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首页> 外文期刊>Modern Pathology >Determination of HER2 Gene Amplification by Chromogenic In Situ Hybridization (CISH) in Archival Breast Carcinoma
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Determination of HER2 Gene Amplification by Chromogenic In Situ Hybridization (CISH) in Archival Breast Carcinoma

机译:发色原位杂交(CISH)在档案性乳腺癌中HER2基因扩增的确定。

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Purpose: To compare the efficacy of chromogenic in situ hybridization (CISH?) with fluorescence in situ (FISH) hybridization and immunohistochemistry (IHC) in determination of the HER2 status in human breast cancer. Materials and Methods: HER2 gene amplification was determined on formalin-fixed paraffin-embedded (FFPE) sections of 62 invasive breast cancers by FISH and followed by CISH using a digoxigenin (DIG)-labeled HER2 DNA probe generated by Subtraction Probe Technology (SPT?), and a biotin-labeled chromosome 17 centromeric (chr.17cen) probe. The sections were heat treated and enzyme digested. After in situ hybridization, the HER2 probe was detected with fluorescein (FITC)-anti-DIG for FISH, followed by peroxidase-anti-FITC and diaminobenzidine (DAB) for CISH. The chr.17cen probe was detected with peroxidase–streptavidin and DAB. For CISH application, HER2 gene copies or chromosome 17 centromeres and morphology of cells were easily visualized simultaneously with a 40 objective under bright-field microscope in hematoxylin-counterstained sections. IHC study of HER2 overexpression was performed on adjacent sections using a panel of three HER2 antibodies (TAB 250, CB11, A0485), and staining was scored according to the criteria specified in the HercepTest. Results: HER2 gene amplification detected by CISH was visualized typically as large DAB-stained clusters or by many dots in the nucleus. FISH and CISH identified HER2 gene amplification in 19% of the tumors. Chromosome 17 polysomy was detected in 31% of the tumors. HER2 overexpression was demonstrated in 19% (TAB 250), 23% (CB11), and 36% (A0485) of the tumors. Complete concordance between the results of CISH with FISH, TAB 250, CB11, and A0485 was seen in 100%, 97%, 94%, and 84% of the cases, respectively. Conclusion: By permitting observation of morphology using a bright-field microscope, CISH is an accurate, practical, and economical approach to screen HER2 status in breast cancers. It is a useful methodology for confirming ambiguous IHC results.
机译:目的:比较发色原位杂交(CISH?),荧光原位(FISH)杂交和免疫组织化学(IHC)在确定人乳腺癌中HER2状况方面的功效。材料和方法:HER62基因扩增是通过FISH在62个浸润性乳腺癌的福尔马林固定石蜡包埋(FFPE)切片上测定的,然后用减法探针技术(SPT? )和生物素标记的17号染色​​体着丝粒(chr.17cen)探针。将切片热处理并酶消化。原位杂交后,用荧光素(FITC)-抗-DIG检测FISH,然后用过氧化物酶-抗FITC和二氨基联苯胺(DAB)检测HER2探针。用过氧化物酶-链霉亲和素和DAB检测到chr.17cen探针。对于CISH应用,在苏木精复染的切片中,在40倍物镜下的明视野显微镜下,可轻松同时观察HER2基因拷贝或17号染色​​体着丝粒和细胞形态。使用一组3种HER2抗体(TAB 250,CB11,A0485)在相邻切片上进行了HC2 HER2过表达的IHC研究,并根据HercepTest中指定的标准对染色进行评分。结果:通过CISH检测到的HER2基因扩增通常以大型DAB染色簇或细胞核中的许多斑点显示。 FISH和CISH在19%的肿瘤中鉴定出HER2基因扩增。在31%的肿瘤中检测到17号染色​​体多态性。在19%(TAB 250),23%(CB11)和36%(A0485)的肿瘤中证实了HER2过表达。 CISH与FISH,TAB 250,CB11和A0485的结果之间完全一致,分别在100%,97%,94%和84%的病例中。结论:通过允许使用明视场显微镜观察形态,CISH是筛查乳腺癌中HER2状况的准确,实用和经济的方法。这是确认模棱两可的结果的有用方法。

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