Changes in human epidermal growth factor receptor 2 status between primary breast/gastric carcinomas and synchronous metastatic lymph nodes: how can we explain them?

Department of Human Pathology “Gaetano Barresi”, University of Messina, 98125 Messina, Italy.

Changes in human epidermal growth factor receptor 2 status between primary breast/gastric carcinomas and synchronous metastatic lymph nodes: how can we explain them?

Antonio Ieni, Valeria Barresi, Giovanni Branca, Luana Licata, Rosario Alberto Caruso, Giovanni Tuccari

Department of Human Pathology “Gaetano Barresi”, University of Messina, 98125 Messina, Italy.

Aim:Previous studies demonstrated discordant expression of human epidermal growth-factor receptor 2 ( HER2) between primary cancer and their recurrence/metastasis. This study further evaluated HER2 status between primary gastric and breast invasive carcinomas and paired metastatic disease to lymph nodes. Methods: This study collected formalin-f xed paraff n-embedded representative tissue blocks from 62 gastric and 65 breast primary carcinomas as well as synchronous metastatic lymph nodes (male:female = 39:88; age ranged between 44 and 95 years with mean age of 69.32 years) for immunohistochemical staining of HER2 expression (DAKO HercepTest?kit). If immunohistochemical HER2 score reached to 2+, HER2 amplif cation was then assessed using f uorescence in situ hybridization (PharmDx?kit DAKO). Results: The discordant HER2 pooled rate, regardless either negative or positive conversion, was 9.67% in primary gastric carcinoma and corresponding nodal metastasis, while the changes in HER2 expression were revealed in 4.61% of mammary and lymph node neoplastic samples. A high-level concordance in HER2 expression between primary carcinoma and synchronous metastatic lymph nodes was conf rmed in both types of cancer; the observed event of discordant HER2 status should be ascribed to intra-tumor heterogeneity, mostly appreciable in gastric cancer. Conclusion: In any case, the shift from positive to negative HER2 expression suggests that trastuzumab could be the targeted treatment choice whereas the opposite shift should be evaluated by a simultaneous HER2 determination in both primary and metastatic lymph nodes.

Breast cancer, epidermal growth-factor receptor 2, gastric cancer, lymph node, metastasis

Ⅰntroduction

Expression or amplif cation of human epidermal growth-factor receptor 2 (HER2) frequently occur in primitive neoplastic tissues from patients with breast carcinoma (BC).[1-4]However, in recent years, several studies have demonstrated that HER2 status may vary in the metastatic lesions compared to the primary tumor,[5-8]and this discrepancy is more frequently found in distant metastases than in loco-regional ones.[9-13]Discordance in HER2 status was not only found between primary BC and its metastases, but also among the consecutive relapses of the same tumor, with similar proportions of cases turning from negative to positive or vice versa and the changes mainly appeared in the second or following progressions.[13-16]

HER2 amplif cation may also be detected in gastric carcinomas (GCs), with a prevalence ranging between7.7% and 25% depending on localization and histology of the cancer,[17-19]a higher rate of HER2 amplif cation occurs in unusual aggressive histology types, such as the hepatoid variant.[20,21]However, until date, there were only a few studies reporting HER2 heterogeneity in paired primary and metastatic GC samples,[22-24]and demonstrating a low rate of discordance in HER2 amplif cation with either positive and negative conversion.[23,24]

The potential divergence in the HER2 status between the primitive BC/GC and their metastasized diseases, or among the successive metastases of the same tumor, has a signif cant clinical relevance since it may modify the patient’s sensitivity to targeted therapies,[8]which might be appropriate for the primitive tumor, but not for the metastases or vice versa.[12-15]For this reason, some investigators proposed that detection of HER2 status should be re-assessed in the neoplastic tissues from metastatic BC to establish whether the therapy is actually appropriate.[1,2,16,17]

Thus, in this study, we evaluated HER2 status in paired samples of BC/GC and synchronous metastatic lymph nodes that were collected during the same surgical and tissue processing procedures, thus limiting and avoiding any potential technical bias due to external factors. Our aim was to explore the eventual HER2 discordance rate between primaryBC and GC samples and corresponding lymph node metastases. The study was approved by review board of University of Messina.

Methods

This cohort contained 127 surgical BC and GC specimens, together with the corresponding regional synchronous metastatic lymph nodes. In brief, 65 primary BC and 62 primary GC (male:female = 39:88; age ranged between 44 and 95 years with mean age of 69.32 years) were retrospectively collected from the archive of the Department of Human Pathology at the University of Messina. No patients had received neo-adjuvant chemotherapy or other therapies before surgery.

The primary GC was classif ed for localization and histology type according to WHO 2010, Lauren’s classif cation and HER2 status of the tumor were available for all cases. Similarly, histology, grade, hormone receptor status, Ki-67, and HER2 status were recorded for all BC cases. Patient identif cation was not disclosed in this publication, and all patients had provided written consent to their medical information being used for research purposes, according with the Helsinki declaration.

For each case, 3 μm thick tissue sections from two different formalin-f xed paraff n-embedded representative tissue blocks of the primary tumor and metastatic lymph nodes (at least four for each case) were prepared and immunohistochemical stained for HER2 expression. In brief, the immunohistochemistry was carried out by using a DAKO HercepTest?kit (Dako, Glostrup, Denmark) with an automated procedure (DAKO Autostainer Link 48) according to manufacturer’s instructions. Antigen retrieval was performed by 3 cycles in 0.01 mol/L citrate buffer pH 6.0 in a microwave oven at 750 W. For HER2 score was used to semiquantitatively assess HER2 expression level, that is, for the primary GC, 0, absent staining; 1+, faint and discontinuous membranous staining in < 10% of neoplastic elements; 2+, light to moderate lateral, baso-lateral or complete membranous staining in > 10% of neoplastic elements; 3+, strong, intense lateral, baso-lateral or complete staining in > 10% of neoplastic elements and for BC, 3+ score was def ned when strong membranous staining was noted in at least 30% cells, 2+ when weak to moderate complete membranous staining was evidenced in 10-30% of tumors cells, 1+ when a faint or weak and incomplete membrane staining was observed and 0 when no staining was observed or when staining was present in < 10% of neoplastic cells.

Furthermore, f uorescence in situ hybridization (FISH) was performed using a HER2 FISH PharmDx?kit (Dako) in those cases with HER2 immunostaining score for 2+ or more. HER2 amplif cation was recorded when HER2 to CEP17 signal ratio was > 2.0.

Fleiss-Cohen weighted K statistics was used to assess the concordance rate between HER2 status of the primary carcinomas and metastatic synchronous lesions. K values between 0 and 0.2 were regarded as no agreement, between 0.21 and 0.4 as fair agreement, between 0.41 and 0.6 as moderate agreement, between 0.61 and 0.8 as substantial agreement, and between 0.81 and 1 as almost perfect agreement. The statistical association between HER2 status and the other histopathological parameters was assessed using Chi-squared test. P < 0.05 was considered statistically signif cant. All statistical analyses were performed using the SPSS package version 6.1.3 (SPSS, Chicago, IL, USA).

Results

Thirty GC cases (48.40%) were localized in the lower third of the stomach, 22 (35.48%) in the middle third and 10 (16.12%) in the upper-third (four of which were localized at gastro-esophageal junction). Thirty-f ve GC cases (56.45%) were diagnosed histopathologically according to the WHO criteria as adenocarcinoma (tubular, papillary, tubulo-papillary, and mucinous), 20 cases (32.25%) as poorly cohesive carcinoma, and 7 cases (11.30%) were mixed both. According to Lauren’s classif cation, 35 cases (56.45%) were classif ed as intestinal type, 20 cases (32.25%) as diffuse and 7 cases (11.30%) as mixed. Thirty-two of these 62 primary GC (51.61%) were recorded as low-grade tumors, while 30 cases were high grade (48.39%). HER2 immunohistochemical staining showed that 11 primary GCs (17.74%) were scored for 3+ HER2 expression, while 4 cases were 2+ (6.42%), 5 cases 1+ (8.10%), and 42 cases (67.74%) were not expressed HER2 at all. FISH analysis revealed no amplif cation in all of these cases with HER2 scores of 2+ or more. Taken together, in primary GC, HER2 was overexpressed in 11 cases (17.74%) but there was no HER2 amplif cation in 51 cases (82.26%). The overall concordance rate of HER2 status in primary GC between corresponding synchronous metastases was 90.32%, whereas a change in HER2 status was observed in 6 (9.68%) [ Table 1], e.g. 4 cases with HER2 amplif cation in the primary GC but no amplif cation in the metastasized tumors [negative conversion; Figure 1a and b], two of these discordant cases did not show HER2 amplif cations in the primitive tumor but amplif ed in the lymph node metastases [positive conversion; Figure 1c and d and Table 2].

In the primary BC, the most frequent histology type was ductal invasive carcinomas with the following grading: 4 G1 (6.25%), 28 G2 (43%), and 33 G3 (50.75%). HER2 overexpression occurred in 14 (21.53%) of primary BC, 4 (6.15%) of which exhibited a score 2+, 2 (3.09%) a score 1+, while 45 (69.23%) cases didn’texpress HER2 at all. FISH analysis was conducted in those cases with the HER2 score of 2+ or more andthe data revealed no HER2 amplif cation in these cases. Among 1+ cases, FISH was carried out in only two selected carcinomas showing high grade, high Ki-67 value, N+ status, and the absence of endocrine receptors expression, but no HER2 amplif cation was identif ed. HER2 was amplif ed in 14 BC cases (21.54%) but there was no HER2 amplif cation in these 51 cases (78.46%). The overall concordance rate was 95.39%, whereas changes in HER2 status between primary carcinoma and corresponding synchronous metastases were evidenced in 3 (4.61%) cases [Table 3]. Two of the discordant cases were HER2 negative in the primitive tumor but positive in the metastasized tumors [Figure 2a and b], whereas one case was HER2 positive in the primary BC and turned to negative in the metastatic tumor [Figure 2c and d and Table 4].

Table 1: Clinicopathological and HER2 concordance in 62 GC patients

Figure 1: Expression of HER2 protein. A score of 3+ HER2 expression was encountered in neoplastic elements in a primary GC (a, ×200) but vanished in the corresponding metastatic lymph node (negative conversion) (b, ×160) (IHC, Mayer’s hematoxylin counterstain). HER2 immunohistochemical negative staining in primary GC (c, ×200), demonstrated a positive reactivity in the metastatic synchronous lymph node (positive conversion) (d, ×200) (IHC, Mayer’s hematoxylin counterstain). HER2: Human epidermal growth factor receptor 2; GC: Gastric carcinomas; IHC: Immunohistochemistry

After that, we performed statistical analyses and found that the K value for the concordance rate in the HER2 status between primitive tumors and metastases was 0.651 (substantial agreement). HER2 amplif cation was signif cantly more frequent in the intestinal-type GC than that of diffuse-type while no signif cant differences in HER2 expression were noted among BC histology types. No statistical signif cant correlation emerged between HER2 and clinicopathological parameters (hormone receptors, growth fraction, pT, pN, and grade) either in GC as well as BC.

Discussion

Figure 2: Expression of HER2 protein. A negative HER2 immunostaining in a primary inf ltrative ductal carcinoma (a, ×160) became positive in the lymph node metastasis (positive conversion) (b, ×120). The strong and complete HER2 immunoreactivity in a case of primary BC (c, ×200) was not present in the synchronous lymph nodal metastasis (negative conversion) (d, ×200) (IHC, Mayer’s hematoxylin counterstain). HER2: Human epidermal growth factor receptor 2; BC: Breast carcinoma; IHC: Immunohistochemistry

Table 2: HER2 discordant status in primary GC and corresponding synchronous nodal metastases

Table 3: Clinicopathological and HER2 concordance in 65 BC patients

Table 4: HER2 discordant status in primary BC and corresponding synchronous nodal metastases

In the current study, we retrospectively analyzed HER2 expression in surgical GC and BC specimens versus the corresponding metastatic lymph nodes. Our results f rstly conf rmed the presence of a high level of concordance in HER2 status between the primary GC/BC and their corresponding lymph node metastases (90.32% and 95.39% respectively), which is consistent with previous observations of metachronous metastases (87.5-94.9%).[19,23,25]Moreover, we also found evidence of HER2 differences between primary carcinomas and their nodal metastases, that is, 9.68% GC cases and 4.61% BC cases did have the discordance between the primary and secondary tumors. Specif cally, four cases had HER2 amplif cations in the primary GC but there were no HER2 amplif cations in the metastatic tumors. In contrast, two of the gastric discordant cases showed no HER2 amplif cations in the primitive tumor but amplif ed in the lymph node metastatic tumors. Similarly, there were two of the discordant BC cases showed negative HER2 in the primitive tumor but became positive in the metastatic tumors, whereas one case was from positive HER2 in the primary BC to negative in the metastases. Therefore, a positive or negative conversion was encountered in either GC or BC cases, although with a different discordance rate. A possible explanation for the discordance observed in GC than in BC cases could be attributed to the most frequent occurrence of a heterogeneity in GC cases, compared to BC.[18,21,26]Hence, the biopsies or tissue microarray assays do not seem adequate for assessment of HER2 expression, in contrast to that elsewhere reported.[27,28]In addition, the multisampling method performed in this study using at least two tissue blocks of primary tumors and four of metastatic lymph nodes could identify more discordant cases and compensate a potential heterogeneous HER2 expression. The possible explanation of HER2 positive conversion may be related to the selection of a new HER2 positive clone in metastatic lymph nodes as a result of disease progression.[29]Loss of HER2 amplif cation (negative conversion) in metastatic tumors could not be only attributed to the development of resistance to trastuzumab therapy since our patients had not been subjected to any neo-adjuvant treatment.[29]

Changes in HER2 status between primary GC/BC and synchronous lymph node metastases may have relevant clinical impact. For example, only HER2 positive GC and BC currently support the use of trastuzumab in these patients; thus, our present f nding suggests a need to reassess HER2 status before trastuzumab treatment. As a matter of fact, assessment of HER2 expression in the primary GC and BC may exclude from the targeted treatment a signif cant percentage of patients with a negative primary tumor, but positive metastases. Finally, the inf uence of discordant HER2 status in the therapeutic management as well as in the prognostic impact of patients affected by GC and BC should be greatly considered in order to correctly identify possible eligible candidates for trastuzumab-based therapy, even among patients with HER2 negative primary carcinomas.

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How to cite this article:Ieni A, Barresi V, Branca G, Licata L, Caruso RA, Tuccari G. Changes in human epidermal growth factor receptor 2 status between primary breast/gastric carcinomas and synchronous metastatic lymph nodes: how can we explain them? J Cancer Metastasis Treat 2015;1:21-6.

Received:23-01-2015;Accepted:02-03-2015.

Source of Support:Nil,Conf ict of Interest:None declared.

Prof. Giovanni Tuccari, Department of Human Pathology “Gaetano Barresi”, A.O.U. Polyclinic G. Martino Via Consolare Valeria 1, 98125 Messina, Italy. E-mail: tuccari@unime.it

10.4103/2394-4722.153445