Skip to main content
PMC home page
BMC Cancer logoLink to BMC Cancer
. 2015 Mar 29;15:199. doi: 10.1186/s12885-015-1217-x

A multiplexed, targeted mass spectrometry assay of the S100 protein family uncovers the isoform-specific expression in thyroid tumours

Juan Martínez-Aguilar 1,2, Roderick Clifton-Bligh 3, Mark P Molloy 1,2,
PMCID: PMC4391164  PMID: 25880590

Abstract

Background

Mounting evidence demonstrates a causal role for S100 proteins in tumourigenesis and several S100 isoforms have shown utility as biomarkers of several types of cancer. The S100 family is comprised of 21 small isoforms, many of them implicated in important cellular functions such as proliferation, motility and survival. Furthermore, in vivo experiments have proven the role of S100 proteins in tumour growth and disease progression, while other studies have shown their prognostic value and involvement in resistance to chemotherapy drugs. Taken together, all these aspects highlight S100 proteins as potential therapeutic targets and as a promising panel of cancer biomarkers. In this work, we have developed a mass spectrometry (MS)-based method for the multiplexed and specific analysis of the entire S100 protein family in tumour tissues and have applied it to investigate the expression of S100 isoforms in the context of thyroid cancer, the main endocrine malignancy.

Methods

Selected Reaction Monitoring (SRM)-MS and stable isotope labelling/label-free analysis were employed to investigate the expression of the 21 S100 protein isoforms in thyroid tissue samples. Specimens included 9 normal thyroid tissues and 27 tumour tissues consisting of 9 follicular adenomas (FA), 8 follicular carcinomas (FTC) and 10 papillary carcinomas (PTC).

Results

The multiplexed and targeted mass spectrometry method led to the detection of eleven S100 protein isoforms across all tissues. Label- and label-free analyses showed the same significant differences and results were confirmed by western blot. S100A6, S100A11 and its putative interaction partner annexin A1 showed the highest overexpression in PTC compared to normal thyroid. S100A13 was also elevated in PTC. Reduced S100A4 expression was observed in FA compared to all other tissues. FA and FTC showed reduction of S100A10 and annexin A2 expression.

Conclusions

Targeted mass spectrometry allows the multiplexed and specific analysis of S100 protein isoforms in tumour tissue specimens. It revealed S100A13 as a novel candidate PTC biomarker. Results show that S100A6, S100A11 and Annexin A1 could help discriminate follicular and papillary tumours. The diagnostic and functional significance of S100A4 and S100A10 reduction in follicular tumours requires further investigation.

Electronic supplementary material

The online version of this article (doi:10.1186/s12885-015-1217-x) contains supplementary material, which is available to authorized users.

Keywords: S100 proteins, Selected reaction monitoring, Mass spectrometry, Thyroid cancer, Tumour tissue samples

Background

Growing evidence links the S100 protein family with cancer [1,2]. This protein superfamily consists of 21 small isoforms (9-13 kDa), which are characterised by their calcium binding ability and conserved primary and secondary structures (the sequence identity among S100 proteins ranges from 16 to 98% [3]). Besides exhibiting some degree of cell specificity, S100 isoform expression depends on environmental factors to regulate important cellular functions such as proliferation and motility. When secreted from cells, some S100 proteins exert chemotactic and angiogenic activities, thereby further contributing to the tumourigenic process [2,4]. Indeed, in vivo experiments have proven the role of several S100 proteins in tumour growth and disease progression [2].

Dysregulation of S100 isoform expression has been observed in numerous cancers [2,5] (see Additional file 1: Table S1). For example, S100A4, S100A6, S100A8, S100A9, S100A11 and S100P have shown altered expression in breast, colorectal, gastric, pancreatic and prostate cancer [6-30]. S100A6, S100A13 and S100B have been found as overexpressed in melanoma [31-33], and likewise other S100 proteins have been identified as biomarkers in cancer of the bladder, lung and oesophagus [34-37]. In many instances, the S100 isoforms have also demonstrated prognostic and predictive value, ultimately representing candidate therapeutic targets. For example, S100A4 elevation in colorectal cancer has been associated with decreased survival rate [6,38] and S100A4 inhibition using regulators of β-catenin signalling such as niclosamide or sulindac has shown reduction of liver metastasis in mouse xenograft models [39,40]; S100A6 overexpression in gastric cancer could serve as independent prognostic predictor associated with poor survival [41] and S100A6 knockdown in gastric cancer cells has been shown to inhibit tumour growth in vivo [42]. Another S100 isoform, S100P, has been described as a key factor in the aggressiveness of pancreatic cancer [30] and has recently been reported as a promising target of monoclonal antibody therapy, significantly reducing tumour growth and metastasis in a mouse model [43].

Despite the promising potential of the S100 family as a biomarker panel, there is an absence of studies that have addressed the family-wide expression of S100 protein isoforms in clinical samples [44]. This is a challenging task when relying on traditional affinity-based procedures (e.g. immunohistochemistry) due to potential S100 antigen cross-reactivity and the serial nature of optimising and performing IHC assay. We recently developed a targeted mass spectrometry (MS) method based on Selected Reaction Monitoring (SRM) that enables unequivocal structural evidence for the detection of the entire S100 protein family in cancer cells [45]. Here, we have adapted and extended its application for the study of tumour tissues and demonstrate this application in the context of thyroid cancer, the principal malignancy of the endocrine system. The targeted MS approach allowed us to establish the first global picture of S100 protein expression in the three most common tumours of the thyroid gland: follicular adenoma (FA), follicular thyroid carcinoma (FTC) and papillary thyroid carcinoma (PTC). While the latter is the major type of thyroid cancer, tumours with follicular growth pattern (FA and FTC) are indeterminate by fine-needle aspiration (FNA) biopsy, hence hampering the pre-operative diagnosis of tumour malignancy [46,47]. Our results revealed isoform-specific association of S100 proteins in thyroid tumours implicating S100 isoforms have diagnostic potential.

Methods

Thyroid tissue samples

Fresh frozen thyroid tissues (9 normal, 9 FA, 8 minimally invasive FTC and 10 classical PTC) were obtained from the neuroendocrine tumour bank at the Kolling Institute of Medical Research, Sydney. Normal samples were obtained from dissection of non-neoplastic tissue from the contralateral lobe of patients who had undergone thyroidectomy or from patients with benign disease where thyroidectomy was indicated. Clinicopathological features are shown in Table 1. All PTC cases showed lymph node metastasis. The research work was conducted with the approval of the human research ethics committees of the Northern Sydney Local Health District (1303-091 M) and Macquarie University (5201300037).

Table 1.

Clinicopathological features of the thyroid tissue samples analysed

Normal tissues Follicular adenomas
Age Sex Age Sex Tumour size (mm)
Normal-1 42 F FA-1 36 M 30
Normal-2 20 F FA-2 51 F 15
Normal-3 78 F FA-3 30 F 30
Normal-4 61 M FA-4 46 F 50
Normal-5 51 M FA-5 46 M 30
Normal-6 34 F FA-6 14 F 8
Normal-7 84 M FA-7 21 M 21
Normal-8 35 M FA-8 68 F 8
Normal-9 29 F FA-9 59 F 10
Follicular thyroid carcinomas
Age of onset Sex Tumour size (mm) T stage Capsular invasion Vascular invasion
FTC-1 43 F 50 3 no yes
FTC-2 37 M 40 3 yes yes
FTC-3 82 M 45 3 encapsulated yes
FTC-4 16 M 13 1 yes no
FTC-5 64 F 40 2 no yes
FTC-6 64 F 25 yes (focal) no
FTC-7 20 M 110 3 no yes
FTC-8 22 M 30 2 yes yes
Papillary thyroid carcinomas
Age of onset Sex Tumour size (mm) T stage Vascular invasion Extra-thyroidal spread
PTC-1 34 F 18 2 no no
PTC-2 24 F 30 2 yes no
PTC-3 50 M 6 4 no yes
PTC-4 59 M 30 3 yes yes
PTC-5 33 F 8 1 no no
PTC-6 32 F 55 4 yes yes
PTC-7 24 F 45 3 no no
PTC-8 33 F 28 3 yes yes
PTC-9 49 M 44 3 no yes
PTC-10 56 M 55 4 yes yes
Open in a new tab

Metabolic (SILAC) labelling of TPC1 cells for a spike-in standard

SILAC RPMI 1640 media (Thermo Scientific Pierce) was supplemented with 240 mg/mL of L-arginine‐HCl (13C615N4) and 40 mg/mL of L‐lysine‐2HCl (13C615N2) (Cambridge Isotope Labs), 10% dialysed FBS (Life Technologies) and 1% Penicillin-Streptomycin (Gibco). The medium was sterile filtered through a 0.22 micron filter. TPC1 thyroid cancer cells were cultured for at least eight doublings at 37°C in a humidified atmosphere with 5% CO2. Upon reaching 70-90% confluence, cells were washed with phosphate buffered saline (PBS), harvested and stored at -80°C until use. Heavy amino acid incorporation was verified by MS.

Cell and tumour sample preparation

TPC1 cells and tumour samples were suspended in lysis buffer (20 mM HEPES, 1% sodium deoxycholate (SDOC), 0.1% SDS, 150 mM NaCl, 1 mM EDTA, pH 8) with complete, EDTA-free protease inhibitor cocktail (Roche), phosphatase inhibitor tablet (Thermo Scientific Pierce) and lysed on ice with sonication (three cycles of 20 s pulses). Lysates were centrifuged (12 000 g, 10 min, 4°C) and the supernatants retained. Protein quantitation was performed with a BCA protein assay kit (Thermo Scientific).

40 ug of protein from tissue samples and 20 ug of protein from metabollically labelled TPC1 cells were mixed in triplicate before SDS-PAGE. A ratio 2:1 of sample protein to labelled protein was employed given that previous tests measuring the abundance of candidate reference proteins showed varying levels of actual tumour protein amount in different samples due to the presence of blood proteins. Labelled TPC1 cells allowed the quantitative analysis of candidate reference proteins and S100 proteins S100A2, S100A6, S100A10, S100A11 and S100A13. It is not unexpected that a particular cell line does not express detectable levels of all S100 isoforms, therefore additional stable isotope-labelled S100 synthetic peptides were spiked into the samples before tryptic digestion (see below for details). While it is conceivable to perform the entire analysis using stable isotope-labelled peptides from reference proteins and S100 proteins, using the SILAC spike-in represents a less expensive approach that does not rely on prior knowledge of the most appropriate peptide sequence to represent the target analyte.

In addition, label-free MS analysis to quantitate all S100 proteins was also carried out as we previously described [45]. To this end, a reference stock sample was prepared, comprised of 700 ug of protein from TPC1 cells grown in normal RPMI medium and 600 ug of protein pooled from the entire set of normal, FA, FTC and PTC tumour lysates. 40 ug of this mixture was loaded onto a Bis-Tris NuPAGE gel for separation. The set of tissue samples was randomised and prepared in batches of four samples (one from each tissue type as far as possible considering the different sample sizes) plus the reference sample. All samples were loaded on gels in triplicate and processed as described below.

Corresponding aliquots of specimens and reference samples were mixed with NuPAGE LDS sample buffer (Invitrogen) and 50 mM dithiothreitol (DTT), incubated at 70°C for 10 min and loaded onto 4-12% Bis-Tris NuPAGE gels (Invitrogen). Proteins were separated using MES running buffer (200 V, 25 min), fixed into the gel with 50% ethanol/10% acetic acid for 1 h and then stained for 1 h with colloidal Coomassie G-250 (Sigma). Gel bands from three mass regions were excised (7-14 kDa, 14-32 kDa and 32-100 kDa), cut into approximately 1 × 1 mm cubes and destained with 50% ACN in 50 mM ammonium bicarbonate (AmBic, pH 8.0). Gel pieces were dehydrated with 100% ACN, speed-vac dried and incubated in 10 mM DTT/100 mM Ambic at 56°C for 1 h followed by treatment with 55 mM iodoacetamide/100 mM AmBic at RT in the dark for 45 min. Gel pieces were dehydrated again, speed-vac dried, rehydrated with 120 uL of 13 ng/uL trypsin solution (sequencing grade modified trypsin (Promega) in 50 mM AmBic and 0.1% SDOC) and kept on ice for 1 h.

Before tryptic digestion, gel pieces from the region 7-14 kDa were spiked with 2 pmol of 13C, 15N stable-isotope labelled peptide standards ELPSFLGK (S100A4), ALNSIIDVYHK (S100A8), NIETIINTFHQYSVK (S100A9) and 1 pmol of SFWELIGEAAK (S100A14) and AVIVLVENFYK (S100A16) (SpikeTides TQL, JPT Peptide Technologies, Germany). This step allowed the inclusion of additional labelled S100 peptides not detected in TPC1 cells according to preliminary tests. All samples were then incubated overnight at 37°C. Peptides were extracted thrice with 0.1% SDOC in ultrasonic waterbath for 10 min and then acidified with 1 uL of formic acid. The precipitate was removed by centrifugation (14000 g, 10 min) and the samples were dried in a speed-vac, ready for LC-SRM-MS.

LC-SRM-MS

The selection of S100 peptides, transitions and optima MS parameters was based on our previous work [45]. The sequences from candidate reference proteins and putative S100 interaction partners annexin A1 (ANXA1) and annexin A2 (ANXA2) were searched by BLAST and Peptide Atlas to identify suitable unique tryptic peptides with more than six amino acids and free of methionine residues. S100 proteins to be quantitated in the tissue samples were detected on preliminary analyses of each sample using the list of SRM transitions reported in Additional file 1: Table S2. These transitions were monitored and also served to assign the retention times of each peptide for subsequent time-scheduled SRM. According to their localisation on the gels, Table 2 lists the peptide sequences and SRM parameters employed for the analysis of S100 proteins and Additional file 1: Tables S3 and S4 the candidate reference proteins in the thyroid tissues.

Table 2.

Targeted S100 peptide sequences (region 7-14 kDa)

Q1 Q3 Rt Protein.peptide.transition ion.isotopologue CE CEXP
846.45 778.41 31.5 S100A1.ELLQTELSGFLDAQK.y7.light 39.3 13
846.45 865.44 31.5 S100A1.ELLQTELSGFLDAQK.y8.light 39.3 13
846.45 1208.62 31.5 S100A1.ELLQTELSGFLDAQK.y11.light 39.3 13
503.27 763.40 23.5 S100A2.ELPSFVGEK. + 2y7.light 22.7 12
503.27 666.35 23.5 S100A2.ELPSFVGEK. + 2y6.light 30.7 11
503.27 579.31 23.5 S100A2.ELPSFVGEK. + 2y5.light 30.7 9
507.27 771.41 23.5 S100A2.ELPSFVGEK. + 2y7.heavy 22.7 12
507.27 674.36 23.5 S100A2.ELPSFVGEK. + 2y6.heavy 30.7 11
507.27 587.33 23.5 S100A2.ELPSFVGEK. + 2y5.heavy 30.7 9
445.75 648.37 25.5 S100A4.ELPSFLGK. + 2y6.light 21.5 19
445.75 551.32 25.5 S100A4.ELPSFLGK. + 2y5.light 25.5 19
445.75 464.29 25.5 S100A4.ELPSFLGK. + 2y4.light 25.5 16
449.76 656.39 25.5 S100A4.ELPSFLGK. + 2y6.heavy 21.5 19
449.76 559.33 25.5 S100A4.ELPSFLGK. + 2y5.heavy 25.5 19
449.76 472.30 25.5 S100A4.ELPSFLGK. + 2y4.heavy 25.5 16
455.22 693.36 16.0 S100A4.TDEAAFQK. + 2y6.light 21.2 20
455.22 564.31 16.0 S100A4.TDEAAFQK. + 2y5.light 21.2 20
455.22 493.28 16.0 S100A4.TDEAAFQK. + 2y4.light 21.2 14
459.23 701.37 16.0 S100A4.TDEAAFQK. + 2y6.heavy 21.2 20
459.23 572.33 16.0 S100A4.TDEAAFQK. + 2y5.heavy 21.2 20
459.23 501.29 16.0 S100A4.TDEAAFQK. + 2y4.heavy 21.2 14
374.22 618.38 18.5 S100A6.ELTIGSK. + 2y6.light 20.3 13
374.22 505.30 18.5 S100A6.ELTIGSK. + 2y5.light 20.3 13
374.22 404.25 18.5 S100A6.ELTIGSK. + 2y4.light 20.3 13
378.22 626.40 18.5 S100A6.ELTIGSK. + 2y6.heavy 20.3 13
378.22 513.31 18.5 S100A6.ELTIGSK. + 2y5.heavy 20.3 13
378.22 412.26 18.5 S100A6.ELTIGSK. + 2y4.heavy 20.3 13
458.25 802.41 17.5 S100A6.LQDAEIAR. + 2y7.light 25.4 13
458.25 674.35 17.5 S100A6.LQDAEIAR. + 2y6.light 23.4 20
458.25 559.32 17.5 S100A6.LQDAEIAR. + 2y5.light 31.4 17
463.25 812.41 17.5 S100A6.LQDAEIAR. + 2y7.heavy 25.4 13
463.25 684.36 17.5 S100A6.LQDAEIAR. + 2y6.heavy 23.4 20
463.25 569.33 17.5 S100A6.LQDAEIAR. + 2y5.heavy 31.4 17
636.85 774.41 24.5 s100A8.ALNSIIDVYHK.y6.light 31.8 13
636.85 974.53 24.5 s100A8.ALNSIIDVYHK.y8.light 31.8 13
636.85 887.50 24.5 s100A8.ALNSIIDVYHK.y7.light 31.8 13
640.86 782.42 24.5 S100A8.ALNSIIDVYHK.y6.heavy 31.9 13
640.86 982.54 24.5 S100A8.ALNSIIDVYHK.y8.heavy 31.9 13
640.86 895.51 24.5 S100A8.ALNSIIDVYHK.y7.heavy 31.9 13
602.98 790.42 30.0 S100A9.NIETIINTFHQYSVK.y13.light 30.4 13
602.98 725.89 30.0 S100A9.NIETIINTFHQYSVK.y12.light 30.4 13
602.98 618.83 30.0 S100A9.NIETIINTFHQYSVK.y10.light 30.4 13
605.65 794.43 30.0 S100A9.NIETIINTFHQYSVK.y13.heavy 30.5 13
605.65 729.90 30.0 S100A9.NIETIINTFHQYSVK.y12.heavy 30.5 13
605.65 622.84 30.0 S100A9.NIETIINTFHQYSVK.y10.heavy 30.5 13
379.21 642.38 18.0 S100A10.DPLAVDK. + 2y6.light 22.5 19
379.21 545.33 18.0 S100A10.DPLAVDK. + 2y5.light 20.5 17
379.21 432.25 18.0 S100A10.DPLAVDK. + 2y4.light 20.5 17
383.22 650.40 18.0 S100A10.DPLAVDK. + 2y6.heavy 22.5 19
383.22 553.34 18.0 S100A10.DPLAVDK. + 2y5.heavy 20.5 17
383.22 440.26 18.0 S100A10.DPLAVDK. + 2y4.heavy 20.5 17
604.80 932.48 26.0 S100A10.EFPGFLENQK. + 2y8.light 26.6 13
604.80 835.43 26.0 S100A10.EFPGFLENQK. + 2y7.light 34.6 13
604.80 466.75 26.0 S100A10.EFPGFLENQK. + 2y8 + 2.light 26.6 13
608.81 940.50 26.0 S100A10.EFPGFLENQK. + 2y8.heavy 26.6 13
608.81 843.45 26.0 S100A10.EFPGFLENQK. + 2y7.heavy 34.6 13
608.81 470.75 26.0 S100A10.EFPGFLENQK. + 2y8 + 2.heavy 26.6 13
386.20 559.32 18.0 S100A11.DPGVLDR. + 2y5.light 24.2 18
386.20 502.30 18.0 S100A11.DPGVLDR. + 2y4.light 24.2 18
386.20 403.23 18.0 S100A11.DPGVLDR. + 2y3.light 20.2 18
391.21 569.33 18.0 S100A11.DPGVLDR. + 2y5.heavy 24.2 18
391.21 512.31 18.0 S100A11.DPGVLDR. + 2y4.heavy 24.2 18
391.21 413.24 18.0 S100A11.DPGVLDR. + 2y3.heavy 20.2 18
530.75 888.45 20.0 S100A11.DGYNYTLSK. + 2y7.light 24.0 14
530.75 725.38 20.0 S100A11.DGYNYTLSK. + 2y6.light 24.0 12
530.75 611.34 20.0 S100A11.DGYNYTLSK. + 2y5.light 24.0 18
534.76 896.46 20.0 S100A11.DGYNYTLSK. + 2y7.heavy 24.0 14
534.76 733.40 20.0 S100A11.DGYNYTLSK. + 2y6.heavy 24.0 12
534.76 619.35 20.0 S100A11.DGYNYTLSK. + 2y5.heavy 24.0 18
519.76 836.45 22.5 S100A13.DSLSVNEFK. + 2y7.light 23.6 13
519.76 723.37 22.5 S100A13.DSLSVNEFK. + 2y6.light 23.6 20
519.76 636.34 22.5 S100A13.DSLSVNEFK. + 2y5.light 23.6 20
523.77 844.47 22.5 S100A13.DSLSVNEFK. + 2y7.heavy 23.6 13
523.77 731.38 22.5 S100A13.DSLSVNEFK. + 2y6.heavy 23.6 20
523.77 644.35 22.5 S100A13.DSLSVNEFK. + 2y5.heavy 23.6 20
372.24 630.38 20.5 S100A13.LIGELAK. + 2y6.light 19.5 19
372.24 517.30 20.5 S100A13.LIGELAK. + 2y5.light 17.5 15
372.24 460.28 20.5 S100A13.LIGELAK. + 2y4.light 25.5 16
376.24 638.40 20.5 S100A13.LIGELAK. + 2y6.heavy 19.5 19
376.24 525.31 20.5 S100A13.LIGELAK. + 2y5.heavy 17.5 15
376.24 468.29 20.5 S100A13.LIGELAK. + 2y4.heavy 25.5 16
624.31 1047.50 20.0 S100A13.SLDVNQDSELK. + 2y9.light 31.3 16
624.31 932.47 20.0 S100A13.SLDVNQDSELK. + 2y8.light 31.3 16
624.31 833.40 20.0 S100A13.SLDVNQDSELK. + 2y7.light 31.3 14
628.32 1055.51 20.0 S100A13.SLDVNQDSELK. + 2y9.heavy 31.3 16
628.32 940.48 20.0 S100A13.SLDVNQDSELK. + 2y8.heavy 31.3 16
628.32 841.41 20.0 S100A13.SLDVNQDSELK. + 2y7.heavy 31.3 14
625.82 1016.54 31.5 S100A14.SFWELIGEAAK. + 2y9.light 29.0 17
625.82 830.46 31.5 S100A14.SFWELIGEAAK. + 2y8.light 29.0 13
625.82 701.42 31.5 S100A14.SFWELIGEAAK. + 2y7.light 32.0 12
629.83 1024.56 31.5 S100A14.SFWELIGEAAK. + 2y9.heavy 29.0 17
629.83 838.48 31.5 S100A14.SFWELIGEAAK. + 2y8.heavy 29.0 13
629.83 709.43 31.5 S100A14.SFWELIGEAAK. + 2y7.heavy 32.0 12
647.87 912.48 31.0 S100A16.AVIVLVENFYK. + 2y7.light 28.0 14
647.87 799.40 31.0 S100A16.AVIVLVENFYK. + 2y6.light 24.0 13
647.87 700.33 31.0 S100A16.AVIVLVENFYK. + 2y5.light 26.0 12
651.88 920.50 31.0 S100A16.AVIVLVENFYK. + 2y7.heavy 28.0 14
651.88 807.41 31.0 S100A16.AVIVLVENFYK. + 2y6.heavy 24.0 13
651.88 708.34 31.0 S100A16.AVIVLVENFYK. + 2y5.heavy 26.0 12
Open in a new tab

Rt: retention time (min), CE: collision energy; CEXP: cell exit potential.

Samples were analysed using a Waters nanoACQUITY UPLC system coupled to the QTRAP 5500 mass spectrometer (AB Sciex). Weak (A) and strong (B) elution solvents were 0.1% FA (v/v) in water and 0.1% FA (v/v) in ACN, respectively. Samples were loaded onto a Waters Symmetry C18 trapping column (180 um × 20 mm, 5 um particle size) and peptides were separated on a Waters BEH C18 nano UPLC column (100 um × 100 mm, 1.7 um particle size) at 35°C under constant flow rate of 0.4 uL/min. Different elution gradients were used depending on the regions from the gel: a) 7-14 kDa: 3% solvent B for 1 min, 3-40% B in 30 min and 40-85% B in 2 min, b) 14-32 kDa: 3% solvent B for 1 min, 3-40% B in 60 min and 40-85% B in 2 min, c) 32-100 kDa: 3% solvent B for 1 min, 3-40% B in 110 min and 40-85% B in 2 min.

Peptide samples were reconstituted with a solution of 2% ACN/0.1% TFA (v/v) and 17.8 fmol/uL of 13C15N stable isotope-labelled peptide ESDTSYVSLK from human C-reactive protein (Auspep, Australia), used as LC loading control for label-free experiments. Blank injections using a 30 min gradient were performed between each sample. The lists of peptide sequences in Table 2 and Additional file 1: Tables S3 and S4 were targeted using three transitions per peptide with corresponding time-scheduled SRM methods employing cycle times of 1 s and transition windows of 240 s for peptides shown in Table 2 and Additional file 1: Table S3 and 360 s for those listed in Additional file 1: Table S4. The nano-ESI source was operated in positive mode at 2.5 kV with interface heater temperature of 150°C. Curtain gas was set to 20 psi, declustering potential at 70 V and both Q1/Q3 were set at unit resolution. Collision energies (CE) for candidate reference peptides were calculated based on the equations CE(2+) = 0.036*m/z + 8.857 and CE(3+) = 0.0544*m/z-2.4099, taken from Skyline. Peptide identities were corroborated by SRM-triggered IDA MS/MS and searched in the UniProt human database using Mascot v. 2.3.0.

Data analysis

The potential for peptide interferences was monitored with AuDIT software [48] and signals marked as problematic were removed. Data were processed with Multiquant 3.0 (AB Sciex) using the MQ4 integration algorithm. Manual inspection of the fragment ion peaks was performed to ensure accurate integration. The respective fragment ion peak areas of each endogenous peptide were summed and divided by the transition areas of the isotopically labelled counterparts. The calculated values of different peptides from the same protein were averaged.

In the case of label-free analyses, co-elution of fragment ions and consistency of retention times were used as a guide for peak identity assignment. Signals with CV less than 20% in transition ratios across samples and replicates were considered to represent interference-free conditions. Summed raw peak areas were first divided by the total peak area of the spiked CRP peptide and then against the peak areas of the same peptides present in a reference pool sample that was prepared in the same batch along with the samples of interest. This was done to compensate for differences in sample preparation and system response as detailed in [45]. Again, the average of different peptides from the same protein was calculated. The normalisation factors previously obtained by isotopic labelling were employed for calculation of relative S100 protein expression, thereby keeping maximum precision in this preceding step and allowing the analysis of S100 proteins not detected in the SILAC spike-in standard or not added as heavy peptides before tryptic digestion.

Identification of the most stably expressed endogenous reference proteins across all the thyroid tissue samples (normal, FA, FTC and PTC) was performed using the geNorm algorithm, developed by Vandesompele et al. [49]. The geometric mean of SRM-based values of the identified reference proteins was employed as the normalisation factor to calculate the relative expression of S100 proteins in each sample. Comparison of relative S100 protein expression was carried out by one-way anova and Tukey’s post hoc test (p < 0.05) using GraphPad Prism 5.0 software, which was also used for linear regressions analyses. Area under the curve (AUC) of a receiver operating characteristic (ROC) curve was calculated using the ROCR R package.

Validation of results by Western Blot

Taking into account the normalisation factors derived from the reference proteins, 10 ug of protein from tissue lysates of normal, FA, FTC and PTC samples were separated on 4-12% Bis-Tris NuPAGE gels and electroblotted onto nitrocellulose (Bio-Rad). The membrane was blocked with 5% skim milk in TBS for 1 h at RT. For S100A4 analysis, the membrane was cut in three sections from around 5-17 kDa, 17-32 kDa and >32 kDa. The sections were incubated overnight at 4°C with a) 5-17 kDa - rabbit polyclonal anti-S100A4 (1:100, AbCam), b) 17-32 kDa - rabbit monoclonal anti-Rab7a (1:500, Cell signaling) and c) rabbit monoclonal anti-β-Tubulin (1:500, Cell signaling). For S100A13 analysis, the membrane was cut in two sections (5-17 kDa and >32 kDa) and incubated overnight with either rabbit monoclonal anti-S100A13 (1:3000, AbCam) or rabbit monoclonal anti-Rab7a (1:500, Cell signaling). The secondary antibody was fluorescence-labelled IRDye 800CW goat anti-rabbit IgG (H + L) (1:10 000 in 5% skim milk in TBST, LI-COR), incubated at RT for 1 h and visualized with the Odyssey infrared imaging system.

Results

Identification of stable endogenous reference proteins in thyroid tumours

Because tumour specimens contain naturally variable amounts of blood proteins, and in the case of thyroid specimens, thyroglobulin, a simple protein quantitation assay would be insufficient for normalising loading quantities which is a requirement for accurate quantitation. Therefore, our first task was to identify endogenous reference proteins within thyroid tumours that could be used for loading normalisation. Traditionally, ‘housekeeping genes/proteins’ like GAPDH and β-actin have been used as normalisation loading controls; however, increasing evidence shows that these may not be the best reference proteins as their expression stability is compromised when compared across different groups of samples or disease states [49,50]. We used SRM to investigate the expression stability of 18 proteins/genes commonly reported as internal reference standards based on gene expression profiling studies [50,51] (Additional file 1: Tables S3 and S4).

In the geNorm method by Vandesompele et al. [49], pairwise comparisons between each of the candidate proteins are carried out and an expression stability value M is calculated, which represents the average pairwise variation across all samples of a particular protein compared with the remaining proteins tested. In a first instance, the geNorm algorithm showed proteasome subunit beta type-4 (PROS26) and proteasome subunit beta type-2 (PSMB2) as the protein pair with the highest stability, followed by several ribosomal proteins, valosin containing protein (VCP), Ras-related protein Rab7a and cyclophilin A. β-Tubulin, β-Actin and GAPDH showed higher variation (see Figure 1a). This result served to verify the consistency of our reference protein dataset since PSMB2, PROS26, ribosomal proteins and VCP are all involved in the ubiquitin-proteasome system [52-55]. In order to minimise the possibility of co-regulation we kept proteins belonging to different functional classes: Rab7a (regulator of endo-lysosomal trafficking), cyclophilin A (regulator of protein folding), PSMB2 (proteasome, proteolytic activity), β-Tubulin (cytoskeletal protein), GAPDH (glycolytic protein) and protein TB2 (receptor accessory protein). We retained and tested β-actin, another cytoskeletal protein, given its frequent use in most expression studies.

Figure 1.

Figure 1

Open in a new tab

Determination of reference proteins using the geNorm algorithm. a) Average expression stability values of candidate reference proteins; b) Determination of the optimal number of reference proteins for normalisation. Pairwise variations Vn/n + 1 are calculated between two sequential normalisation factors and stepwise inclusion of the most stable remaining control protein.

From the selected subset, Rab7a and cyclophilin A were the most stable proteins identified (Figure 1a) and pairwise variation analysis of the corresponding normalisation factors helped to determine that Rab7a, cyclophilin A and PSMB2 compose a minimal set of stable endogenous reference proteins in thyroid tissues (Figure 1b).

Detection of S100 protein family by targeted MS

Our targeted MS assay for all members of the S100 protein family revealed that the following eleven S100 protein isoforms were detected across all normal, FA, FTC and PTC tissues: S100A1, S100A2, S100A4, S100A6, S100A8, S100A9, S100A10, S100A11, S100A13, S100A14 and S100A16 (Figure 2 and Additional file 1: Figure S1). The MS assay employing the SILAC spike-in standard was highly reproducible with median coefficient of variation (CV) of 5.8%. Although each S100 peptide has its own MS characteristics, our previous work with spiking experiments of six stable isotope-labelled peptides (ELPSFVGEK, S100A2; ELPSFLGK, S100A4; LQDAEIAR, S100A6; DPGVLDR, S100A11; LIGELAK, S100A13 and AVIVLVENFYK, S100A16) demonstrated linear response with up to 3 pmol on-column [45] and we have made broad estimates of the limits of quantitation to be approximately 0.5 fmol (considering lowest concentration with CV <20%), which is consistent with the commonly observed detection limits for peptide SRM being in the sub-femtomolar range [56].

Figure 2.

Figure 2

Open in a new tab

Differential expression of S100 proteins in normal thyroid and tumour tissues, analysed by spike-in SILAC-SRM. Normalised expression values were log-transformed and significant changes of S100 protein isoform expression were identified by one-way anova followed by Tukey’s post hoc test (*p < 0.05, **p < 0.01, ***p < 0.001). Results are expressed against the mean S100 protein expression in normal thyroid tissue samples.

Targeted MS revealed S100A13 as a novel candidate marker of PTC

As shown in Figure 2, S100A13 was found overexpressed in tumours of PTC origin (log2fc = 1.03, p < 0.05) compared to normal thyroid. Additionally, increased expression of S100A13 was generally observed in FA and FTC specimens, although this varied considerably amongst these samples. Analysis of four publicly available gene expression datasets, three of them comparing matched normal-PTC tumour samples, confirmed the overexpression of S100A13 mRNA transcripts in PTC (Additional file 1: Figure S2). The SRM-based results were validated by Western Blot (Figure 3a) and were highly correlated (r2 = 0.86) (Figure 3b).

Figure 3.

Figure 3

Open in a new tab

Validation of SRM-based results and correlated expression of S100 proteins with ANXA1 and ANXA2. a) Western blot of S100A13 showing overexpression in PTC tissues; b) Western Blot of S100A13 (S100A13/Rab7a, one PTC outlier excluded) showed agreement with SRM-based results; c) Western blot of S100A4, β-tubulin and Rab7a in thyroid tumours and normal thyroid . β-tubulin presented higher variation (CV = 46%) than Rab7a (CV = 19%); d) Normalised S100A4 expression (S100A4/Rab7a) was well correlated with that from SRM analysis. e) Expression of S100A11 and its interaction partner ANXA1 are highly correlated across all samples, and are overexpressed in PTC; f) Expression of S100A10 and its interaction partner ANXA2 are also highly correlated across all samples, and are both reduced in FA and FTC.

S100A4 is frequently reduced in tumours of follicular origin

S100A4 expression was greatly decreased in benign follicular adenomas compared with normal thyroid tissue. FTCs expressed higher levels of S100A4 than FAs, but still less than normal thyroid and PTC specimens (Figure 2). Western Blot confirmed the quantitative MS results of S100A4 expression in the tissue samples (Figure 3c and d).

S100A6, S100A11 and ANXA1 are markedly overexpressed in PTC and can discriminate tumours of papillary and follicular histology

S100A6 and S100A11 were more abundant in PTCs compared to normal thyroid (log2fc = 1.39 and log2fc = 1.44, respectively), as previously reported [57,58]. ANXA1 is a putative S100A11 interaction partner [59] that we found to be highly overexpressed in PTC (log2fc = 2.25) and well correlated with S100A11 expression (r2: 0.81, Figure 3e). AUC values after ROC curve analysis demonstrated the high discriminatory power of each of these proteins to distinguish PTC from FA + FTC tissues in this cohort: S100A6 AUC = 0.99, S100A11 AUC = 0.99, ANXA1 AUC = 1.

FA and FTC show reduced levels of S100A10 and ANXA2

Significantly decreased abundance of S100A10 and its known binding partner ANXA2 [60] was shown for FA (log2fc = - 2.47) and FTC (log2fc = -1.84) when compared against normal thyroid samples. A similar result was obtained with reference to PTC (Figure 3f). The expression of ANXA2 and S100A10 was highly correlated in all samples (r2: 0.93, Figure 3f).

Other S100 protein isoforms

No significant expression differences were observed for S100A1, S100A2, S100A8, S100A9, S100A14 and S100A16 in FA, FTC and PTC specimens with respect to normal thyroid tissue, except for S100A2 and S100A8 in FA. S100A8 and S100A9 are known to form heterodimers and their coordinated expression was observed in all tissues examined (Additional file 1: Figure S3).

Results based on label-free SRM of S100 proteins

The analysis of S100 proteins by label-free SRM provided essentially the same results as those found by stable-isotope labelling (see Figure 4 and Additional file 1: Figure S4). The median CV was higher, 19.9%, which is in line with the results obtained in the analysis of cell lines in our previous work [45] and with other studies by label-free SRM using a spiked standard [61]. S100A1 was not detected in the TPC1 cell line used for SILAC spike-in quantitation and it was analysed using the label-free approach only. Figure 5 shows that label-free SRM analyses are also well correlated with Western blot results, as in the case of SRM with stable-isotope labelling (Figure 3b and d)

Figure 4.

Figure 4

Open in a new tab

Label-free analysis of S100 proteins is well correlated with labelling-based quantitation: a) Global comparison between label-based and label-free SRM data of S100 proteins in thyroid tissues (relative values against normal tissues); b) Comparison removing two upper extreme values.

Figure 5.

Figure 5

Open in a new tab

Comparison of label-free SRM and Western blot analysis of S100A4 and S100A13. (S100A4, r2 0.93; S100A13, r2 0.80).

Discussion

The S100 protein family represents a promising panel of biomarkers for cancer and other diseases. However, methods are lacking for the quantitative screening of multiple S100 protein isoforms in clinical specimens. Here, we have showed that targeted MS using SRM enables the specific and multiplexed quantitation of S100 proteins in a large-scale study with 37 tissues of thyroid origin. As our method provided relative quantitation between samples it was necessary to investigate which proteins in thyroid tissues could act as stable endogenous reference proteins, which in this case were Rab7a, cyclophilin A and PSMB2. To the best of our knowledge, this is the first study to identify these loading control proteins for thyroid cancer specimens. Of note, others have already detected dysregulation of β-actin and tubulin isoforms in FA, FTC and PTC [62], hence supporting our strategy. Additionally, Western blot corroborated the variation in expression levels of β-tubulin and Rab7a across different tissue samples (CV of 46% vs. 19%, respectively, Figure 3c).

The MS method harnesses the high accuracy and precision of SILAC-based MS quantitation and expands the number of targeted S100 protein isoforms through the use of label-free SRM. Although the quantitation with the SILAC spike-in achieved greater precision than the label-free experiments, both approaches identified the same significant changes in the tissue samples and were well correlated. Isotope-labelled peptide standards offer an advantage in that LC retention time and non-specific peptide interferences can be readily determined. Moreover, the SRM technique can readily be configured to measure protein concentration through the inclusion of quantified stable isotope peptide standards [63]. While we have determined the appropriate normalisation factors for relative quantitation of S100 proteins in thyroid samples, to extend this to other cancer types we recommend using the SILAC spike-in standard to establish these factors. The full accompaniment of S100 proteins can then be quantitated by label-free SRM of SDS-PAGE fractionated samples, which we have shown to be an effective approach to minimise sample matrix background [45].

Our experiments revealed the novel observation of increased S100A13 in PTC compared with FA, FTC and normal thyroid tissue, and this was supported by Western blot and previous studies of mRNA transcript levels. S100A13 gene silencing in lung cancer cells has been observed to decrease the invasive potential in vitro [64]. Moreover, S100A13 is known to participate in a multi-protein complex that facilitates the release of fibroblast growth factor 1 (FGF-1) [65]. Increased FGF-1 expression has been previously observed in differentiated thyroid cancer (DTC) [66]. Binding of secreted FGFs with heparan sulphate proteoglycans enables signalling through receptor tyrosine kinases to activate MAPK and PI3K/AKT pathways which contribute to tumour growth and angiogenesis [67]. Interestingly, S100A13 upregulation has recently been linked to resistance to the chemotherapeutic agents dacarbazine or temozolomide in melanoma patients [68]. Others have shown S100A13 to be an angiogenic marker [32]. Extrapolating these findings to thyroid cancer implicates S100A13 as a new oncogenic factor in PTC, and this could warrant evaluation of the effectiveness of inhibiting S100A13-driven release of FGF-1.

Overexpression of S100A6 in PTC has been observed previously [57], but more studies are needed to understand its functional significance. S100A11 has recently been shown to reduce the loss of contact inhibition, anchorage-independent growth and resistance to anoikis in PTC cells and enhance the activity of PTC-associated oncogenes such as BRAFV600E and TRK-T3 [58]. We have shown that S100A11 expression is consistent among normal and follicular histotypes, despite being elevated in PTC. The MS method demonstrated that S100A6, S100A11 and ANXA1 differentiate PTC from follicular tumours and that ANXA1 is highly correlated with S100A11 expression. While not directly analysed here, the utility of our findings could be explored for distinguishing the follicular variant of PTC.

FA and FTC cannot be readily distinguished by cytologic evaluation of FNA biopsies, which poses an important diagnostic issue. Our findings using the MS assay show the loss of S100A4 in follicular adenoma tissue compared with follicular thyroid carcinoma, so this difference in expression has diagnostic potential. A previous study did not report the decrease of S100A4 in FA [69]. Our result might be explained by considering that tumour tissue analysis by MS allows the inclusion of both cancer and stromal S100A4-positive cells, which are known to cooperate to drive tumour progression and metastasis [70]. Since S100A4 has well-established pro-migratory, invasive and angiogenic activities [71], it would be of interest to examine S100A4 expression in metastatic radioactive iodine-refractory DTC, where it could emerge as a possible therapeutic target. A proof of concept has already been demonstrated in a mouse model with anaplastic thyroid carcinoma, showing absence of metastasis in mice inoculated with S100A4-shRNA knockdown cells [72].

The reduced expression of S100A10 in FA and FTC was well correlated with the expression of its interaction partner ANXA2. The S100A10-ANXA2 complex anchors to the plasma membrane via the ANXA2 subunits and has an active role in the trafficking of ion channels [60]. A previous IHC study showed only low S100A10 immunoreactivity in PTC tissues while essentially all normal, FA and FTC samples were S100A10-negative [73]. Our results show clearly higher levels of S100A10-ANXA2 in normal tissues compared with FA and FTC. Whether or not loss of S100A10 in the tumour microenvironment exerts a functional role in follicular thyroid neoplasia is a subject of future investigations.

Conclusions

We have demonstrated the use of targeted mass spectrometry for the multiplexed and specific analysis of S100 protein isoforms in thyroid tumour specimens. This approach provides unambiguous structural evidence of S100 protein isoform expression thereby overcoming potential problems of antigen cross-reactivity that can interfere with affinity detection methods. This study led to the global characterisation of S100 protein expression in thyroid tumours and highlighted several S100 protein isoforms for potential diagnostic and therapeutic evaluation. S100A13 emerged as a novel candidate PTC biomarker. Our results indicate that S100A6, S100A11 and ANXA1 have utility to discriminate follicular and papillary thyroid tumours. The diagnostic and functional significance of S100A4 and S100A10 reduction in follicular tumours warrants further investigations.

Acknowledgements

J.M-A acknowledges Macquarie University for the award of an MQRes PhD scholarship and Northern Translational Cancer Research Unit for research scholar funding. M.P.M. acknowledges support from the Cancer Institute NSW and Northern Translational Cancer Research Unit. R.C-B was supported by National Health and Medical Research Council of Australia (1061411). We thank Dr. Dana Pascovici for assistance with statistical analysis. Aspects of this research were carried out at the Australian Proteome Analysis Facility supported by the Australian Government’s National Collaborative Research Infrastructure Scheme.

Abbreviations

DTC

Differentiated thyroid cancer

FA

Follicular adenoma

Fc

Fold change

FGF-1

Fibroblast growth factor-1

FTC

Follicular thyroid carcinoma

IHC

Immunohistochemistry

MS

Mass spectrometry

SRM

Selected reaction monitoring

PTC

Papillary thyroid carcinoma

Additional file

Additional file 1: Table S1. (1.2MB, docx)

Types of cancer where the altered expression of S100 proteins/genes has been observed. For more details, readers are encouraged to consult the reviews [1-5] and literature focused on each S100 protein/cancer. Table S2. List of precursors (Q1) and fragment ions (Q3) for detection of S100 peptides. CE: Collision energy, CEXP: Cell exit potential. Table S3. Targeted peptide sequences of candidate reference proteins in the region 14-32 kDa. Table S4. Targeted peptide sequences of candidate reference proteins in the region 32-100 kDa. Figure S1. Expression of S100 proteins S100A1, S100A14 and S100A16 in normal and tumour thyroid tissues as analysed by the MS assay. Normalised expression values (against reference proteins) were log-transformed and significant changes of S100 protein expression were identified by one-way anova followed by Tukey’s post hoc test. Results are expressed against the mean S100 protein expression in normal tissue samples; *p<0.05, **p<0.01, ***p<0.001. Figure S2. S100A13 mRNA expression in matched normal-tumour samples from GEO Series a) GSE3467 b) GSE33630 and c) GSE3678. Samples in d) GSE9115 are not matched. Groups were analysed by unpaired (GSE9115) or paired t test (matched samples); *p<0.05, **p<0.01, ***p<0.001. Figure S3. S100A8 and S100A9 expression showed good correlation in the normal and tumour tissues. The graph was plotted with log2 values of SRM-based normalised S100 protein expression. Figure S4. Relative expression of S100 proteins in thyroid tissues according to label-free SRM data Figure S4. (cont). Relative expression of S100 proteins in thyroid tissues according to label-free SRM data.

Footnotes

Competing interests

The authors declare that they have no competing interests.

Authors’ contributions

J.M-A designed, performed the experiments, analysed data and wrote the manuscript. R.C-B designed the experiments, interpreted data. M.P.M designed the experiments, interpreted data, supervised the experiments, and wrote the manuscript. All authors read and approved the final manuscript.

Contributor Information

Juan Martínez-Aguilar, Email: juan.martinez-aguilar@students.mq.edu.au.

Roderick Clifton-Bligh, Email: jclifton@med.usyd.edu.au.

Mark P Molloy, Email: mark.molloy@mq.edu.au.

References

  • 1.Salama I, Malone PS, Mihaimeed F, Jones JL. A review of the S100 proteins in cancer. Eur J Surg Oncol. 2008;34(4):357–64. doi: 10.1016/j.ejso.2007.04.009. [DOI] [PubMed] [Google Scholar]
  • 2.Chen H, Xu C, Jin Q, Liu Z. S100 protein family in human cancer. Am J Cancer Res. 2014;4(2):89–115. [PMC free article] [PubMed] [Google Scholar]
  • 3.Gross SR, Sin CG, Barraclough R, Rudland PS. Joining S100 proteins and migration: for better or for worse, in sickness and in health. Cell Mol Life Sci. 2014;71(9):1551–79. doi: 10.1007/s00018-013-1400-7. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 4.Marenholz I, Heizmann CW, Fritz G. S100 proteins in mouse and man: from evolution to function and pathology (including an update of the nomenclature) Biochem Biophys Res Commun. 2004;322(4):1111–22. doi: 10.1016/j.bbrc.2004.07.096. [DOI] [PubMed] [Google Scholar]
  • 5.Sedaghat F, Notopoulos A. S100 protein family and its application in clinical practice. Hippokratia. 2008;12(4):198–204. [PMC free article] [PubMed] [Google Scholar]
  • 6.Huang L, Xu Y, Cai G, Guan Z, Sheng W, Lu H, et al. S100A4 over-expression underlies lymph node metastasis and poor prognosis in colorectal cancer. World J of Gastroenterol. 2011;17(1):69–78. doi: 10.3748/wjg.v17.i1.69. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 7.Rudland PS, Platt-Higgins A, Renshaw C, West CR, Winstanley JH, Robertson L, et al. Prognostic significance of the metastasis-inducing protein S100A4 (p9Ka) in human breast cancer. Cancer Res. 2000;60(6):1595–603. [PubMed] [Google Scholar]
  • 8.Wang YY, Ye ZY, Zhao ZS, Tao HQ, Chu YQ. High-level expression of S100A4 correlates with lymph node metastasis and poor prognosis in patients with gastric cancer. Ann Surg Oncol. 2010;17(1):89–97. doi: 10.1245/s10434-009-0722-z. [DOI] [PubMed] [Google Scholar]
  • 9.Tsukamoto N, Egawa S, Akada M, Abe K, Saiki Y, Kaneko N, et al. The expression of S100A4 in human pancreatic cancer is associated with invasion. Pancreas. 2013;42(6):1027–33. doi: 10.1097/MPA.0b013e31828804e7. [DOI] [PubMed] [Google Scholar]
  • 10.Saleem M, Kweon MH, Johnson JJ, Adhami VM, Elcheva I, Khan N, et al. S100A4 accelerates tumorigenesis and invasion of human prostate cancer through the transcriptional regulation of matrix metalloproteinase 9. Proc Natl Acad Sci U S A. 2006;103(40):14825–30. doi: 10.1073/pnas.0606747103. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 11.Cross SS, Hamdy FC, Deloulme JC, Rehman I. Expression of S100 proteins in normal human tissues and common cancers using tissue microarrays: S100A6, S100A8, S100A9 and S100A11 are all overexpressed in common cancers. Histopathology. 2005;46(3):256–69. doi: 10.1111/j.1365-2559.2005.02097.x. [DOI] [PubMed] [Google Scholar]
  • 12.Komatsu K, Andoh A, Ishiguro S, Suzuki N, Hunai H, Kobune-Fujiwara Y, et al. Increased expression of S100A6 (Calcyclin), a calcium-binding protein of the S100 family, in human colorectal adenocarcinomas. Clin Cancer Res. 2000;6(1):172–7. [PubMed] [Google Scholar]
  • 13.Yang YQ, Zhang LJ, Dong H, Jiang CL, Zhu ZG, Wu JX, et al. Upregulated expression of S100A6 in human gastric cancer. J Dig Dis. 2007;8(4):186–93. doi: 10.1111/j.1751-2980.2007.00311.x. [DOI] [PubMed] [Google Scholar]
  • 14.Ohuchida K, Mizumoto K, Yu J, Yamaguchi H, Konomi H, Nagai E, et al. S100A6 is increased in a stepwise manner during pancreatic carcinogenesis: clinical value of expression analysis in 98 pancreatic juice samples. Cancer Epidemiol Biomarkers Prev. 2007;16(4):649–54. doi: 10.1158/1055-9965.EPI-06-0157. [DOI] [PubMed] [Google Scholar]
  • 15.Rehman I, Cross SS, Azzouzi AR, Catto JW, Deloulme JC, Larre S, et al. S100A6 (Calcyclin) is a prostate basal cell marker absent in prostate cancer and its precursors. Br J Cancer. 2004;91(4):739–44. doi: 10.1038/sj.bjc.6602034. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 16.Arai K, Takano S, Teratani T, Ito Y, Yamada T, Nozawa R. S100A8 and S100A9 overexpression is associated with poor pathological parameters in invasive ductal carcinoma of the breast. Curr Cancer Drug Targets. 2008;8(4):243–52. doi: 10.2174/156800908784533445. [DOI] [PubMed] [Google Scholar]
  • 17.Duan L, Wu R, Ye L, Wang H, Yang X, Zhang Y, et al. S100A8 and S100A9 are associated with colorectal carcinoma progression and contribute to colorectal carcinoma cell survival and migration via Wnt/beta-catenin pathway. PLoS One. 2013;8(4):e62092. doi: 10.1371/journal.pone.0062092. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 18.Wang L, Chang EW, Wong SC, Ong SM, Chong DQ, Ling KL. Increased myeloid-derived suppressor cells in gastric cancer correlate with cancer stage and plasma S100A8/A9 proinflammatory proteins. J Immunol. 2013;190(2):794–804. doi: 10.4049/jimmunol.1202088. [DOI] [PubMed] [Google Scholar]
  • 19.Shen J, Person MD, Zhu J, Abbruzzese JL, Li D. Protein expression profiles in pancreatic adenocarcinoma compared with normal pancreatic tissue and tissue affected by pancreatitis as detected by two-dimensional gel electrophoresis and mass spectrometry. Cancer Res. 2004;64(24):9018–26. doi: 10.1158/0008-5472.CAN-04-3262. [DOI] [PubMed] [Google Scholar]
  • 20.Hermani A, Hess J, De Servi B, Medunjanin S, Grobholz R, Trojan L, et al. Calcium-binding proteins S100A8 and S100A9 as novel diagnostic markers in human prostate cancer. Clin Cancer Res. 2005;11(14):5146–52. doi: 10.1158/1078-0432.CCR-05-0352. [DOI] [PubMed] [Google Scholar]
  • 21.Meding S, Balluff B, Elsner M, Schone C, Rauser S, Nitsche U, et al. Tissue-based proteomics reveals FXYD3, S100A11 and GSTM3 as novel markers for regional lymph node metastasis in colon cancer. J Pathol. 2012;228(4):459–70. doi: 10.1002/path.4021. [DOI] [PubMed] [Google Scholar]
  • 22.Liu XG, Wang XP, Li WF, Yang S, Zhou X, Li SJ, et al. Ca2 + -binding protein S100A11: a novel diagnostic marker for breast carcinoma. Oncol Rep. 2010;23(5):1301–8. doi: 10.3892/or_00000764. [DOI] [PubMed] [Google Scholar]
  • 23.Mori M, Shimada H, Gunji Y, Matsubara H, Hayashi H, Nimura Y, et al. S100A11 gene identified by in-house cDNA microarray as an accurate predictor of lymph node metastases of gastric cancer. Oncol Rep. 2004;11(6):1287–93. [PubMed] [Google Scholar]
  • 24.Ohuchida K, Mizumoto K, Ohhashi S, Yamaguchi H, Konomi H, Nagai E, et al. S100A11, a putative tumor suppressor gene, is overexpressed in pancreatic carcinogenesis. Clin Cancer Res. 2006;12(18):5417–22. doi: 10.1158/1078-0432.CCR-06-0222. [DOI] [PubMed] [Google Scholar]
  • 25.Rehman I, Azzouzi AR, Cross SS, Deloulme JC, Catto JW, Wylde N, et al. Dysregulated expression of S100A11 (calgizzarin) in prostate cancer and precursor lesions. Hum Pathol. 2004;35(11):1385–91. doi: 10.1016/j.humpath.2004.07.015. [DOI] [PubMed] [Google Scholar]
  • 26.Dong L, Wang F, Yin X, Chen L, Li G, Lin F, et al. Overexpression of S100P promotes colorectal cancer metastasis and decreases chemosensitivity to 5-FU in vitro. Mol Cell Biochem. 2014;389(1–2):257–64. doi: 10.1007/s11010-013-1947-5. [DOI] [PubMed] [Google Scholar]
  • 27.Maciejczyk A, Lacko A, Ekiert M, Jagoda E, Wysocka T, Matkowski R, et al. Elevated nuclear S100P expression is associated with poor survival in early breast cancer patients. Histol Histopathol. 2013;28(4):513–24. doi: 10.14670/HH-28.513. [DOI] [PubMed] [Google Scholar]
  • 28.Ge F, Wang C, Wang W, Wu B. S100P predicts prognosis and drug resistance in gastric cancer. Int J Biol Markers. 2013;28(4):5000034. doi: 10.5301/jbm.5000034. [DOI] [PubMed] [Google Scholar]
  • 29.Basu GD, Azorsa DO, Kiefer JA, Rojas AM, Tuzmen S, Barrett MT, et al. Functional evidence implicating S100P in prostate cancer progression. Int J Cancer. 2008;123(2):330–9. doi: 10.1002/ijc.23447. [DOI] [PubMed] [Google Scholar]
  • 30.Arumugam T, Simeone DM, Van Golen K, Logsdon CD. S100P promotes pancreatic cancer growth, survival, and invasion. Clin Cancer Res. 2005;11(15):5356–64. doi: 10.1158/1078-0432.CCR-05-0092. [DOI] [PubMed] [Google Scholar]
  • 31.Ribe A, McNutt NS. S100A6 protein expression is different in Spitz nevi and melanomas. Mod Pathol. 2003;16(5):505–11. doi: 10.1097/01.MP.0000071128.67149.FD. [DOI] [PubMed] [Google Scholar]
  • 32.Massi D, Landriscina M, Piscazzi A, Cosci E, Kirov A, Paglierani M, et al. S100A13 is a new angiogenic marker in human melanoma. Mod Pathol. 2010;23(6):804–13. doi: 10.1038/modpathol.2010.54. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 33.Hamberg AP, Korse CM, Bonfrer JM, de Gast GC. Serum S100B is suitable for prediction and monitoring of response to chemoimmunotherapy in metastatic malignant melanoma. Melanoma Res. 2003;13(1):45–9. doi: 10.1097/00008390-200302000-00008. [DOI] [PubMed] [Google Scholar]
  • 34.Bulk E, Sargin B, Krug U, Hascher A, Jun Y, Knop M, et al. S100A2 induces metastasis in non-small cell lung cancer. Clin Cancer Res. 2009;15(1):22–9. doi: 10.1158/1078-0432.CCR-08-0953. [DOI] [PubMed] [Google Scholar]
  • 35.Davies BR, O'Donnell M, Durkan GC, Rudland PS, Barraclough R, Neal DE, et al. Expression of S100A4 protein is associated with metastasis and reduced survival in human bladder cancer. J Pathol. 2002;196(3):292–9. doi: 10.1002/path.1051. [DOI] [PubMed] [Google Scholar]
  • 36.Zhang H, Zhao Q, Chen Y, Wang Y, Gao S, Mao Y, et al. Selective expression of S100A7 in lung squamous cell carcinomas and large cell carcinomas but not in adenocarcinomas and small cell carcinomas. Thorax. 2008;63(4):352–9. doi: 10.1136/thx.2007.087015. [DOI] [PubMed] [Google Scholar]
  • 37.Chen H, Ma J, Sunkel B, Luo A, Ding F, Li Y, et al. S100A14: novel modulator of terminal differentiation in esophageal cancer. Mol Cancer Res. 2013;11(12):1542–53. doi: 10.1158/1541-7786.MCR-13-0317. [DOI] [PubMed] [Google Scholar]
  • 38.Gongoll S, Peters G, Mengel M, Piso P, Klempnauer J, Kreipe H, et al. Prognostic significance of calcium-binding protein S100A4 in colorectal cancer. Gastroenterology. 2002;123(5):1478–84. doi: 10.1053/gast.2002.36606. [DOI] [PubMed] [Google Scholar]
  • 39.Sack U, Walther W, Scudiero D, Selby M, Kobelt D, Lemm M, et al. Novel effect of antihelminthic Niclosamide on S100A4-mediated metastatic progression in colon cancer. J Natl Cancer Inst. 2011;103(13):1018–36. doi: 10.1093/jnci/djr190. [DOI] [PubMed] [Google Scholar]
  • 40.Stein U, Arlt F, Smith J, Sack U, Herrmann P, Walther W, et al. Intervening in beta-catenin signaling by sulindac inhibits S100A4-dependent colon cancer metastasis. Neoplasia. 2011;13(2):131–44. doi: 10.1593/neo.101172. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 41.Wang XH, Zhang LH, Zhong XY, Xing XF, Liu YQ, Niu ZJ, et al. S100A6 overexpression is associated with poor prognosis and is epigenetically up-regulated in gastric cancer. Am J Pathol. 2010;177(2):586–97. doi: 10.2353/ajpath.2010.091217. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 42.Zhang J, Zhang K, Jiang X, Zhang J. S100A6 as a potential serum prognostic biomarker and therapeutic target in gastric cancer. Dig Dis Sci. 2014;59(9):2136–44. doi: 10.1007/s10620-014-3137-z. [DOI] [PubMed] [Google Scholar]
  • 43.Dakhel S, Padilla L, Adan J, Masa M, Martinez JM, Roque L, et al. S100P antibody-mediated therapy as a new promising strategy for the treatment of pancreatic cancer. Oncogenesis. 2014;3:e92. doi: 10.1038/oncsis.2014.7. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 44.Cancemi P, Di Cara G, Albanese NN, Costantini F, Marabeti MR, Musso R, et al. Large-scale proteomic identification of S100 proteins in breast cancer tissues. BMC Cancer. 2010;10:476. doi: 10.1186/1471-2407-10-476. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 45.Martínez-Aguilar J, Molloy MP. Label-free Selected Reaction Monitoring enables multiplexed quantitation of S100 protein isoforms in cancer cells. J Proteome Res. 2013;12(8):3679–88. doi: 10.1021/pr400251t. [DOI] [PubMed] [Google Scholar]
  • 46.Cooper DS, Doherty GM, Haugen BR, Kloos RT, Lee SL, Mandel SJ, et al. Revised American Thyroid Association management guidelines for patients with thyroid nodules and differentiated thyroid cancer. Thyroid. 2009;19(11):1167–214. doi: 10.1089/thy.2009.0110. [DOI] [PubMed] [Google Scholar]
  • 47.Baloch ZW, Cibas ES, Clark DP, Layfield LJ, Ljung BM, Pitman MB, et al. The National Cancer Institute Thyroid fine needle aspiration state of the science conference: a summation. Cytojournal. 2008;5(6):1742–6413. doi: 10.1186/1742-6413-5-6. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 48.Abbatiello SE, Mani DR, Keshishian H, Carr SA. Automated detection of inaccurate and imprecise transitions in peptide quantification by multiple reaction monitoring mass spectrometry. Clin Chem. 2010;56(2):291–305. doi: 10.1373/clinchem.2009.138420. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 49.Vandesompele J, De Preter K, Pattyn F, Poppe B, Van Roy N, De Paepe A, et al. Accurate normalization of real-time quantitative RT-PCR data by geometric averaging of multiple internal control genes. Genome Biol. 2002;3(7):18. doi: 10.1186/gb-2002-3-7-research0034. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 50.Eisenberg E, Levanon EY. Human housekeeping genes, revisited. Trends Genet. 2013;29(10):569–74. doi: 10.1016/j.tig.2013.05.010. [DOI] [PubMed] [Google Scholar]
  • 51.de Jonge HJ, Fehrmann RS, de Bont ES, Hofstra RM, Gerbens F, Kamps WA, et al. Evidence based selection of housekeeping genes. PLoS One. 2007;2(9):e898. doi: 10.1371/journal.pone.0000898. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 52.Shcherbik N, Pestov DG. Ubiquitin and ubiquitin-like proteins in the nucleolus: multitasking tools for a ribosome factory. Genes Cancer. 2010;1(7):681–9. doi: 10.1177/1947601910381382. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 53.Voges D, Zwickl P, Baumeister W. The 26S proteasome: a molecular machine designed for controlled proteolysis. Annu Rev Biochem. 1999;68:1015–68. doi: 10.1146/annurev.biochem.68.1.1015. [DOI] [PubMed] [Google Scholar]
  • 54.Stavreva DA, Kawasaki M, Dundr M, Koberna K, Muller WG, Tsujimura-Takahashi T, et al. Potential roles for ubiquitin and the proteasome during ribosome biogenesis. Mol Cell Biol. 2006;26(13):5131–45. doi: 10.1128/MCB.02227-05. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 55.Dai RM, Li CC. Valosin-containing protein is a multi-ubiquitin chain-targeting factor required in ubiquitin-proteasome degradation. Nat Cell Biol. 2001;3(8):740–4. doi: 10.1038/35087056. [DOI] [PubMed] [Google Scholar]
  • 56.Lange V, Picotti P, Domon B, Aebersold R. Selected reaction monitoring for quantitative proteomics: a tutorial. Mol Syst Biol. 2008;4:222. doi: 10.1038/msb.2008.61. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 57.Sofiadis A, Dinets A, Orre LM, Branca RM, Juhlin CC, Foukakis T, et al. Proteomic study of thyroid tumors reveals frequent up-regulation of the Ca2+ -binding protein S100A6 in papillary thyroid carcinoma. Thyroid. 2010;20(10):1067–76. doi: 10.1089/thy.2009.0400. [DOI] [PubMed] [Google Scholar]
  • 58.Anania MC, Miranda C, Vizioli MG, Mazzoni M, Cleris L, Pagliardini S, et al. S100A11 overexpression contributes to the malignant phenotype of papillary thyroid carcinoma. J Clin Endocrinol Metab. 2013;98(10):2013–1652. doi: 10.1210/jc.2013-1652. [DOI] [PubMed] [Google Scholar]
  • 59.Seemann J, Weber K, Gerke V. Structural requirements for annexin I-S100C complex-formation. Biochem J. 1996;319(Pt 1):123–9. doi: 10.1042/bj3190123. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 60.Rescher U, Gerke V. S100A10/p11: family, friends and functions. Pflugers Arch. 2008;455(4):575–82. doi: 10.1007/s00424-007-0313-4. [DOI] [PubMed] [Google Scholar]
  • 61.Zhang H, Liu Q, Zimmerman LJ, Ham AJ, Slebos RJ, Rahman J, et al. Methods for peptide and protein quantitation by liquid chromatography-multiple reaction monitoring mass spectrometry. Mol Cell Proteomics. 2011;10(6):27. doi: 10.1074/mcp.M110.006593. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 62.Sofiadis A, Becker S, Hellman U, Hultin-Rosenberg L, Dinets A, Hulchiy M, et al. Proteomic profiling of follicular and papillary thyroid tumors. Eur J Endocrinol. 2012;166(4):657–67. doi: 10.1530/EJE-11-0856. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 63.Gerber SA, Rush J, Stemman O, Kirschner MW, Gygi SP. Absolute quantification of proteins and phosphoproteins from cell lysates by tandem MS. Proc Nat Acad Sci. 2003;100(12):6940–5. doi: 10.1073/pnas.0832254100. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 64.Pierce A, Barron N, Linehan R, Ryan E, O'Driscoll L, Daly C, et al. Identification of a novel, functional role for S100A13 in invasive lung cancer cell lines. Eur J Cancer. 2008;44(1):151–9. doi: 10.1016/j.ejca.2007.10.017. [DOI] [PubMed] [Google Scholar]
  • 65.Prudovsky I, Mandinova A, Soldi R, Bagala C, Graziani I, Landriscina M, et al. The non-classical export routes: FGF1 and IL-1alpha point the way. J Cell Sci. 2003;116(Pt 24):4871–81. doi: 10.1242/jcs.00872. [DOI] [PubMed] [Google Scholar]
  • 66.Eggo MC, Hopkins JM, Franklyn JA, Johnson GD, Sanders DS, Sheppard MC. Expression of fibroblast growth factors in thyroid cancer. J Clin Endocrinol Metab. 1995;80(3):1006–11. doi: 10.1210/jcem.80.3.7533768. [DOI] [PubMed] [Google Scholar]
  • 67.Brooks AN, Kilgour E, Smith PD. Molecular pathways: fibroblast growth factor signaling: a new therapeutic opportunity in cancer. Clin Cancer Res. 2012;18(7):1855–62. doi: 10.1158/1078-0432.CCR-11-0699. [DOI] [PubMed] [Google Scholar]
  • 68.Azimi A, Pernemalm M, Frostvik Stolt M, Hansson J, Lehtio J, Egyhazi Brage S, et al. Proteomics analysis of melanoma metastases: association between S100A13 expression and chemotherapy resistance. Br J Cancer. 2014;110(10):2489–95. doi: 10.1038/bjc.2014.169. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 69.Ito Y, Yoshida H, Tomoda C, Uruno T, Miya A, Kobayashi K, et al. S100A4 expression is an early event of papillary carcinoma of the thyroid. Oncology. 2004;67(5–6):397–402. doi: 10.1159/000082924. [DOI] [PubMed] [Google Scholar]
  • 70.Schmidt-Hansen B, Klingelhofer J, Grum-Schwensen B, Christensen A, Andresen S, Kruse C, et al. Functional significance of metastasis-inducing S100A4(Mts1) in tumor-stroma interplay. J Biol Chem. 2004;279(23):24498–504. doi: 10.1074/jbc.M400441200. [DOI] [PubMed] [Google Scholar]
  • 71.Mishra SK, Siddique HR, Saleem M. S100A4 calcium-binding protein is key player in tumor progression and metastasis: preclinical and clinical evidence. Cancer Metastasis Rev. 2012;31(1–2):163–72. doi: 10.1007/s10555-011-9338-4. [DOI] [PubMed] [Google Scholar]
  • 72.Shi Y, Zou M, Collison K, Baitei EY, Al-Makhalafi Z, Farid NR, et al. Ribonucleic acid interference targeting S100A4 (Mts1) suppresses tumor growth and metastasis of anaplastic thyroid carcinoma in a mouse model. J Clin Endocrinol Metab. 2006;91(6):2373–9. doi: 10.1210/jc.2006-0155. [DOI] [PubMed] [Google Scholar]
  • 73.Ito Y, Arai K, Nozawa R, Yoshida H, Higashiyama T, Takamura Y, et al. S100A10 expression in thyroid neoplasms originating from the follicular epithelium: contribution to the aggressive characteristic of anaplastic carcinoma. Anticancer Res. 2007;27(4C):2679–83. [PubMed] [Google Scholar]

Articles from BMC Cancer are provided here courtesy of BMC

RESOURCES