Image analysis as an adjunct to manual HER‐2 immunohistochemical review: a diagnostic tool to standardize interpretation

Dobson, Lynne; Conway, Catherine; Hanley, Alan; Johnson, Alex; Costello, Sean; O’Grady, Anthony; Connolly, Yvonne; Magee, Hilary; O’Shea, Daniel; Jeffers, Michael; Kay, Elaine W.

doi:10.1111/j.1365-2559.2010.03577.x

Cited by 63 publications

(64 citation statements)

References 40 publications

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“…It has been mentioned that IHC 2+ result variability is principally caused by tissue quality, fixation time, type of antibody used and lack of standardization among users (3,12). In this sense, our experience indicates that IHC 2+ misevaluation depends on low Her-2 protein levels contained in samples analyzed, but principally on resolution capacity limitations of IHC methodology to quantify low target protein levels.…”

Section: Resultsmentioning

confidence: 84%

Accurate breast cancer diagnosis through real-time PCR her-2 gene quantification using immunohistochemically-identified biopsies

2012

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Abstract. her-2 gene amplification and its overexpression in breast cancer cells is directly associated with aggressive clinical behavior. The her-2 gene and its Her-2 protein have been utilized for disease diagnosis and as a predictive marker for treatment response to the antibody herceptin. Fluorescent in situ hybridization (FISH) and immunohistochemistry (IHC) are the most common FDA-approved methodologies involving gene and protein quantification, respectively. False positive or negative her-2/Her-2 patient results may result in inappropriate treatment administration. To support accurate quantification and interpretation of results, in this study we have standardized qPCR analysis using previously identified IHC samples, obtaining very significant and clinically useful results.

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Section: Resultsmentioning

confidence: 84%

Accurate breast cancer diagnosis through real-time PCR her-2 gene quantification using immunohistochemically-identified biopsies

2012

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“…26 A recent large study 34 reported the rate of IHC 2þ at 24% by manual scoring and 14% were amplified by FISH, using the ratio of greater than 2.0. The rate of IHC 2þ by IA in one study 17 was 11.2% and FISH was positive in 26% of the cases. In our study, the FISHþ rate ranged from 1% to 14% (median, 5.3%), although a higher FISHþ rate was seen from 2008 onward; however, this was associated with higher numbers of IHC 2þ cases.…”

Section: Commentmentioning

confidence: 88%

“…9 One of the suggestions was that image analysis (IA) could be an effective tool for objective interpretation, and that validation and calibration of IA instrumentation is essential before implementation in the laboratory. Studies [10][11][12][13][14][15][16][17][18][19] have shown IA to be more objective and reproducible with higher correlation with the fluorescence in situ hybridization (FISH) assay. However, most of these studies included small series of cases and were not reflective of routine clinical practice.…”

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confidence: 99%

Evaluation of HER2/neu Status by Immunohistochemistry Using Computer-Based Image Analysis and Correlation With Gene Amplification by Fluorescence In Situ Hybridization Assay: A 10-Year Experience and Impact of Test Standardization on Concordance Rate

Sarode¹,

Xiang²,

Christie³

et al. 2015

Archives of Pathology &Amp; Laboratory Medicine

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College of American Pathologists proposed several recommendations for human epidermal growth factor receptor 2 (HER2) test standardization. One suggestion was that image analysis (IA) could be useful for scoring of HER2/ neu immunohistochemistry. The utilization of IA in a realworld practice in a large cohort of cases has not been previously reported.Objectives.-To compare HER2/neu quantification by IA with gene amplification by fluorescence in situ hybridization (FISH); to determine sensitivity, specificity, and concordance rates with the FISH assay; and to determine association between HER2 status with estrogen receptor (ER), progesterone receptor (PR), and Ki-67 expression.Design.-We evaluated HER2 results performed by immunohistochemistry and FISH in conjunction with ER, PR, and Ki-67 in 3093 invasive breast cancer cases from 2002 to 2011.Results.-The overall concordance between immunohistochemistry and FISH was 87.3% (1768 of 2026). When analyzed by year, there was an improvement in the positive concordance rate from 49.4% (44 of 89) to 95.0% (57 of 60) (P , .001). The negative concordance rate was at least 95% with a median false-negative rate of 1.5%. In the FISHþ group, amplification ratio showed significant correlation with IA scores (P , .001). Positive versus negative HER2 status was associated with lower ER and PR levels (P , .001) and higher Ki-67 expression (P , .001).Conclusion.-Scoring of HER2/neu by IA was associated with high false-positive rates before 2008. Improvement in concordance rate after 2008 may be due to proper tissue handling, improved HER2/neu scoring by IA, and assay standardization.

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“…Hence, distinction between complete and incomplete membrane staining and cytoplasmic staining may be difficult. This may be one explanation for the high variation in concordance rates (75-91%) [16]. Recently, an IA system has been developed to assess the continuity of membrane immunoreactivity in addition to intensity, showing a concordance rate of 95% with FISH [16].…”

Section: Introductionmentioning

confidence: 99%

Digital image analysis of membrane connectivity is a robust measure of HER2 immunostains

Brügmann

Eld

Lelkaitis

et al. 2011

Breast Cancer Res Treat

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The purpose of this study was to develop and validate a new software, HER2-CONNECT(TM), for digital image analysis of the human epidermal growth factor receptor 2 (HER2) in breast cancer specimens. The software assesses immunohistochemical (IHC) staining reactions of HER2 based on an algorithm evaluating the cell membrane connectivity. The HER2-CONNECT algorithm was aligned to match digital image scorings of HER2 performed by 5 experienced assessors in a training set and confirmed in a separate validation set. The training set consisted of 167 breast carcinoma tissue core images in which the assessors individually and blinded outlined regions of interest and gave their HER2 score 0/1+/2+/3+ to the specific tumor region. The validation set consisted of 86 core images where the result of the automated image analysis software was correlated to the scores provided by the 5 assessors. HER2 fluorescence in situ hybridization (FISH) was performed on all cores and used as a reference standard. The overall agreement between the image analysis software and the digital scorings of the 5 assessors was 92.1% (Cohen's Kappa: 0.859) in the training set and 92.3% (Cohen's Kappa: 0.864) in the validation set. The image analysis sensitivity was 99.2% and specificity 100% when correlated to FISH. In conclusion, the Visiopharm HER2 IHC algorithm HER2-CONNECT(TM) can discriminate between amplified and non-amplified cases with high accuracy and diminish the equivocal category and thereby provides a promising supplementary diagnostic tool to increase consistency in HER2 assessment.

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Image analysis as an adjunct to manual HER‐2 immunohistochemical review: a diagnostic tool to standardize interpretation

Cited by 63 publications

References 40 publications

Accurate breast cancer diagnosis through real-time PCR her-2 gene quantification using immunohistochemically-identified biopsies

Accurate breast cancer diagnosis through real-time PCR her-2 gene quantification using immunohistochemically-identified biopsies

Evaluation of HER2/neu Status by Immunohistochemistry Using Computer-Based Image Analysis and Correlation With Gene Amplification by Fluorescence In Situ Hybridization Assay: A 10-Year Experience and Impact of Test Standardization on Concordance Rate

Digital image analysis of membrane connectivity is a robust measure of HER2 immunostains

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