Serotonin and Dopamine Receptor Expression in Solid Tumours Including Rare Cancers

Selection of tumour types for immunohistochemistry was based on results from preclinical studies (colon cancer, ovarian cancer, breast cancer, pancreatic cancer, melanoma) [5‐8, 12] or tumour characteristics (high vascularity for renal cell carcinoma, dopamine production for pheochromocytoma, and serotonin-induced proliferation of precursor cells for gastrointestinal stromal tumours (GIST)) [17, 18].

Formalin-fixed paraffin-embedded primary tumour tissues of colon cancer (n = 12), ovarian cancer (n = 12), breast cancer (n = 12), renal cell carcinoma (n = 14), and pancreatic cancer (n = 12) were used. A minimum of 12 tumours were selected per tumour type, because if 0/12 tumour samples show expression, the chance that it is relevant in >10% of patients is low. Furthermore, 3 tissue microarrays (TMA) were used, namely a melanoma TMA containing 36 tumour samples, a pheochromocytoma TMA containing 63 tumour samples, and a GIST TMA containing 76 tumour samples. The TMAs contained 3 cores with a diameter of 0.6 mm per patient.

Tissue samples used in this study were archival material. According to the Dutch Medical Research Involving Human Subjects act, no approval of the Institutional Review Board was required.

Formalin-fixed, 4 μm thick paraffin-embedded sections and TMAs were deparaffinized and rehydrated. Antigen retrieval was performed using heated citrate buffer (pH 6.0) for 5-HTR1B, 5-HTR2B, DRD1, and DRD2 or tris/EDTA buffer (pH 9.0) for CD31 for 15 min. For DRD2, slides were blocked with phosphate-buffered saline (PBS; pH 7,4) plus 0.1% Tween-20 for 20 min at room temperature. Endogen peroxidase was blocked in all slides with 1% H₂O₂ in PBS for 30 min at room temperature. For 5-HTR1B, additional avidin/biotin (avidin/biotin blocking kit (SP-2001); Vector Laboratories, Brunschwig Chemie, Amsterdam, The Netherlands) and human serum blocks were performed. The sections were incubated with the primary antibody for 1 h at room temperature for 5-HTR2B, DRD1, and CD31 or overnight at 4 °C for 5-HTR1B and DRD2. Primary antibodies used were mouse monoclonal 5-HTR1B 1:100 (clone 499,325; MAB5858, R&D systems, Abingdon, United Kingdom), mouse monoclonal 5-HTR2B 1:1000 (clone H-11; sc-376,834, Santa Cruz Biotechnology, Bio-Connect, Huissen, The Netherlands), mouse monoclonal DRD2 1:100 (clone B-10, sc-5303, Santa Cruz Biotechnology), rat monoclonal DRD1 1:75 (clone 1–1-F11 s.E6; D2944, Sigma Aldrich, Zwijndrecht, The Netherlands), and mouse monoclonal CD31 1:50 (clone JC70A; IR610, DAKO, Glostrup, Denmark). Subsequently, tissue sections were incubated with secondary antibodies (1:100 dilution or in case of 5-HTR1B a 1:300 dilution; all from DAKO). Between steps, slides were washed with PBS or in case of DRD2 with PBS plus 0.1% Tween-20. Staining was visualized using 3,3′-diaminobenzidine (DAB) and hematoxylin for counterstaining. Positive and negative controls (including immunoglobulin class-matched control sera) were included for each staining. Colon, testis, and prostate tissue served to validate the stainings as positive and negative controls. In addition standard hematoxylin & eosin (H&E) stainings were performed to evaluate tissue morphology.

After immunohistochemical staining, slides were digitally scanned using the NanoZoomer (Hamamatsu Photonics, Shizuoka, Japan) and were scored using accompanied NanoZoomer Digital Pathology (NDP) software. All slides were scored by two independent investigators (M.P. and C.M. or H.H.) and compared to assure a minimal inter-observer difference. As an extra control, random slides were also evaluated by a pathologist (H.H.).

Tissue morphology was evaluated using H&E-stained slides. Staining intensity of the tumour cells and percentage of positive tumour cells was scored. Staining intensity of tumour cells was scored as negative (0), low (1), moderate (2), or high (3). The percentage of positive tumour cells was scored as no positive cells (0), 1–4% positive cells (1), 5–24% positive cells (2), 25–49% positive cells (3), 50–74% positive cells (4), and 75–100% positive cells (5). Receptor expression was scored using an immunoreactive score (IRS) to account for the heterogeneous staining in the section slides [19]. The IRS was defined by multiplying the staining intensity (category 0–3) with the percentage of positive tumour cells (category 0–5), creating a range from 0 to 15. Receptor expression was considered negative if IRS was 0, low if the IRS was 1 to 5, and high if the IRS was 6 to 15. For TMAs, at least two evaluable cores had to be present per tumour in order to consider it a representative score.

Receptor expression on tumour-associated blood vessels was only assessed on the whole tissue sections, as blood vessels were only in limited numbers or not at all present in the TMA samples due to their small diameter. Serotonin and dopamine receptor expression was scored by staining intensity (ranging from 0 to 3). Receptor expression was considered negative if intensity was 0, low if intensity was 1, and high if intensity was 2 or 3, CD31 staining was performed to confirm localization of tumour vessels.