Koji, Oda Miyo, Ogawa Katsunari, Kaneko Yoshie, Shimizu Tomomi, Tanaka Yuna, Marubashi Yukari, Ishida Katsunari, Takai Chikako, Taoka Chie, Kimura Shuji, Shiroma Noriyuki
Department of Anatomical Pathology, Hiroshima University Hospital, Japan.
Department of Anatomical Pathology, Hiroshima University Hospital, Japan.
Pathol Res Pract. 2016 Dec;212(12):1126-1132. doi: 10.1016/j.prp.2016.09.014. Epub 2016 Oct 4.
Although updated HER2 testing guidelines have been improved by a collaboration between the American Society of Clinical Oncology (ASCO) and the College of American Pathologists (CAP) in 2013, HER2 evaluation is still problematic because of issues involving CEP17 polysomy, heterogeneity, and HER2 score 2+ cases. The aim of this retrospective study was to evaluate the relationship between HER2 gene heterogeneity, or so called CEP17 polysomy, using breast carcinoma cells sampled by scraping and the IHC score graded by automated image analysis using whole slide image.
We randomly selected 23 breast carcinoma cases with a HER2 score 0, 24 cases with a HER2 score 1+, 24 cases with HER2 score 2+, and 23 cases with HER2 score 3+ from the records of patients with breast cancer at Hiroshima University Hospital. We compared the results of fluorescent in situ hybridization (FISH) using formalin-fixed, paraffin-embedded (FFPE) tissues and cytological samples and compared the HER2 score calculated using an automated image analysis using wholly scanned slide images and visual counting.
We successfully performed the FISH assay in 78 of 94 cases (83%) using FFPE tissues and in all 94 (100%) cases using cytological samples. Frequency of both HER2 amplification and CEP17 polysomy was higher when cytological samples were used than when FFPE tissue was used. Frequency of HER2 heterogeneity using cytological samples was higher that than using FFPE tissue, except for the IHC score 3+ cases.
When assessment of HER2 status based on FISH using FFPE tissue cannot be accomplished, FISH using cytological samples should be considered. When intensity of HER2 is heterogeneous in the tumor tissue, particularly in cases regarded as score 2+, they should be evaluated by automated image analysis using the whole slide image.
尽管美国临床肿瘤学会(ASCO)和美国病理学家学会(CAP)在2013年合作对HER2检测指南进行了更新,但由于存在CEP17多体性、异质性以及HER2评分2+病例等问题,HER2评估仍存在问题。本回顾性研究的目的是利用刮取的乳腺癌细胞评估HER2基因异质性(即所谓的CEP17多体性)与使用全玻片图像自动图像分析分级的免疫组化(IHC)评分之间的关系。
我们从广岛大学医院乳腺癌患者记录中随机选取HER2评分为0的23例乳腺癌病例、HER2评分为1+的24例病例、HER2评分为2+的24例病例以及HER2评分为3+的23例病例。我们比较了使用福尔马林固定、石蜡包埋(FFPE)组织和细胞学样本进行荧光原位杂交(FISH)的结果,并比较了使用全扫描玻片图像自动图像分析和视觉计数计算的HER2评分。
我们使用FFPE组织在94例中的78例(83%)成功进行了FISH检测,使用细胞学样本在所有94例(100%)中成功进行了检测。使用细胞学样本时HER2扩增和CEP17多体性的频率均高于使用FFPE组织时。除了IHC评分为3+的病例外,使用细胞学样本时HER2异质性的频率高于使用FFPE组织时。
当无法基于FFPE组织进行FISH评估HER2状态时,应考虑使用细胞学样本进行FISH检测。当肿瘤组织中HER2强度存在异质性时,尤其是在被视为评分2+的病例中,应使用全玻片图像通过自动图像分析进行评估。
