Abstract
In August 2006, the Australian government approved subsidized trastuzumab therapy for human epidermal growth factor receptor 2 (HER2)-positive early breast cancer, and it was mandated that HER2 testing should be performed using in situ hybridization (ISH) rather than immunohistochemistry (IHC). Here we review results of the first regulated, nationwide program to provide HER2 ISH testing for all newly diagnosed breast cancer patients, with a particular emphasis on cases where IHC and ISH results were discordant. Data from all laboratories participating in the program were collated. Cases with an equivocal ISH test result [by chromogenic ISH (CISH) or silver ISH (SISH)] were tested centrally by fluorescence ISH. Most laboratories also performed HER2 IHC, and 200 cases with discordant IHC and ISH results were selected for further analysis in a central laboratory. A total of 26 laboratories were involved and 53,402 tests were reported. Over a 4-year period the HER2 positivity rate decreased for primary cancers from 23.8 to 14.6 %, but remained relatively constant for samples from metastases. Average ISH reporting times were <5 days for all yearly reporting periods. Test-repeat rates decreased for CISH (8.9–3.6 %) and SISH (13.7–8.4 %). Only 12 of 196 cases remained discordant after retesting in a central laboratory. These findings demonstrate the successful implementation of a regulated, national program that continues to collect data on HER2 status. The results also highlight the differences in IHC interpretation between local laboratories and a central, more experienced, laboratory. This model could be used to establish future biomarker-testing programs in other countries.
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Introduction
The human epidermal growth factor receptor 2 (HER2) gene is amplified in ~15–20 % of breast cancers and has been linked with poor prognosis [1–6], making it an attractive molecular target for breast cancer therapy. Trastuzumab (Herceptin®; F. Hoffmann-La Roche Ltd, Basel, Switzerland) is an anti-HER2 monoclonal antibody with proven survival benefits in the treatment of women with HER2-positive metastatic breast cancer (MBC) [7–11] and early breast cancer (EBC) [12–15]. Evaluation of the HER2 status of all breast cancers at diagnosis is recommended to predict the potential benefit from trastuzumab treatment [16, 17].
HER2 testing is performed by either immunohistochemistry (IHC) or in situ hybridization (ISH). IHC uses anti-HER2 antibodies to detect HER2 protein expression levels, and is assessed semiquantitatively by the proportion and intensity of staining. ISH uses DNA probes to determine HER2 gene copy number. To ensure accurate HER2 testing, as well as consistent and appropriate patient selection for trastuzumab therapy, the American Society of Clinical Oncology (ASCO) and the College of American Pathologists (CAP) convened an expert panel to compile and publish HER2 testing recommendations that included an algorithm to define positive, negative, and equivocal HER2 results according to both HER2 protein expression and gene amplification [18]. According to the ASCO/CAP guidelines, a HER2-positive result by IHC is uniform, intense staining of >30 % of invasive tumor cells (3+) and a positive result by ISH is >6 HER2 gene copies per nucleus or a HER2 gene:chromosome enumeration probe 17 (CEP17) signal ratio of >2.2 [18].
A minority of the ASCO/CAP panel expressed the view that IHC is not a sufficiently accurate assay to determine HER2 status [18], and two large trials have shown discordance between local and central HER2 testing by IHC [19] or by both IHC and fluorescence ISH (FISH) [20]. Analysis of concordance between a local and a high-volume central laboratory in a phase IV trial [21] also showed poor concordance of IHC results, and concluded that HER2 testing is most accurate when performed at a high-volume central laboratory.
In Australia, ~14,000 new breast cancer cases are diagnosed annually [22]. Patients with HER2-positive MBC, determined by either IHC or ISH, are eligible for trastuzumab therapy as part of the Herceptin program administered by Medicare Australia. Patients with HER2-positive EBC are also eligible for trastuzumab therapy under the Australian government-funded Pharmaceutical Benefits Scheme. The Pharmaceutical Benefits Advisory Committee specified that HER2 positivity should be demonstrated by ISH in these patients. This requirement led to the development of the Australian In Situ Hybridization Program, a nationwide program utilizing ISH as the HER2 testing platform. The program was launched as a multicenter, coordinated project, with the primary objective being to provide accurate tumor ISH testing for all patients diagnosed with EBC. Accurate testing is critical in guiding the provision of trastuzumab therapy to those who are likely to derive the most benefit from the treatment.
Here, we include details of the HER2 positivity rates recorded across Australia from October 2006 to September 2010 for patients with EBC or MBC, along with other test-related data; including result turnaround times and repeat testing rates. Most laboratories continue to use IHC in parallel with ISH and we also document the results of a reevaluation of 200 samples that had shown discordance between local IHC results and ISH results from a central reference laboratory.
Methods
Study design
The Australian In Situ Hybridization Program is a nationwide, multicenter, coordinated project sponsored by Roche Products Pty Limited (Dee Why, Australia) and overseen by the Australian HER2 Testing Advisory Board. Details of establishing of this program, including identification, training, certification, and accreditation of all laboratories, as well as the implementation of standardized reporting protocols, have been described previously [22].
Sample selection
The majority of samples for HER2 ISH testing were from excised tumors from women aged ≥18 years with EBC or MBC. Approximately 10 % of samples were core biopsies and <1 % were from fine needle aspiration cell block material, or from male breast cancer patients.
HER2 testing
All local laboratories were responsible for the provision of an accurate and timely HER2 testing service to support clinical decision-making in their area. Figure 1 shows the ISH assay algorithm used to determine HER2 positivity. A validated single-probe ISH test was used for all samples, with a CEP17 probe used for equivocal cases, defined as 4–6 HER2 signals per nucleus. Cases that remained equivocal following dual-probe testing (defined as a HER2:CEP17 ratio of 1.8–2.2) or which were non-diagnostic due to a weak signal, were sent to a central reference laboratory for FISH testing using the PathVysion® kit (Vysis/Abbott, Illinois, USA). IHC was used in conjunction with ISH as a quality control, both to assess tumor heterogeneity and to assist in the overall assessment of difficult-to-assess cases. In the initial phase of the program, IHC was used by some laboratories lacking the facility to perform ISH, to triage cases to be sent for ISH testing at one of the program laboratories. This practice gradually diminished over time, such that the vast majority of invasive cancer cases were submitted for ISH testing regardless of whether IHC had been performed, or of the IHC result.
All laboratories initially used a chromogenic ISH kit (CISH; SPoT-Light® CISH, Invitrogen, California, USA). Approximately 1 year after the launch of the program, silver ISH (SISH; Inform™, Ventana Medical Systems, Inc., Arizona, USA) was also included as an alternative ISH testing assay, with a third option (DuoCISH™, Dako, Glostrup, Denmark) included 6 months later. All kits were used in accordance with the ISH assay algorithm (Fig. 1) and, from March 2008, the scoring of all HER2 tests adhered to the 2007 ASCO/CAP recommendations [18].
Data collection
All HER2 test results, reporting times, test-repeat rates, and the proportion of tests performed on core biopsies were recorded. Means of each parameter were calculated for each laboratory and state during the measurement periods of October–September for 2006–2007, 2007–2008, 2008–2009, and 2009–2010. Mean HER2 positivity rates were also calculated for each laboratory and state for the four 12-month time periods.
Comparison of IHC and ISH results
Two hundred invasive carcinomas were selected from patients, in which IHC had been performed at a local laboratory and the paraffin blocks or unstained sections had been forwarded to a central reference laboratory for ISH testing. All selected cases had shown discordance between local IHC and central ISH results. The cases included were either IHC 0/IHC 1+ that showed HER2 gene amplification (false-negative, n = 31) or IHC 3+ that showed no HER2 gene amplification (false-positive, n = 169). The central laboratory performed IHC on archived, unstained sections from all the cases using the 4B5 antibody (Ventana Medical Systems, Inc.) on the Ventana BenchMark Immunostainer (Ventana Medical Systems, Inc.). The stained slides were then assessed by a pathologist blinded to both the original IHC result, and to the HER2 gene amplification status. In cases of uncertainty a second pathologist independently assessed the slide and, if necessary, the case was viewed by both pathologists together and a consensus score reached.
Results
HER2 positivity rates
By September 2010, the Australian In Situ Hybridization Program had been running for 4 years and had performed 53,402 ISH tests. Overall, 26 laboratories were approved for ISH testing. In the final reporting period, eight laboratories used CISH and 18 used SISH assays.
The total number of ISH tests conducted between October 2006 and September 2010, as well as the HER2 positivity rates for samples from EBC and MBC, are shown in Tables 1 and 2. Between October 2006 and September 2010, the overall HER2 ISH positivity rate was 16.9 % for EBC and 22.5 % for MBC. The HER2 positivity rate for EBC decreased each year from 23.8 % in the first 12-month period to 14.6 % in the final 12 months, whereas the MBC HER2 positivity rate varied from 22.6 % in the first 12-month period to 25.1, 21.3, and 21.6 % in the second, third, and fourth 12-month periods, respectively.
The majority of tumor specimens used for HER2 testing were obtained from excised tumors. The proportion of core biopsy samples tested remained consistently low and rarely exceeded 10 %. Testing of core biopsies was actively discouraged unless the HER2 status was required for a clinical decision regarding neoadjuvant therapy.
Reporting time data were provided by 17 of 18 laboratories in the first 12 months, 20 of 22 laboratories in the second 12 months, and all 26 laboratories in the final two 12-month periods. The average ISH reporting time from the date of the request for a HER2 test remained relatively unchanged between the reporting periods (4.9, 4.7, 4.6, and 4.5 days, respectively). For individual laboratories, average reporting times ranged from 1.3 to 12.9 days in the first 12 months, from 1.6 to 10.5 days in the second 12 months, from 1.0 to 10.2 days in the third 12 months, and from 1.3 to 10.9 days in the final 12 months. Average reporting times were longer than 7 days for 2 out of 17, 4 out of 20, 6 out of 26, and 4 out of 26 laboratories for the four consecutive reporting periods.
ISH test-repeat rates for each laboratory are shown in Table 3. In the first 12 months the overall ISH test-repeat rate was 8.9 %, decreasing to 8.2 % in the second 12 months for laboratories using CISH. Twelve laboratories changed from using CISH to SISH in the second 12-month period. Repeat rates were higher (13.7 %) in these laboratories, although this was primarily caused by a global silver wash contamination issue that was subsequently addressed and resolved. In the third 12-month reporting period, test-repeat rates were 4.9 % for laboratories using CISH and 7.2 % for laboratories using SISH. In the final reporting period, test-repeat rates were 3.6 % for laboratories using CISH and 8.4 % for laboratories using SISH.
Retesting of discordant IHC/ISH cases
Of the 200 discordant cases selected, four were considered unsuitable for assessment due to the presence of considerable artifact(s), insufficient tissue, or loss or damage to the section during processing. Of the remaining 196 cases retested by IHC, 184 (94 %) showed concordance between the results of the repeat IHC and ISH. Eleven of the 12 cases that remained discordant (91.6 %) were false-negative and one was false-positive. The details of these 12 cases are shown in Table 4.
An analysis of the cases that were now concordant following retesting showed that there were 45 cases reclassified from IHC 3+ to IHC 2+ (equivocal). Of those, 14 (31 %) had a chromosome 17 polysomy. Of the 161 cases that were originally scored as IHC 3+ but did not show gene amplification by ISH, 116 (72 %) were scored as IHC 0 or IHC 1+ after retesting.
Discussion
Since the inception of the Australian In Situ Hybridization Program in October 2006, the number of HER2 ISH tests has increased each year; reflecting a shift toward HER2 ISH testing of all breast cancer samples (rather than the previous practice of triaging samples for ISH testing on the basis of IHC results). There was a 112 % increase in ISH testing reported between the first and last time period for patients with EBC, which is attributable to a greater understanding of the ISH testing program (i.e., all patients should be tested for ISH, regardless of IHC results), laboratory implementation of the ISH testing algorithm, and an increased number of laboratories qualified to report ISH. In addition, there is greater awareness among oncologists and breast surgeons that trastuzumab therapy should be available to all EBC patients with a positive ISH result. By comparison, ISH reporting of MBC cases was low and increased by just 20 % between the first and last reporting periods. Initial ISH testing of MBC cases is not a requirement of the Herceptin program administered by Medicare Australia. The smaller increase observed, may also reflect the fact that many patients presenting with MBC could have previously had their primary tumor tested for HER2 and therefore, may have received trastuzumab in the adjuvant setting [23]. In patients with EBC there was a reduction in HER2 positivity rates reported between the time periods (from 23.8 to 14.6 %) which reflects a shift toward the use of ISH testing for all samples without prior IHC triaging. The HER2 positivity rate of 14.6 % is comparable to rates reported in the literature [2–6, 24]. Although the average HER2 positivity rate among patients with MBC was higher than for EBC for all time periods and showed variations across the reporting period (22.6, 25.1, 21.3, and 21.6 % for the first, second, third, and fourth 12-month periods, respectively), these rates were also similar to those reported in the literature [2–6, 25, 26], suggesting that MBC is associated with a higher HER2 positivity rate than EBC and reflecting a more aggressive tumor cohort.
The decision to make trastuzumab therapy available to patients with HER2-positive EBC following an ISH-positive test is supported by recent guidelines for HER2 testing [27], which favor ISH over IHC due to its greater test accuracy, objectivity, and reproducibility. However, it should be noted that the use of ISH testing alone is associated with some risks, including an increased likelihood of failing to detect heterogeneity, overscoring highly polysomic cases (when a single probe is used), and missing cases with low HER2 amplification. IHC is, therefore, a valuable tool for the assessment of equivocal or difficult cases and remains an important quality assurance measure. As such, we feel that the use of ISH testing, together with additional IHC testing as required, ensures the provision of accurate testing by all local laboratories, with a central laboratory providing further evaluation by FISH as necessary.
The efficiency of all laboratories involved in this nationwide program was illustrated by the consistently short overall reporting time for ISH tests, with average reporting times reduced slightly in the second 12-month period, despite the inclusion of four new laboratories and the fact that 12 laboratories switched to SISH testing. Average reporting times remained consistent in the third and fourth 12-month periods (4.6 and 4.5 days, respectively). For those laboratories that continued to use CISH, the test-repeat rates also decreased over the reporting period, reflecting the improvements in testing proficiency as a result of increasing experience. In the second reporting period, test-repeat rates were higher than expected for laboratories using SISH (13.7 %); however, this was attributed to a contamination of the silver wash which was reported in a number of countries outside Australia, and the test-repeat rate fell during the final two reporting periods to 7.2 and 8.4 %, respectively.
This study has demonstrated that there are inherent inaccuracies in local laboratory staining and/or assessment of HER2 IHC, where ISH is considered the “gold standard” test. This is highlighted by the fact that 72% of the 161 cases originally scored as IHC 3+ by local laboratories but found to be non-amplified by ISH were subsequently scored as IHC 0 or IHC 1+ by a central laboratory. However, our study has shown that very good concordance (94 %) exists between IHC and ISH when both tests are performed and interpreted by experienced laboratories and pathologists. There were a range of factors contributing to the discordance in the remaining 12 cases, including monosomy of chromosome 17 (three cases), and clonal amplification of HER2 (one case). All of these cases showed only a low level amplification of the HER2 gene (HER2:CEP17 ratio range 2.3–5.48). There is some debate regarding the relative importance of HER2:CEP17 ratio versus HER2 copy number in assessing ISH [28, 29] and there was discordance between the two methods in 6/12 of our cases, reflecting the lack of an IHC 3+ score.
Although IHC/ISH discordance has been demonstrated previously in the setting of some clinical trials involving centralized retesting by FISH [20], our study has focused specifically on discordant cases. It remains unclear whether the laboratory test procedure, the pathologist’s interpretation, or both, contribute to the observed discordances. Therefore, a valuable additional analysis will be to compare results from small- and large-testing volume laboratories; however, this was not possible with the existing data.
The emphasis on accurate HER2 testing has been highlighted by the ASCO/CAP expert panel [18]. As well as recommending an updated scoring system for HER2 assessment, multiple factors that can cause variation in HER2 testing accuracy were identified, including fixation methods and assay reagents used [18]. Several standard assays exist for HER2 testing, which could result in a high degree of testing inaccuracy. The Australian In Situ Hybridization Program, as well as adhering to the ASCO/CAP HER2 testing guidelines, uses standardized HER2 testing kits (CISH, SISH, or DuoCISH) to minimize interlaboratory variation. All pathologists participating in the Australian In Situ Hybridization Program are required to perform a minimum number of 50 ISH tests annually, and each laboratory must perform a minimum of 150 tests annually. This ensures that there is a sufficient level of experience in participating laboratories. Participation in appropriate quality assurance programs is also mandatory. Further efforts to ensure the implementation of a highly accurate and robust HER2 testing system as part of this nationwide program included the emphasis on testing the excised tumor wherever possible, as testing on core biopsies may be less reliable [30]. Our data indicate that core biopsies were used for HER2 testing in <10 % of cases in most laboratories.
In summary, these findings demonstrate the successful implementation of a regulated, nationwide testing program that continues to collect data on HER2 testing in patients with breast cancer. We feel that the implementation of a high standard of training, accreditation, and quality assurance, as well as a streamlined approach to testing and reporting, have been fundamental to the success of this program. This methodology could be used as a model for the establishment of HER2 testing in other countries or for the implementation of other new biomarker-testing initiatives.
Abbreviations
- amp:
-
Amplification
- ASCO:
-
American Society of Clinical Oncology
- CAP:
-
College of American Pathologists
- CEP17:
-
Chromosome enumeration probe 17
- Chr:
-
Chromosome
- CISH:
-
Chromogenic in situ hybridization
- EBC:
-
Early breast cancer
- FISH or (f):
-
Fluorescence in situ hybridization
- HER2:
-
Human epidermal growth factor receptor 2
- IHC:
-
Immunohistochemistry
- ISH:
-
In situ hybridization
- MBC:
-
Metastatic breast cancer
- SISH or (s):
-
Silver in situ hybridization
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Acknowledgments
The sponsor of this study was Roche Products Pty Limited, Dee Why, New South Wales, Australia.
Support for third-party writing assistance for this manuscript was provided by F. Hoffmann-La Roche Ltd.
Conflict of interest
Michael Bilous has held a consultant/advisory role with F. Hoffmann-La Roche Pty Ltd. Adrienne L. Morey, Richard Bell, and Stephen B. Fox have held consultant/advisory roles with Roche. Adrienne L. Morey has held a consultant/advisory role with Pfizer. Jane E. Armes has held a consultant/advisory role with the HER2 Testing Advisory Committee. Glenn D. Francis has held consultant/advisory roles with Roche Pharmaceuticals, Roche Ventana Medical Systems, Merck Serano, and Astra Zeneca. Brigid Waite is an employee of Roche Products Pty Ltd. Glenda McCue has held a consultant/advisory role with Woolomin Consulting. Gelareh Farshid has held a consultant/advisory role with the Australian HER2 Advisory Board. Peter H. Button, Margaret C. Cummings, Wendy A. Raymond, and Peter D. Robbins have no conflict of interest to disclose.
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Bilous, M., Morey, A.L., Armes, J.E. et al. Assessing HER2 amplification in breast cancer: findings from the Australian In Situ Hybridization Program. Breast Cancer Res Treat 134, 617–624 (2012). https://doi.org/10.1007/s10549-012-2093-6
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DOI: https://doi.org/10.1007/s10549-012-2093-6