Background
Treatment with the non-steroidal antiestrogen (AE) tamoxifen has been the first-line endocrine treatment of choice for breast cancer patients for more than 30 years. However, the third-generation aromatase inhibitors (AIs) anastrozole, letrozole and exemestane have in large randomized trials shown to be comparable or superior to tamoxifen as treatment for postmenopausal women with hormone receptor (HR) positive metastatic breast cancer [
1‐
6]. The objective response rates ranged from 21% to 33% with clinical benefit rate varying between 49% and 59% [
1,
2,
4], necessitating improvements in treatments and development of response predictors to the different options.
Expression of the estrogen receptor (ER) is a prerequisite for estrogen dependent tumor growth and ER positivity in the primary tumor has been used as a selection criterion for endocrine therapy since 1975 [
7]. Furthermore, ER is also well known to be an important prognostic factor, indicating good prognosis [
8]. The progesterone receptor (PR) is an estrogen-inducible protein and improved response rates have been seen in tumors, which besides ER, also express PR [
9‐
11], with increasing ER and PR scores being associated with better response to tamoxifen in ER positive metastatic breast cancer [
12]. Today, most laboratories perform immunohistochemical (IHC) determination of both ER and PR and a good correlation between the quantitative level determined with the classical ligand-binding assays and the immunohistochemical scores have been found for both ER and PR [
12].
The third-generation AIs anastrozole, letrozole and exemestane suppress total-body aromatization by 98%, more than 99% and 98%, respectively [
13,
14], demonstrating the superior suppressive potency of these drugs compared to the previous first- and second-generation compounds [
15]. Furthermore in studies with direct measurements of estrogen levels in tumor tissue, AI treatment resulted in nearly complete suppression of intratumoral estrogen levels [
16‐
20]. The intratumoral estrogen level may arise from local estrogen production in carcinoma cells or surrounding cells as well as from the uptake of peripherally generated estrogens, and so it has been debated whether the
in situ estrogen production in the carcinoma cells is the major contributor to estrogen-stimulated tumor growth and thus may be a predictor of response to treatment with AIs [
14,
21‐
24]. Biochemically determined intratumoral aromatase enzyme activity has shown correlation with response to treatment with AI [
25], and classic estrogen-dependent genes and proliferation markers changed in most tumors during treatment irrespective of response [
26], supporting the hypothesis that
in situ estrogen synthesis may be used as a predictive marker for response to treatment with aromatase inhibitor. Attempts have been made to measure the aromatase protein in the tumor tissue as an alternative to the biochemical assay. The aromatase protein has been detected in both fibroblasts, adipose cells, benign duct cells and invasive cancer cells and the results have been contradictory with respect to which cell types in the breast express the aromatase protein [
27‐
33]. A promising new aromatase antibody (#677) has shown immunoreactivity in carcinoma cells, stromal cells or fibroblasts, adipocytes, normal epithelium, and inflammatory cells [
31]. The multiplicative SIP score for carcinoma cells ("Proportion of aromatase immunopositivity" multiplied with "Relative intensity of aromatase immunoreactivity") was positively correlated with the aromatase enzyme activity measured by the biochemical tritiated-water release assay [
32], indicating that aromatase expression in the carcinoma cells may be a predictive marker for response to AI treatment. Furthermore, since PR expression is induced by estrogen binding to ER, it may be hypothesised that high PR expression in combination with aromatase expression in primary tumor tissue identifies patients with superior benefit from AI treatment.
Due to the difficulties regarding determination of the aromatase protein expression and activity, cyclooxygenase-2 (COX-2) has been proposed as a surrogate marker for aromatase expression [
34]. COX-2 is an isoform of the prostaglandin endoperoxidase synthetase that catalyzes key steps in the metabolism of arachidonic acid to prostaglandin E2 (PGE2), thereby regulating the synthesis of aromatase [
35‐
37]: Expression of aromatase is controlled by unique promoters that lie upstream of tissue-specific exons. These first exons are alternatively spliced onto a common site upstream of the translation initiation codon in exon II. The aromatase mRNAs have unique 5'-untranslated regions, but the sequences encoding the aromatase enzyme are identical. In tumor tissue aromatase is up regulated by switching from the weak promoter I.4 to the strong promoters IIa and I.3. Switching from promoter I.4 to IIa and I.3 is likely to be mediated by the induction of COX-2 [
38], which is expressed in a variety of cancers including invasive breast cancer [
39‐
41].
The aim of this study was to explore whether the expression level of the aromatase protein in carcinoma cells alone or in combination with PR expression in the primary tumor may be predictive for response to treatment with the AI letrozole or the AE tamoxifen in the advanced breast cancer setting. The predictive utility of COX-2 for endocrine treatment as well as a surrogate marker for aromatase expression was also investigated. We have prepared tissue micoarrays (TMAs) and performed IHC analyses of ER, PR, COX-2 and aromatase in primary tumor tissue from 88 of the 907 patients who participated in the multicenter randomized phase III P025 trial which compared first-line tamoxifen or letrozole treatment in postmenopausal women with locally advanced or metastatic breast cancer [
2,
3]. A semi-quantitative IHC score has been determined for each of the four parameters. For aromatase expression, an evaluation of IHC staining in whole sections versus staining in TMAs was performed as previously described for ER, PR and COX-2 [
42].
Methods
This study was derived from the P025 study, an international, multicenter, double-blind, randomized, two-arm, phase III clinical trial comparing letrozole with tamoxifen as first-line treatment for postmenopausal women with advanced breast cancer [
2]. The P025 study was conducted in accordance with the ethical principles that originated in the Helsinki II declaration and the appropriate local ethics review boards have approved the study, number by local ethical review board: 01025-KF12-138-99.
For this current sub-study it was possible to collect primary tumor material from 68 Danish patients and from 20 patients from the rest of Europe. Thus, altogether, paraffin blocks containing primary tumor material from 88 patients were collected. Sixty-five tumors were classified as invasive ductal and 12 as invasive lobular carcinoma. Three tumor samples were classified as neither lobular nor ductal and eight samples were not suitable for classification. Three of the 88 patients were originally allocated to a combination treatment of letrozole and tamoxifen. This combination therapy arm was stopped in the original P025 study and the patients were excluded from the intention to treat analysis, thus 85 patients are included in the present study, unless for comparison of aromatase expression in WS and TMAs where tissue from all 88 tumors were included. The end-point Time To Progression (TTP), is defined as described by Mouridsen
et al. 2001 [
2]. All patient data used in this study were provided by Novartis Phama AG, (Basel Switzerland) to the Danish Breast Cancer Cooperative Group (DBCG), following agreement with the departments who treated the patients.
Immunohistochemical staining of ER, PR and COX-2
Sections, 3 μm, were dewaxed in coconut oil and rehydrated in a graded series of ethanol. Slides were preheated for 10 min. and boiled for 15 min. in microwave oven at 600 W in TEG buffer (pH = 9, Bie & Berntsen, Denmark) for antigen retrieval and rinsed in tap water. All immunostainings were performed at room temperature using the automated immunostainer Tech-mate 500 (Dako, Denmark), according to the following protocol: Slides were washed in TBS + 0.1% BRIJ-35 detergent (AX-LAB, Denmark) and incubated with primary antibody diluted in TBS + 0.1% BRIJ-35 + 1% BSA (Bovine Serum Albumin) + 15 nM sodiumazide for 60 min. After washing, endogenous peroxidase activity was blocked using 3% H2O2 in TBS + 0.1% BRIJ-35. The ChemMate EnVision+ Detection Kit (Peroxidase/Dab, Rabbit/Mouse, K5007, Dako, Denmark) was used as detection system for the primary antibodies. After washing, slides were counterstained with haematoxylin and dehydrated in graded series of ethanol, and finally mounted with Pertex (Histolab, Denmark). The following primary antibodies, all monoclonal mouse subtype IgG1, were used: ER, clone ER1D5, 1:200 (Immunotech); PR, clone 16, 1:200 (Novocastra); COX-2, no 6111104, 1:150 (Cayman Chemicals). The specificity of the immunoreactions was verified by substitution of the primary antibody with the corresponding concentration of mouse IgG1, X 0931 (Dako, Denmark). In addition, positive control slides with breast tumor tissue or other tissue known to stain positive were included in every run. All stainings of the individual antigens were performed in a single run in order to minimize interserial staining variation.
Immunohistochemical staining of Aromatase
All aromatase staining as well as evaluation of the staining was conducted by the author Hironobu Sasano. Sections, 3 μm, were stained and analyzed as described in Sasano et al. 2005 [
32]. In brief: tissue sections were immunostained by a biotin-streptavidin method using a Histofine kit (Nichirei Co. Ltd., Tokyo, Japan). The antigen-antibody complex was subsequently visualized with 3.3'-diaminobenzidine solution (DAB) and counterstained with hematoxylin. Evaluation of aromatase IHC was performed by assessing the approximate percentage of carcinoma cell staining (proportion score) and classifying the proportion score values as the following: 0 = <1%, 1 = 1–25%, 2 = 26–50%, 3 = 51–75% and 4 = 76–100% immunopositive cells. The relative intensity of aromatase immune-positive cells was classified as follows: 0 = no immunoreactivity, 1 = weak, 2 = moderate and 3 = intense immunoreactivity. The SIP score is the proportion score multiplied with the relative intensity score. The evaluation of the aromatase immunoreactivity was performed without the knowledge of response to treatment.
Preparation of tissue microarrays
TMA blocks were constructed using the TMA-builder from Histopathology Ltd. (AH-diagnostics, Denmark). Targets for arraying (areas with representative invasive tumor) were identified by marking the corresponding areas on haematoxylin-eosin stained sections from each paraffin block. Two tissue cores with a diameter of 2 mm were transferred from each donor block to the recipient TMA block. Kidney tissue was placed in the first core of the upper left and right corner of the TMA block to ensure correct orientation when examining the slides. All analyses were performed on TMAs [
42], whereas analysis for aromatase was performed on whole sections (WS) as well.
Evaluation of ER, PR and COX-2 immunohistochemical staining
All specimens were evaluated without knowledge of the clinical data. TMA slides were evaluated by light microscopy and the authors Katrine L. Henriksen scored all the samples and Birgitte B. Rasmussen has been consulted in cases of doubt. Only invasive tumor components were considered when assessing the staining. Semi-quantitative determination of ER and PR was performed according to the method described by Allred
et al. [
43]. This method was also used for semi-quantitative determination of the non-nuclear cytoplasmatic marker COX-2. In brief: The proportion of positive stained cells was judged as 0 = no cells stained, 1 = between 0 and 1% stained positive, 2 = between 1 and 10% stained positive, 3 = between 10 and 33% stained positive, 4 = between 33 and 66% stained positive, 5 = between 66 and 100% stained positive. In addition to the proportion score, an intensity score was made based on the average intensity of staining, 0 = negative, 1 = weak, 2 = intermediate and 3 = strong. The intensity score and the proportion score was added to obtain the total score referred to as the Allred score, which is 0 or between 2 and 8, 0 and 2 were interpreted as negative. Only nuclear staining was judged when scoring ER and PR, whereas cytoplasmatic staining was scored for COX-2.
Evaluation of Aromatase immunohistochemical staining
Evaluation of aromatase staining in WS was done using the SIP score as described in Sasano et al. 2005 [
32]. As described above, when preparing TMAs only areas containing primary tumor was used, thus instead of determining a SIP score the determination of "relative intensity of aromatase immunoreactivity" in carcinoma cells was scored for TMAs and not the "proportion of aromatase immunopositivity". Consequently no SIP score was obtained for the TMA sections.
Statistical Analysis
Chi-square test was used to evaluate if the patients in the present study represent the entire study population of patients. The Kappa score was used to evaluate the agreement of aromatase immunointensity of carcinoma cells on whole sections (WS) versus TMAs, and for this analysis results from all 88 collected tumor samples were included. The Systematic difference between the scores on TMA and whole sections was analysed with Wilcoxon's Signed Rank Sum test on the difference (TMA-WS) and the Concordance is determined as the number of samples with no difference in scoring value in relation to the number of samples with a different scoring value and
P-values for evaluation of WS versus TMA are given (Table
1). The association of aromatase expression with COX-2, as well as the agreement between expression of aromatase with ER and PR was done by calculating the Kappa score and
P-values are given. Time to progression (TTP) was the primary endpoint in the P025 trial and was defined as the interval between the date of randomisation and the earliest date of disease progression. Kaplan-Meier plots were used to illustrate univariate survival and differences in TTP between subgroups were evaluated by the Wilcoxons rank sum test. A multivariate Cox proportional hazards model was used to investigate the effect of treatment and each of the parameters aromatase, COX-2 and PR, expressed as semi-quantitative IHC results. Interaction between treatment and aromatase expression was further investigated by subgroup analysis within each treatment group. When analysis of grouped scoring values was applied, scoring values were grouped as follows: For ER, PR and COX-2-expression "high" is defined as Allred score 7 or 8, "low" as Allred score 3 to 6 and "negative" as 0 or 2. For Aromatase, "high" is defined as SIP score 9 and 12, "low" as SIP score 1,2,3,4,6 or 8, and "negative" as SIP score 0 (See Table
2). In all tests, a
P-value < 0.05 was used as level of significance.
Table 1
Comparison of carcinoma cell aromatase immunointensity in TMA and WS
| 26% | (p < 0.002) | 0.0048 (-0.080–0.17) (P = 0.41) |
Table 2
Semi-quantitative IHC results: ER, PR, COX-2 and Aromatase
negative
| ≤ 2 | 3 | 2 | 5 |
Low
| 3 | 0 | 0 | 0 |
| 4 | 1 | 1 | 2 |
| 5 | 2 | 1 | 3 |
| 6 | 6 | 3 | 9 |
High
| 7 | 10 | 8 | 18 |
| 8 | 21 | 19 | 40 |
N.A. (not assessable)
| 3 | 5 | 8 |
Total positive
| 40 | 32 | 72 |
PR level (Allred score)
|
negative
| ≤ 2 | 9 | 9 | 18 |
Low
| 3 | 3 | 1 | 4 |
| 4 | 5 | 3 | 8 |
| 5 | 4 | 5 | 9 |
| 6 | 1 | 6 | 7 |
High
| 7 | 6 | 0 | 6 |
| 8 | 14 | 12 | 26 |
N.A. (not assessable)
| 4 | 3 | 7 |
Total positive
| | 33 | 27 | 60 |
COX-2 level (Allred score)
|
negative
| ≤ 2 | 13 | 11 | 24 |
Low
| 3 | 0 | 2 | 2 |
| 4 | 5 | 4 | 9 |
| 5 | 10 | 2 | 12 |
| 6 | 7 | 6 | 13 |
High
| 7 | 5 | 7 | 12 |
| 8 | 1 | 0 | 1 |
N.A. (not assessable)
| 5 | 7 | 12 |
Total positive
| | 28 | 21 | 49 |
Aromatase level (Carcinoma cell SIP score)
|
negative
| 0 | 10 | 5 | 15 |
Low
| 1 | 3 | 3 | 6 |
| 2 | 9 | 3 | 12 |
| 3 | 2 | 3 | 5 |
| 4 | 5 | 9 | 14 |
| 6 | 8 | 5 | 13 |
| 8 | 0 | 2 | 2 |
High
| 9 | 2 | 3 | 5 |
| 12 | 2 | 1 | 3 |
N.A. (not assessable)
| 5 | 5 | 10 |
Total positive
| 30 | 30 | 60 |
Discussion
In this small retrospective sub-study of the P025 trial we have analyzed aromatase, COX-2, ER and PR expression by semi-quantitative IHC in primary tumor material from 9.4% of the patients included in the original study. The patients in our study were rather equally distributed regarding allocation to letrozole or tamoxifen. Our aim was to investigate whether aromatase- or COX-2 expression could be used as single markers for treatment, or if aromatase in combination with PR expression, could be used to select patients for treatment with either tamoxifen or letrozole. Furthermore, the utility of COX-2 as a surrogate IHC marker for aromatase as well as the feasibility of analysing aromatase expression by TMAs was evaluated.
In spite of the many resources and efforts applied to understand the basis of development, progression and prediction of response to treatment of breast cancer, only three predictive markers (ER, PR and HER-2) are recommended for routine IHC testing in breast cancer. Two of these, ER and PR, are predictive for response to endocrine treatment [
45]. Since aromatase is the key enzyme in the estrogen synthesis and is expressed in both breast carcinoma cells, surrounding stromal cells as well as endothelial and benign breast cells [
27,
34], many attempts have been made to evaluate the importance of aromatase expression in the different cell types in the breast for local estrogen production and for utility as prognostic and predictive marker. The obtained results have been contradictory [
26‐
29,
33,
46,
47]. However, recent data have shown that the aromatase antibody #677 is very specific for IHC detection of the aromatase protein [
31,
32]. Although it has been assumed that the estrogen production in the surrounding stromal cells contributes significantly to the estrogen level within the carcinoma cells, it was found that only the IHC staining of aromatase in the carcinoma cells was correlated to the aromatase enzyme activity in the breast tissue [
32]. Therefore, in this study we have firstly evaluated whether carcinoma cell aromatase detection with the #677 antibody gave comparable results in TMA and WS. The observed systematic difference and higher aromatase carcinoma cell staining intensity in WS compared to TMA can be explained by the marked heterogeneity of aromatase expression in the tumor tissue as illustrated in Figure
1E. Thus, the present study can not support TMA analysis of aromatase and accordingly, we have used the aromatase results obtained from WS when analyzing aromatase expression in relation to COX-2, ER and PR.
As mentioned previously, COX-2 is an enzyme that regulates the production of prostaglandins, which in turn regulate the synthesis of aromatase [
36,
37]. Several studies have found association between COX-2 expression and aromatase expression at the transcriptional level [
35,
36,
48], and at the protein level using IHC [
27,
49,
50], supporting that COX-2 may be used as a surrogate marker for aromatase content in tumor tissue [
41]. This is in contrast to our finding, in which we compared the expression of COX-2 and aromatase in invasive carcinoma cells scored by semi-quantitative IHC and found no association between the aromatase expression (SIP score) and COX-2 expression (Allred score). We assume that the lack of association may be due to the complex regulation of the aromatase expression and activity, involving both COX-2 induced prostaglandins, but also many other stimulatory compounds e. g. cyclic-adenosine-monophosphate, glucocorticoids, interleukine-6 and tumor necrosis factor-α [
26,
51‐
57].
We found no association between carcinoma aromatase and PR expression, whereas a strong trend towards association between aromatase and ER in the carcinoma cells was found. This result is supported by Miki et al. who found no correlation between PR status and aromatase mRNA expression level in carcinoma cells and a significant association between aromatase mRNA and ER status in carcinoma cells [
58]. This would imply that
in situ estrogen production in the carcinoma cells is not the major source for ER-induced PR expression, an observation also supported by another recent study [
46] in which aromatase, like ER, was expressed in inherently less aggressive tumors.
In carcinoma cells neither COX-2 nor aromatase expression alone were able to select groups of patients with superior benefit from tamoxifen therapy, but for patients with aromatase positive tumors a high PR expression identified a group of patients for whom endocrine treatment resulted in significantly longer TTP (P = 0.023). For letrozole treatment, patients with aromatase positive tumor cells and high PR expression had longer progression free survival (P = 0.059). This was not observed for patients treated with tamoxifen, indicating that in advanced disease the superiority of letrozole to tamoxifen is primarily observed in the group of patients with aromatase positive and high PR expression in the primary tumor cells.
Acknowledgements
We kindly acknowledge the participating Danish and European Pathology Departments for supplying paraffin embedded tumor material: Aalborg Sygehus, Bispebjerg Hospital, Hjørring Sygehus, Hvidovre Hospital, Nykøbing Falster Sygehus, Odense Universitetshospital, Rigshospitalet, Roskilde Sygehus, Slagelse Sygehus, Svendborg Sygehus, Sønderborg Sygehus, Vejle Sygehus, Viborg Sygehus, J.W. Goethe-Universität, Universitätsklinikum Hamburg-Eppendorf, Centre Regional Francois Baclesse, Centre Hospitalier Général André-Boulloche, Kuopio University Hospital and Turku University Hospital. Katsuhiko Ono, Department of Pathology, Tohoku University School of Medicine, Japan and Birgit S. Hansen, Annegrethe Schaadt, Vinni Bredahl, and Heidi Frogne, Department of Pathology, Roskilde Sygehus, Roskilde, Denmark are acknowledged for excellent technical assistance. This study was supported financially by "Fonden til fremme af klinisk eksperimentiel cancerforskning specielt vedrørende cancer mammae" and Novartis Pharma AG Basel, Switzerland.
Competing interests
D. B. Evans is an employee and share holder of Novartis Pharma AG. The rest of the authors declare that they have no competing interests.
Authors' contributions
AEL supervised the study and participated in drafting and writing of the manuscript. KLH carried out the IHC studies of COX-2, ER and PR and participated in drafting and writing of the manuscript. BBR supervised the IHC studies of COX-2, ER and PR and participated in writing the manuscript. HS carried out all IHC studies of aromatase. SM performed the statistical analysis. DE, BE and HM has participated in its design and coordination. All authors read and approved the final manuscript.