Oxidative damage and response to Bacillus Calmette-Guérin in bladder cancer cells expressing sialyltransferase ST3GAL1

Background

Treatment with Bacillus Calmette-Guérin (BCG) is the gold standard adjuvant immunotherapy of non-muscle invasive bladder cancer (NMIBC), although it fails in one third of the patients. NMIBC expresses two tumor-associated O-linked carbohydrates: the disaccharide (Galβ1,3GalNAc) Thomsen-Friedenreich (T) antigen, and its sialylated counterpart (Siaα2,3Galβ1,3GalNAc) sialyl-T (sT), synthesized by sialyltransferase ST3GAL1, whose roles in BCG response are unknown.

Methods

The human bladder cancer (BC) cell line HT1376 strongly expressing the T antigen, was retrovirally transduced with the ST3GAL1 cDNA or with an empty vector, yielding the cell lines HT1376_sT and HT1376_T, that express, respectively, either the sT or the T antigens. Cells were in vitro challenged with BCG. Whole gene expression was studied by microarray technology, cytokine secretion was measured by multiplex immune-beads assay. Human macrophages derived from blood monocytes were challenged with the secretome of BCG-challenged BC cells.

Results

The secretome from BCG-challenged HT1376_sT cells induced a stronger macrophage secretion of IL-6, IL-1β, TNFα and IL-10 than that of HT1376_T cells. Transcriptomic analysis revealed that ST3GAL1 overexpression and T/sT replacement modulated hundreds of genes. Several genes preserving genomic stability were down-regulated in HT1376_sT cells which, as a consequence, displayed increased sensitivity to oxidative damage. After BCG challenge, the transcriptome of HT1376_sT cells showed higher susceptibility to BCG modulation than that of HT1376_T cells.

Conclusions

High ST3GAL1 expression and T/sT replacement in BCG challenged-BC cancer cells induce a stronger macrophage response and alter the gene expression towards genomic instability, indicating a potential impact on BC biology and patient’s response to BCG.

The intravesical inoculation with the Bacillus Calmette-Guérin (BCG) is the most effective adjuvant therapy of non-muscle invasive bladder cancers (NMIBC) after transurethral resection. However, one third of the patients fail to respond and experience recurrence after treatment. The reasons why BCG therapy fail are still unclear, although it is well established that the anti-tumor activity of BCG depends on its ability to elicit an effective local immune response [1,2,3].

Glycosylation, one of the most frequent post-translational modification of proteins, undergoes profound changes in all types of cancer [4], including bladder cancer (BC) [5,6,7,8]. The aberrant expression of glycoconjugates is often caused by the deranged regulation of their biosynthetic enzymes: the glycosyltransferases [9]. The Thomsen-Friedenreich (T) antigen is a disaccharide (Galβ1,3GalNAc) O-linked to serine or threonine residues of glycoproteins (Additional file 1A), whose aberrant expression in cancer has been associated with malignancy [10,11,12,13] and used as a possible target for therapy [14,15,16]. Its sialylated counterpart, the sialyl-T (sT) (Siaα2,3Galβ1,3GalNAc-O-Ser/Thr) structure and its main biosynthetic enzyme, the sialyltransferase ST3GAL1, are also aberrantly expressed in a variety of cancers [17, 18] [reviewed in [19, 20]]. In BC, the expression of T/sT antigens is also aberrant and it influences invasion and immune recognition [21,22,23]. In a previous work [24], we have shown that the mRNA of ST3GAL1 was overexpressed in NMIBC but not in muscle invasive BC or in benign bladder tumors and ST3GAL1 plays the major role in the sialylation of the T antigen in BC. The T antigen has been suggested as a useful marker of BCG response [23], even though the relationship between ST3GAL1/sT and BCG response has never been established.

In this study, we investigated the effects of the alternative expression of the T or sT antigens on the ability of BC cells to activate macrophages in response to BCG challenge and on the transcriptome of BC cells, utilizing the HT1376 cell line in which the T antigen was replaced by the sT antigen, by retroviral transduction with the ST3GAL1 cDNA. This cell line was chosen because of its low ST3GAL1 expression and its high and homogenous reactivity with the T antigen-specific lectin PNA [24]. The gene expression and cytokine profiles of the cell lines expressing either the T or the sT antigens after BCG challenge and the ability of their secretome to stimulate cytokine release by macrophages was studied.

Generation of ST3GAL1-expressing cell lines

The HT1376 cell line was established from a primary invasive transitional cell cancer of the bladder [25]. Cells were grown in DMEM (4.5 g/L glucose, Sigma), containing 10% foetal calf serum (FCS, Sigma), 2 mM L-glutamine (Sigma) and 100 μg/mL penicillin/streptomycin (Sigma). HT1376 cells expressing ST3GAL1 were generated by transduction with a retroviral vector obtained with the ViraPower Lentiviral Expression System (Invitrogen), according to manufacturer’s instructions. The cDNA of the whole coding region of human ST3GAL1 was obtained by PCR amplification of the cDNA of the colon cancer cell line HT29 with the following primer pair: forward primer: 5’-CACCATGGTGACCCTGCGGAAGAGG-3′; reverse primer: 5’-TCATCTCCCCTTGAAGATCCGG-3′. Amplification was performed for 35 cycles of the following program: denaturation 94 °C 1 min; annealing 60 °C 1 min; extension 72 °C 1 min. The PCR product was gel isolated and cloned into the pLenti6/V5 Directional TOPO cloning vector (Invitrogen) which drives the expression of inserted genes under the control of the cytomegalovirus promoter. A negative control retroviral vector was prepared with an empty plasmid. After transduction with negative control- or ST3GAL1-expressing vectors, HT1376 cells were selected with 4 μg/mL of blasticidin. The replacement of the T antigen with the sT antigen was evaluated as loss of cell reactivity with the fluorescent labeled lectin from Arachis hypogea (peanut agglutinin, PNA), conjugated with fluorescein isothiocyanate (PNA-FITC). Although selected cells were mainly negative to PNA-FITC as detected by FACS analysis, a small population of PNA-FITC positive cells was still present. To obtain a population of cells homogeneously negative for the T antigen, about 100 ST3GAL1-transduced HT1376 cells were seeded in a 10 cm Petri dish and after one month, PNA-FITC negative colonies were selected and pooled. This polyclonal cell population homogeneously negative for T antigen expression is thereafter referred to as HT1376_sT. The polyclonal cell population obtained after transduction with the negative control retroviral vector followed by blasticidin selection is referred to as HT1376_T.

Flow cytometry

Cells were incubated with PNA-FITC for 30 min at 4 °C in the dark, washed and analyzed by flow cytometry. Sialidase treatment was performed with 20 mU of Clostridium perfringens sialidase (Roche Diagnostics), for 90 min at 37 °C.

Real time RT-PCR

Total RNA was isolated using the GenElute Mammalian Total RNA Purification kit and DNase treatment (Sigma), according to the manufacturer’s instructions. One microgram of total RNA was reverse transcribed, using the random-primers based High Capacity cDNA Archive Kit (Applied Biosystems). The expression level of ST3GAL1 (Hs00161688_m1; NM_173344.2 and NM_003033.3) was evaluated with the TaqMan assay system in a 7500 Fast Real-Time PCR System (Applied Biosystems) using the TaqMan Universal PCR Master Mix Fast, as previously described [24, 26, 27]. The efficiency of the amplification reaction for each primer-probe was above 95% (as determined by the manufacturer). Normalized mRNA expression was computed as the number of mRNA molecules of the gene of interest per 1000 mRNA molecules of the endogenous control β-actin gene, calculated using the 2^-ΔCT×1000 formula [28].

Sialyltransferase activity assay

Cell pellets were homogenized in water and the protein concentration of the homogenates was determined by the Lowry method. The activity of ST3GAL1 was measured in the homogenates in the range of time and substrate concentration linearity in a 25 μL volume containing: 50 mM of 2-(N-morpholino)ethanesulphonic acid (MES) buffer pH 6.5, 0.5% Triton X-100, 23.5 μg of Galβ1,3GalNAcα1-O-benzyl (benzyl-T; Sigma) as acceptor substrate, 15 μM (640 Bq) of CMP-[¹⁴C]Sia (Amersham) and 50 μg of homogenate proteins. Reactions were incubated at 37 °C, for 2 h and the products were then isolated by hydrophobic chromatography in SepPak C18 Classic Cartridge (Waters). The columns were washed with water and eluted with 1 mL acetonitrile, which was counted in a liquid scintillation counter. The incorporation on endogenous substrates, in the absence of the acceptor substrate, was subtracted.

BCG challenge of HT1376 cells

Commercial Connaught BCG (ImmuCyst, Sanofi Pasteur SA, France) was suspended in PBS containing 0.05% Tween 80 and stored at − 80 °C. Before each assay, BCG aggregates were discarded by centrifugation (300 × g for 5 min). To assess BCG internalization, bacteria were stained with 2 μg/mL of 5-(and-6-)(((4-chloromethyl)benzoyl)amino)tetramethylrhodamine (CMTR, Invitrogen) for 2 h in culture medium, incubated with HT1376_T or HT1376_sT cells in a 1:10 cell/bacteria ratio for 2 h at 37 °C and analyzed by flow cytometry. To assess cytokine secretion, HT1376_T or HT1376_sT cells were challenged with unstained BCG for 2 h at 37 °C, the medium was removed and the cells were washed twice with PBS and incubated with fresh medium for 16 h. Conditioned media were used for cytokine analysis and to challenge macrophages, while cell pellets were used for RNA extraction and transcriptomic analysis.

Determination of cytokine concentration

The concentration of cytokines IL-1β, IL-2, IL-4, IL-6, IL-8, IL-10, IL-12, IL-17, IFN-γ and TNF-α was measured in a 96-well strip plate from a commercial MIBA kit (Bio-Rad), as recommended by manufacturer’s instructions. Fluorescence was read in a Luminex 100 Bio-Plex Liquid Array Multiplexing System reader (Bio-Rad) and the data analyzed with the Bio-Plex Manager v5 software (Bio-Rad).

Macrophage preparation and stimulation

Mononuclear cells were isolated by Ficoll-Hypaque density gradient centrifugation (GE Healthcare) from the peripheral blood of healthy blood-donors. For this use, no study approval was necessary. The only authorization required was that obtained from the Blood Collection Service of the Pizzardi Hospital in Bologna, Italy, which keeps the rights on donors’ blood samples. Macrophages were obtained by differentiation of monocytes by culture in RPMI 1640 (Sigma) medium supplemented with 20% FCS, 2 mM L-glutamine and 100 μg/mL penicillin/streptomycin. After 7 days, monocyte-derived macrophages were detached with a cell scraper and dispensed in 24 well plates at a cell density corresponding approximately to 50% of confluence. One day later, macrophages were incubated with standard unconditioned culture medium or with the media conditioned by HT1376_T or HT1376_sT cells either BCG-challenged (as described above) or mock challenged. After 2 h, the conditioned media were replaced by fresh medium, which was collected 24 h later and stored at − 80 °C for the detection of cytokines secreted by macrophages.

H₂O₂ treatment

Cells in exponential growth phase were incubated in serum-free medium containing 5 mM H₂O₂ for 1 h. The medium was then replaced with fresh complete medium and the cells were harvested and analyzed 24 h later. Mock-treated cells were incubated as above without H₂O₂. The cytotoxic effect of H₂O₂ was determined by counting the number of cells in six replicas seeded in 6-wells plates. Representative fields were photographed with an inverted phase contrast microscope.

Whole transcriptome analysis by expression microarray

Total RNA was isolated by the guanidinium thiocyanate-method [29] and converted to labelled single strand cDNA (ssDNA) by the commercial Whole Transcript Expression kit (Ambion), according to the manufacturer’s instructions. Labelled ssDNA fragments were hybridized in a Human Transcriptome Array 2.0 overnight. After staining with phycoerythrin-streptavidin, fluorescence was read in a GeneChip Scanner 3000 7G (Affymetrix). After statistical analysis (see below), array data were functionally analyzed by the ArrayStar v2.0 software (DNASTAR) and through a literature search of the biological roles of modulated genes. Gene nomenclature followed the HUGO Gene Nomenclature Committee rules (https://www.genenames.org/) in italic uppercase letters. With exception of cytokines, proteins had the same name as the gene, represented in regular uppercase.

Statistical methods

Microarray raw data were background-subtracted, normalized and summarized with the robust multi-array average (RMA) algorithm implemented in the Affy package of Bioconductor (www.bioconductor.org), which utilizes R software. Differentially expressed genes between query and control assay were selected by application of the two tail ANOVA, followed by the Benjamini-Hochberg false discovery rate test with a p or q ≤ 0.05 cut-off and by the log₂ expression ratio, considering only variations ≥0.5. MIBA data were analyzed by ANOVA, followed by Tukey multiple comparison test. H₂O₂ toxicity data were analyzed by the Student’s t test. The software used was Graphpad Prism, version 7.0.

ST3GAL1-expression leads to replacement of T with sT antigen in HT1376 cells

The mock-transduced cell line HT1376_T, like the wild type HT1376, expressed high and homogeneous T expression, while the ST3GAL1-transduced cell line HT1376_sT displayed an homogeneous low PNA reactivity which could be reverted to high reactivity after sialidase treatment (Additional file 1B). Both the ST3GAL1 activity (Additional file 1C) and the ST3GAL1 mRNA measured by real time PCR (Additional file 1D) were very high in HT1376_sT although almost undetectable in HT1376_T. The level of ST3GAL1 activity and PNA reactivity reached by HT1376_sT cells was similar to that displayed by the wild type BC cell line 5637 strongly expressing ST3GAL1 (data not shown [24]). This is consistent with the notion that, in BC cells, ST3GAL1-mediated α2,3 sialylation of galactose (Additional file 1A) masks the T antigen [24].

IL-6 and IL-8 secretion by HT1376_T and HT1376_sT cells

To assess the effect of ST3GAL1 overexpression and the consequent replacement of the T with the sT antigen on cytokine production following BCG stimulation, we challenged the two HT1376 cell lines with BCG. Among the several cytokines tested (IL-1β, IL-2, IL-4, IL-6, IL-8, IL-10, IL-12, IL-17, IFN-γ and TNF-α), only IL-8 was detectable in media conditioned by unchallenged HT1376_T or HT1376_sT cells. After BCG challenge, IL-6 became detectable in both HT1376_sT and HT1376_T cells, while the IL-8 secretion showed a clear tendency to up-regulation after BCG challenge, especially in HT1376_T cells (Fig. 1a). The p values are reported in Additional file 2.

BCG-stimulation of HT1376 cells. a: Secretion of IL-6 and IL-8. HT1376_T, (white circles) and HT1376_sT (black circles) cells were challenged with BCG for 2 h, then they were washed and cultured in medium for 16 h. Cytokine concentration was determined as described in Materials and Methods section. Data of three independent experiments are reported. Statistical analysis is reported in Additional file 2. b: Time course of BCG uptake. HT1376T (white circles) and HT1376sT (black circles) cells were challenged with CMTMR-labelled BCG for 2 and 6 h, as described in the Methods section. BCG internalization was estimated as mean fluorescence intensity of the cells, measured by flow cytometry Data of three independent experiments are reported

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To establish whether the different IL-8 production by HT1376_sT after BCG challenge was due to a higher BCG uptake by these cells, we measured BCG internalization by the two HT1376 cell populations by flow cytometry. As shown in Fig. 1b, there were no significant differences in the uptake of fluorescent BCG by HT1376_T and HT1376_sT cells, ruling out the possibility that differences in cytokine production by BCG-stimulated HT1376_T and HT1376_sT was dependent on different BCG internalization rate.

HT1376_sT cells induce a stronger macrophage secretory response after BCG stimuli

To investigate the role played by ST3GAL1 expression and the consequent T/sT replacement on the stimulation of innate immunity by BCG-challenged BC cells, the secretion of cytokines by human macrophages stimulated with the secretome of BCG-challenged BC cells was measured. Unstimulated macrophages secreted high levels of IL-8 and very low levels of TNF-α, IL-6, IL-1β and IL-10. This pattern of secretion was not significantly changed by stimulation with the secretome of BCG-unchallenged HT1376_T or HT1376_sT cells (Fig. 2). In contrast, the secretome from both BCG-challenged cell lines, in particular that from HT1376_sT, significantly increased the secretion of IL-6, IL-1β, TNF-α and IL-10 whereas IL-8 secretion was hardly affected by the secretome of BCG-challenged cells, regardless of their ST3GAL1 expression (Fig. 2). It should be noted that the level of secretion of IL-8 and IL-6 by macrophages was about 10 and 3-fold higher, respectively, than the level of either in HT1376 cells (Fig. 1), ruling out the possibility of a significant contamination of cytokines secreted by macrophages with those secreted by HT1376 cells. The cytokines IL-2, IL-4, IL-12 and IL-17 were not secreted by macrophages in any of the tested conditions (data not shown). The p and q values are reported in Additional file 2.

Cytokine secretion by human macrophages treated with conditioned media of BC cell lines. Cytokine secretion was measured in culture media conditioned by unstimulated macrophages (MΦ, grey circles) or stimulated with conditioned media from BCG-challenged or unchallenged BC cell lines: HT1376_T, (white circles); HT1376_sT (black circles). Cells were challenged with BCG for 2 h, then they were washed and allowed to condition the culture medium for 16 h. The conditioned culture media of BCG-challenged or unchallenged cells was used to stimulate human monocyte-derived macrophages for 24 h. MØ: cytokines released by unstimulated macrophages; MØ + unchallenged: cytokines released by macrophages stimulated with the conditioned medium of unchallenged HT1376 cells; MØ + BCG-challenged: cytokines released from macrophages stimulated with the conditioned medium of BCG-challenged cells. Data of three independent experiments are reported. Statistical analysis is reported in Additional file 2

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HT1376_sT cells display down-regulation of genes preserving genomic stability

The impact of ST3GAL1 overexpression and of T replacement by sT on the global transcriptional activity of HT1376 cells was evaluated by expression microarray technology. Of the 254 genes, which displayed ST3GAL1-dependent modulation by at least a log₂ expression ratio ≥ 1.0 (meaning a fold change of at least 2) with p or q values ≤0.05, 106 were up-regulated and 148 were down-regulated. The complete list of genes showing significant modulation (changes equal or higher than 2-fold) in HT1376_sT vs. HT1376_T is reported in Additional file 3. At least 29 genes putatively regulating malignancy because of their involvement in the control of apoptosis, cell growth, angiogenesis, inflammation or proteolysis, were differentially expressed in HT1376_sT cells, compared with HT1376_T cells (Additional file 4). A search in the literature revealed that 18 genes were modulated towards increased malignancy and 14 towards decreased malignancy (Additional file 4). Remarkably, among the 18 genes modulated towards increased malignancy in HT1376_sT cells, 11 down-regulated genes can be collectively referred to as “caretaker genes” because of their involvement in DNA repair and mitotic fidelity (Additional file 4). Moreover, if threshold was lowered to include genes down-regulated above 1.3-fold, the number of down-regulated caretaker genes rose to 34 (Table 1). As a functional validation of gene expression data, cells were exposed to the genotoxic effects of the oxidizing agent H₂O₂. As expected for a cell line with impaired DNA repair mechanisms, H₂O₂ -treatment resulted in a reduced viability in HT1376_sT than in HT1376_T cells (Fig. 3a and b).

Cytotoxic effect of H₂O₂ on HT1376_T and HT1376_sT cells. a: cells were treated with 5 mM H₂O₂ or mock-treated as described in Methods and counted. Data of six experiments are reported. The HT1376_sT cells are more susceptible to the toxic effect of H₂O₂ (**p = 0.005 according to Student’s t test). b: phase contrast micrograph of representative fields of the two cell populations treated as described above, showing the stronger cytotoxic effects of H₂O₂ on HT1376_sT. Scale bar: 100 μm

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HT1376_sT cells display increased transcriptomic changes after BCG challenging

To investigate the effect of a differential T/sT expression on BCG challenging, the global transcriptional activity was also compared in BCG-challenged HT1376_T and HT1376_sT cell lines. While in HT1376_sT cells a group of 38 genes showed significant modulation by BCG (p and q values ≤0.05) with a log₂ expression ratio ≥ 0.5 (fold change at least 1.4) (Additional information 5), the tendency to modulation showed by a few genes in HT1376_T cells never reached statistical significance (data not shown). Modulated genes in HT1376_sT cells fell into several broad functional categories (Additional information 5). In particular, a set of genes related to “aminoacid and protein biosynthesis” were prevalently down-regulated in BCG-challenged HT1376_sT cells (Additional file 5). This functional category includes genes involved in the biosynthesis and transport of aminoacids, attachment of aminoacids to tRNAs and regulation of translation. Other categories of modulated genes include “cell growth” and “inflammatory and immune response” (Additional file 5).

The overexpression of ST3GAL1 has been widely studied in cellular models of breast cancer and found to be responsible for increased malignancy [30,31,32]. In contrast, very little is known on the role of this enzyme in BC biology. In this work, we have performed an exhaustive analysis of a BC experimental system in which through the overexpression of ST3GAL1, the constitutively expressed T antigen was replaced by its sialylated counterpart, the sT carbohydrate structure. Both structures are biologically active, being receptors either for galectins or siglecs, as well as for sugar binding receptors of microorganisms [33]. Thus, the phenotypic changes we report after ST3GAL1 overexpression could be attributable either to the lack of T antigen or expression of sT or both. The modulation of the immune response, in particular, the secretion of cytokines, is a well known functional consequence of BCG interaction with BC cells [1, 34, 35]. Our study confirms that BCG induces IL-6 and IL-8 secretion by BC cells and shows a tendency to higher IL-8 secretion by BCG-stimulated cells expressing sT. In BC patients, plasma [36] and tissue [37] IL-6 levels are elevated and associated with tumor progression and poor prognosis. Previous studies have indicated that BCG stimulates IL-6 production in urine of patients and BC cell lines [38], inducing non apoptotic cell death [39]. Increased urinary IL-8 level also correlates with progression in BC patients [40], although a high urinary IL-8 level after BCG instillation is a prognostic factor of successful outcome [41, 42]. Our data indicate that after BCG challenge, only the secretion of IL-6 and, to a lesser extent, IL-8 were stimulated while the other cytokines remained undetectable. This is consistent with clinical observations reporting that a few cytokines, including IL-6 and IL-8, were detectable in urine after a first intravesical BCG administration, while other cytokines required multiple BCG instillations [43].

After BCG challenge, the secretome of BC cells expressing the sT structure showed higher capacity to stimulate cytokine secretion by macrophages, further supporting the notion that the sT antigen potentiates the BC response to BCG.

An inflammatory environment can either promote or inhibit tumor progression, consistent with the notion that inflammation is a double edge sword which can both eradicate the tumor but also fuel its growth. Macrophages are differentiated either as pro-inflammatory M1 or anti-inflammatory M2 phenotypes, even if in many cases they are in an intermediate condition. While a variable capacity to secrete IL-6, IL-1β and TNF-α is shared by differentially polarized macrophages, an IL-12 low/IL-10 high phenotype is the hallmark of M2 macrophages [44], which are known to promote tumor growth [45]. The macrophages used in this study secreted IL-6, IL-8, IL-1β and TNF-α but no IL-12 and little IL-10 and are probably representative of an intermediate condition between the two extreme phenotypes. The nature of the macrophages associated with BC is indeed variable as indicated by the different level of expression of the M2-specific marker CD163 among patients [46]. Interestingly, the predominance of M2 macrophages is associated with higher stage and grade [46] and with a worse response to BCG [47].

The most prominent transcriptomic change we observed because of ST3GAL1 expression and the consequent replacement of the T with the sT antigen in HT1376 cells was the decreased expression of several genes involved in different mechanisms of DNA repair and in the accuracy of chromosomal segregation. This resulted in increased sensitivity of HT1376_sT cells to the cytotoxic effect of H₂O_2. This is of interest if one considers that the generation of reactive oxygen species by BCG is a crucial mechanism of BCG-induced damage to BC cells [48]. Interestingly, also in glioma cells, ST3GAL1 expression resulted in transcriptomic changes affecting malignancy and the cell cycle [49], supporting the notion that a carbohydrate structure on the cell surface can generate an “outside in” flow of information modulating gene expression [20].

BCG challenge resulted in a deeper modulation of the transcriptome in HT1376_sT than in HT1376T, suggesting that the replacement of the T with the sT antigen on the cell surface changes the development of the genetic program triggered by BCG contact.

Even though genes involved in inflammatory and immune response were found to be modulated by BCG challenge in HT1376sT cells, little or no changes were observed in genes encoding cytokines, including those whose expression was stimulated by BCG-challenge. Possible discrepancies between gene and protein expression can be explained considering that multiple mechanisms operating at postranscriptional and postranslational levels (including non-coding RNAs, translation regulatory mechanisms, proteasomal activity) regulate protein expression. In addition, as shown for IL-1β, cytokine secretion can be regulated by the release of preformed molecules from intracellular stores, rather than at the level of gene transcription [50]. The soluble factors responsible for the stimulation of cytokine secretion by macrophages are conceivably a very complex cocktail of bioactive compounds of protein and non-protein nature, including biologically active molecules (e.g. prostaglandins, glycosaminoglycans) which are not primary gene products but products of multiple enzymatic reactions. For these reasons, the nature of the molecules secreted by BC cells responsible for the effect on macrophages may not be directly related to the gene expression profile.

In conclusion, our data show that ST3GAL1 expression and the consequent replacement of the T by the sT antigen in BC cells induce transcriptomic changes with a putative impact on multiple cellular functions associated with increased malignancy and susceptibility to oxidative damage and strengthens the inflammatory response of macrophages. This indicates that ST3GAL1 and T/sT carbohydrate structures can be factors with multiple clinical implications in BC.

BC:

bladder cancer

BCG:

Bacillus Calmette-Guérin

CMTMR:

5-(and-6)-(((4-chloromethyl)benzoyl)amino)tetramethylrhodamine

DMEM:

Dulbecco’s modified Eagle medium

FCS:

Foetal calf serum

FITC:

Fluorescein isothiocyanate

Gal:

Galactose

GalNAc:

N-acetylgalactosamine

GlcNAc:

N-acetylglucosamine

MES:

(N-morpholino)ethanesulphonic acid

MIBA:

Multiplex immune-beads assay

NMIBC:

Non-muscle invasive bladder cancer

PBS:

Phosphate-buffered saline

PNA:

Peanut (Arachis hypogea) agglutinin

RPMI:

Roswell Park Memorial Institute

Sia:

sialic acid

We thank Dr. Francesca Borsetti and Dr. Enzo Spisni, BIGEA Department of the University of Bologna for the help with the multiplex immune-beads assays, Dr. Christine M. Betts for the critical reading of the manuscript and Dr. Maria Letizia Bacchi-Reggiani (DIMES) for advices in statistical analysis.

Funding

This work was supported by: Portuguese Foundation for Science and Technology (FCT) PhD grants SFRH/BD/45120/2008 (Paulo F. Severino), SFRH/BD/81860/2011 (Mariana Silva) and SFRH/BD/100970/2014 (Mylène Carrascal), Liga Portuguesa Contra o Cancro 2011 (Mylène A. Carrascal); Prémio Bluepharma Inovação Universidade de Coimbra and the Santander Totta/ Universidade NOVA de Lisboa prizes (Paula Videira). Grants from the University of Bologna (Fabio Dall’Olio). Mariangela Catera and Giulia Venturi are PhD students supported by grants from the University of Bologna.

Availability of data and materials

The datasets generated during the current study are available from the corresponding author on reasonable request.

Authors and Affiliations

1. Centro de Estudos de Doenças Crónicas, CEDOC, NOVA Medical School/Faculdade de Ciências Médicas, Universidade NOVA de Lisboa, Campo dos Mártires da Pátria, 130, 1169-056, Lisbon, Portugal

   Paulo F. Severino, Mariana Silva, Mylene Carrascal & Paula A. Videira

2. UCIBIO, Departamento Ciências da Vida, Faculdade de Ciências e Tecnologia, Universidade NOVA de Lisboa, 2829-516, Caparica, Portugal

   Paula A. Videira

3. Dipartimento di Medicina Specialistica, Diagnostica e Sperimentale, Sede di Patologia Generale, Università di Bologna, Via S. Giacomo 14, 40126, Bologna, Italy

   Paulo F. Severino, Nadia Malagolini, Mariella Chiricolo, Giulia Venturi, Roberto Barbaro Forleo, Mariangela Catera & Fabio Dall’Olio

4. Centro Interdipartimentale Ricerche sul Cancro “Giorgio Prodi”, Università di Bologna, Bologna, Italy

   Annalisa Astolfi

Contributions

P.F.S and M.S. performed the bulk of the experimental work, analysed data and helped writing the manuscript. M. Car, G.V., M. Cat and R.B.F. performed part of the experimental work. N.M. and M. Chir. contributed to the establishment of transduced cell lines. A.A. performed microarray experiments and analysed microarray data. P.A.V. and F.D conceived the work, analysed the data and wrote the manuscript. All authors revised critically the manuscript, have given final approval of the version to be published and agree to be accountable for all aspects of the work in ensuring that questions related to the accuracy or integrity of any part of the work are appropriately investigated and resolved.

Corresponding authors

Correspondence to Paula A. Videira or Fabio Dall’Olio.

Ethics approval and consent to participate

This study does not use samples from diseased persons. The blood used for the preparation of monocyte-derived macrophages was from healthy blood donor voluntaries. For this, no study approval was necessary. The only authorization required was that obtained from the Blood Collection Service of the Pizzardi Hospital in Bologna, Italy, which keeps the rights on donors’ blood samples. This authorization is available to the Editor.

Consent for publication

Not applicable.

Competing interests

The authors declare that they have no competing interests.

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