Dulbecco’s modified Eagle’s medium (DMEM) and fetal bovine serum (FBS) were obtained from PAA (Somerset, UK) or Sigma-Aldrich (Dorset, UK). Precision Plus Protein Colour standards and nitrocellulose were from Bio-Rad. RPMI-1640 medium, 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (MTT), dimethyl sulfoxide (DMSO) and propidium iodide were from Sigma-Aldrich. All other reagents were obtained from Sigma-Aldrich unless otherwise stated.

Diaspirin [bis(2-carboxyphenyl) succinate; PN508] and fumaryl diaspirin [bis(2-carboxyphenyl) fumarate; PN517] were prepared as previously described (37). Aspirin is commercially available as acetylsalicylic acid, and the synthesis of the other compounds is as described in supplementary information (provided upon request). The compounds tested are shown in Fig. 1.

These were prepared using the method described for PN508/PN517 (37) using sebacoyl chloride and terephthaloyl chloride, respectively. Both were recrystallised from 90/10 toluene ethanol mixture. PN511 is a white solid [mpt 135–136°C; literature mpt 139–142°C [see e.g. (45)]; IR (cm⁻¹): 2917, 2854, 1754, 1683, 1604]. PN512 is a white solid [mpt 295–300°C, IR (cm⁻¹): 1736, 1698, 1605]. The molar masses of the products were confirmed as 442 and 406 respectively by titration with standardised sodium hydroxide using the method described previously (37). Samples submitted for accurate mass spectrometry returned the following data: PN511 m/z (CI) 460.1964 (M + NH₄⁺, C₂₄H₂₆O₈NH₄ requires 460.1966); PN512 m/z (CI) 424.1025 (M + NH₄⁺, C₂₂H₁₄O₈NH₄ requires 424.1027).

PN524 was prepared by reaction of 3-bromobenzoyl chloride with salicylic acid in the presence of 1 mole-equivalent of pyridine. 3-Bromobenzoyl chloride is available commercially but can also be produced from 3-bromobenzoic acid by the action of excess thionyl chloride (SOCl₂). Refluxing for 2–3 h (with trapping of the evolved gases) until all of the solid material had dissolved, followed by removal of any excess thionyl chloride by distillation, gave an almost quantitative yield that can be used immediately in the subsequent step. Salicylic acid (0.1 mol, 13.81 g) was dissolved in THF (50 ml) and stirred. Pyridine (0.1 mol, 8.2 ml) was then added and the mixture was stirred magnetically while 3-bromobenzoyl chloride (~13.25 ml) was added slowly over 2–3 min. The temperature rose to 35–40°C during the addition. Pyridinium chloride was precipitated and stirring was continued for a further 12–24 h. Ice-cold water (200 ml) was then added and the mixture was stirred thoroughly. The mixture was extracted with diethyl ether (150 ml) by vigorous magnetic stirring. The ether layer was then separated and extracted with 10% Na₂CO₃ solution (150 ml) to remove the PN524 from unwanted by-products. The carbonate layer was then acidified with concentrated HCl until a precipitate was seen (pH 2.0–3.0). The precipitate was taken up in diethyl ether, separated and dried with anhydrous MgSO₄ before rotary evaporation of the ether. A clean white solid (17.0 g, 53%) was obtained. Recrystallisation was achieved from boiling hexane with some acetone added, by cooling to −15°C for 24–36 h. White crystals were obtained [mpt 140–142°C; IR (cm⁻¹): 3068, 1738, 1682, 1605]. The molar mass of the product was confirmed as 321 by titration with standardised sodium hydroxide using the method described previously (37).

PN525 was prepared in an analogous way using 4-methylbenzoyl chloride in place of 3-bromobenzoyl chloride. The product is a white solid and was recrystallized from toluene [mpt 148–150°C, IR (cm⁻¹): 1734, 1674, 1605]. The molar mass of the product was confirmed as 256 by titration with standardised sodium hydroxide using the method described previously (37).

Methyl salicylate (13.0 ml) was placed in a 100-ml conical flask. Pyridine (8.1 ml) was then added and the mixture was stirred magnetically while benzoyl chloride (11.6 ml) was added slowly over 2–3 min. The temperature rose to 48–50°C during the addition. Crystals of pyridinium chloride precipitated and stirring was continued for a further 2 h. Hexane (50 ml) was then added and the mixture was stirred thoroughly. The resulting heavy white precipitate (~35 g) was filtered and allowed to air dry before being shaken vigorously with water (100 ml) to dissolve the pyridinium chloride by-product. The remaining solid was filtered under vacuum and dried at 60°C. The yield was 15–16 g (~65%). This crude product had a mpt of 82–85°C. The product was recrystallised by dissolving in the minimum volume of hot acetone and then adding hot hexane until the solution just remained clear. The solution was then cooled to −15°C for a minimum of 24 h. A white solid [12.0 g, mpt 84–86°C; IR (cm⁻¹): 1737, 1715, 1605] was obtained. The literature mpt is 83.8–84°C (51).

Isopropyl salicylate was reacted with a slight excess of 3-bromobenzoyl chloride in the presence of pyridine with no additional solvent. Isopropyl salicylate is available commercially but we also prepared small quantities from 2-propanol and salicylic acid by refluxing them with a catalytic quantity of concentrated H₂SO₄. A ratio of 25 g salicylic acid to 100 ml 2-propanol was used with 1–2 ml of concentrated H₂SO₄. After a minimum of 12 h refluxing, the excess 2-propanol was removed by rotary evaporation. The residue of oily solid was shaken with 10% NaHCO₃, with more solid bicarbonate added until all the unreacted salicylic acid had dissolved. This mixture was then extracted well with diethyl ether before separating the ether layer, drying over anhydrous MgSO₄ and removing the ether by rotary evaporation. A low yield (3–5 g; 9–15%) of almost pure isopropyl salicylate (tlc) was obtained and used without further purification. 3-Bromobenzoyl chloride was obtained as described for the preparation of PN524 above. Isopropyl salicylate (1.90 g) was mixed with pyridine (1.6 ml) and was then added carefully to 3-bromobenzoyl chloride (2.38 g). An immediate reaction produced a near-solid product. The reaction vessel was protected with a silica gel guard tube and left at room temperature for 2–3 days to complete the reaction. Water (20 ml) was added to the tube which was stoppered and shaken vigorously. A sticky oil was released which was taken up in diethyl ether, washed with 10% NaHCO₃ (20 ml) and then water (20 ml). The ether layer was dried over anhydrous MgSO₄ and rotary evaporated to give a clear, pale yellow oil (3.4 g; 87%). A solid product was obtained by dissolving the oil in a little warm diethyl ether and then diluting with boiling hexane or light petroleum ether until a cloudy solution was observed. Storing this mixture at −15°C for 2–3 days gave white crystals [mpt 49–51°C, IR (cm⁻¹): 2979, 1735, 1703, 1606].

The human colorectal adenocarcinoma cell line SW480 (supplied by ECACC) was cultured in Leibovitz’s L-15 medium containing 10% (v/v) FBS supplemented with 1% L-glutamine-penicillin-streptomycin (Sigma-Aldrich). The human colorectal adenocarcinoma cell lines LoVo and HCT-116, the human breast carcinoma cell line MCF-7 and the human endothelial cell line EA.hy926 were all kindly provided by Dr Wang (University of Wolverhampton) and maintained in DMEM containing 10% (v/v) FBS supplemented with 1% L-glutamine-penicillin-streptomycin (Sigma-Aldrich). The A549 human lung adenocarcinoma cell line was provided by Dr Safrany (University of Wolverhampton) and maintained in RPMI-1640 medium supplemented with 10% FBS with 1% L-glutamine-penicillin-streptomycin. In cytotoxicity experiments for IC₅₀ determinations, to minimize medium-specific variation, cells were cultured and tested in DMEM containing 10% (v/v) FBS supplemented with 1% L-glutamine-penicillin-streptomycin. The murine adenocarcinoma cell line MAC13 [supplied by Professor Double, University of Bradford (38)] was maintained in RPMI-1640 medium supplemented with 10% FBS/1% pen/strep solution/1% glutamine. The SW480 cell line was maintained in L-15 medium, was cultured at 37°C and regularly passaged at ~80% confluency. All other cells were cultured at 37°C in a humidified incubator with 5% CO₂ and regularly passaged at ~80% confluency.

Compounds were prepared as a stock (0.5 M) in DMSO, prior to addition to cells. The cytotoxic effect of aspirin and the other novel compounds was evaluated using the MTT assay (39) with modification (40). Briefly, 10⁴ cells/well were cultured overnight in 96-well microtitre plates. Twenty-four hours after the initial seeding, the culture medium was discarded, and the cells were incubated with medium containing drugs at the requisite concentration and incubated for the tested time at 37°C, then replaced with medium containing 300 μl of 0.5 mg/ml MTT per well and incubated for 3 h at 37°C, then replaced with 200 μl of DMSO and incubated for 10 min at 37°C to develop a coloured formazan complex. Absorbance was recorded at 540 nm using a visible plate reader (Labsystems Multiskan MS). Viability is reported as the percentage of treated cells relative to the cells in control wells. Compound anti-proliferative activity, stated as IC₅₀ values, was determined by interpolation or using non-linear regression analysis using GraphPad Prism Statistics Software package (ver. 6.0; San Diego, CA, USA).

For the evaluation of toxicity (in vitro) to the MAC13 cell line, when plated cells reached 90% confluency they were treated with either PBS, aspirin, DiA or F-DiA dissolved in PBS. After 48 h at 37°C the cells were washed in PBS twice before 0.5 ml trypsin-EDTA (10%) was added, and the cell numbers were determined using a Coulter Counter.

For evaluation of the activity described in Figs. 3–5, the compounds were prepared as a 1 M stock solution in DMSO and sonicated to achieve solubility. DMSO concentrations never exceeded 0.5% of the medium volume. The medium containing drugs was sonicated until all visible particles were dissolved. The pH was subsequently adjusted to 7.6 with NaOH. Aspirin (Sigma, USA) was solubilized in water using 10 M NaOH and the pH was adjusted to 7.0.

Staining for cell surface phosphatidylserine residues was carried out using an Annexin V -FITC apoptosis detection kit (Oncogene Research Products) according to the manufacturer’s instructions. The percentage of apoptotic cells was measured using BD FACS Aria II (BD Biosciences, Franklin Lakes, NJ, USA). A negative control without the Annexin V -FITC antibody and DAPI were used to assess the background signal.

After drug treatment, SW480 cells were trypsinized and pelleted for 5 min at 1,600 rpm. The supernatant was removed. The cells were suspended in 100 μl citrate buffer and 450 μl of solution A [10 mg trypsin type IX-S in 500 ml stock solution (2 g trisodium citrate, 121 mg Tris-base, 1044 mg spermine tetrahydrochloride, 2 ml Nonidet NP-40 in 2l dH₂O, pH 7.6)] was added to the samples and vortexed for 2 min. Subsequently, 375 μl solution B (250 mg trypsin inhibitor, 50 mg RNAse A in 500 ml stock solution, pH 7.6) was added to the samples, vortexed briefly and incubated for 10 min at room temperature. Next, 250 μl solution C (208 mg propidium iodide, 500 mg spermine tetrahydrochloride in 500 ml stock solution, pH 7.6) was added to the samples and vortexed briefly and incubated on ice in the dark for 10 min. Distribution of cells in the different phases of the cell cycle was analysed using BD FACS Aria II.

For the analysis of NF-κB-driven transcription, cells were transfected with the 3′ enhancer CONA (3x κB ConA-Luc) (supplied by Professor R.T. Hay, University of Dundee) and pCMV-β-galactosidase (Promega) plasmids as described previously (41). The relative luciferase activity was calculated as units of luciferase activity per unit of β-galactosidase activity.

Following treatment, cytoplasmic and nuclear extracts were prepared as previously described (42). The protein concentration was determined using a Bradford assay (Bio-Rad). Protein extracts (20–50 μg) were resolved using discontinuous SDS-PAGE with a 10% gel, and immunoblotting was conducted using standard procedures. Primary antibodies used were: rabbit anti-cyclin D1 (Thermo Scientific, USA; 1:1000), sheep anti-IκB (a kind gift from R.T. Hay) and mouse anti-actin as a loading control. Proteins were detected using western blotting luminol reagent (Santa Cruz, USA). ImageJ software (NIH) was employed for densitometric analysis of the western blots.

NMRI nude mice from the Aston colony were treated with MAC13 cells (5×10⁶) sub-cut into their flanks. Once the tumour was established, it was dissected and small fragments were re-transplanted (subcutaneously) into more mice. Mice (~20 g in weight) were selected at random and administered PBS or DiA or F-DiA, dissolved in PBS (1 mg/kg) intravenously. Animals were randomly divided (6 animals/group). Medication was administered intravenously daily. The mice were monitored daily for weight, food and water consumption. Tumour size was recorded using callipers. Prior to the animal model experiment, as much as 5 mg/kg compound was given to several control mice and no toxicity was observed (data available upon request). The experiment ended when the control mouse tumours started to ulcerate. All animal experiments were conducted under Home Office Licence in accordance with the UK Animals (Scientific Procedures) Act 1986.

Values are expressed as means ± SD or SEM. To evaluate the difference in means between groups in the animal study, one-way ANOVA followed by Tukey’s post-hoc test was undertaken.

To understand the molecular basis for the antitumour effects of aspirin and identify more effective alternatives, we previously synthesised a series of derivatives of the aspirin molecule. These studies revealed that diaspirin (DiA) and fumaryl diaspirin (F-DiA) inhibit proliferation of CRC cell lines at significantly lower concentrations than aspirin (37). To extend these studies and identify further lead molecules, we synthesised an additional series of aspirin derivatives (Fig. 1). Cytotoxicity (MTT) assays demonstrated that at 0.5 mM (pharmacologically relevant dose for aspirin), DiA (PN508) and F-DiA (PN517) and to an even greater extent, isopropyl m-bromobenzoylsalicylate (PN529) reduced the viability of SW480 CRC cells (Fig. 2A). To investigate the specificity of compound toxicity in more detail, we tested the capacity of DiA, F-DiA and PN529 to affect proliferation of a number of established cell lines in vitro (Fig. 2B and Table I), controlling for any variability that could arise from cell culture conditions through culturing all cells with DMEM as the basal medium. While we noted that culturing SW480 cells in their non-native medium (DMEM rather than L-15 medium) reduced the sensitivity of the cells to the compounds tested, DiA and F-DiA in this assay system arguably showed a modicum of specificity towards the other CRC cell lines tested (HCT116 and LoVo), and given our finding that PN529 can induce necrosis (37), we focused our attention on the anti-proliferative activity of DiA and F-DiA in more detail in vitro and in vivo.

The major anti-proliferative effect of aspirin is recognised to be the induction of apoptosis. However, the mechanism by which DiA and F-DiA act against CRC cells is as yet unknown. To further understand this mechanism, we used Annexin V assays to investigate the effects of aspirin derivatives on apoptotic cell death. We found that both compounds (3 mM) induced a significant increase in the percentage of SW480 CRC cells undergoing apoptosis, compared to the carrier (DMSO)-treated controls (Fig. 3). This increase in apoptosis was paralleled by a decrease in the percentage of viable cells, confirming the death-inducing capacities of the agents (data not shown). Time course studies revealed that 3 mM F-DiA mediated a significant increase in apoptosis within 3 h of treatment (Fig. 3), while a more prolonged (>5 h) exposure was required before DiA-mediated apoptosis was evident (data not shown). In contrast to the diaspirin compounds, aspirin at 3 mM had minimal effect on cell growth/death after an 18-h exposure (data not shown), which is in keeping with previous studies showing that 5 mM aspirin is required to induce detectable apoptosis of these cells within this time frame (41). Taken together, these data indicate that the diaspirin compounds induce apoptosis of CRC cells and that this occurs at a lower concentration than for aspirin and that F-DiA is the more active of the compounds.

Having established that the aspirin analogues induce apoptosis, we next aimed to determine whether the underlying mechanism is similar to that of aspirin. Understanding the mechanism of action of these agents may not only identify novel apoptotic pathways, but may also reveal structural aspects of aspirin that are important for its antitumour activity. Degradation of cyclin D1 is an early response to aspirin and is critical for its apoptotic activity (29). Therefore, we firstly examined the effects of the agents on cellular levels of this protein. We found that both DiA (3 mM, 18 h) and F-DiA (3 mM, 18 h) induced a marked decrease in cyclin D1 levels (Fig. 4A). Furthermore, this decrease was time-dependent and for both agents, preceded the induction of apoptosis (Fig. 4B). However, unlike the G2/M cell cycle arrest observed in response to aspirin, DiA- and F-DiA-mediated depletion of cyclin D1 was not associated with significant changes in the cell cycle profile (Fig. 4C).

NF-κB is a ubiquitously expressed transcription factor that plays a critical role in cell growth and death. It generally resides in the cytoplasm as a heterodimer of the RelA/P50 subunits, bound to the inhibitor protein, IκB. In response to a variety of agents, IκB is degraded allowing NF-κB to translocate to the nucleus and regulate expression of target genes. Thoms et al previously demonstrated that aspirin-induced degradation of cyclin D1 is linked to the induction of apoptosis through stimulation of this pathway (29). Moreover, cyclin D1 is transcriptionally activated by NF-κB. To determine whether DiA- and F-DiA-mediated depletion of cyclin D1 and induction of apoptosis are also associated with modulation of NF-κB signalling, we firstly examined the effects of these agents on IκBα. Fig. 5A demonstrates that both DiA and F-DiA induced a marked decrease in cytoplasmic levels of this protein, suggestive of proteasome-mediated degradation.

Following aspirin-mediated degradation of IκB, RelA translocates from the cytoplasm to the nucleoplasm and then to a nuclear compartment, the nucleolus (41,43). This nucleolar compartmentalisation of RelA causes a reduction in basal levels of NF-κB transcriptional activity, which is critical for the apoptotic effects of the agent. Immunocytochemical analysis demonstrated that DiA and F-DiA induced a substantial increase in nucleoplasmic RelA, confirming that these agents stimulated the NF-κB pathway. However, in contrast to aspirin, the protein did not accumulate specifically in nucleoli (Fig. 5B and C). Time-course studies demonstrated that for both compounds, translocation of RelA to the nucleoplasm was subsequent to degradation of cyclin D1, but preceded the induction of apoptosis (Fig. 5C). They also demonstrated that F-DiA-mediated nucleoplasmic accumulation of RelA was more rapid and significant than that induced by DiA, in keeping with the apoptotic effects of the agents. Indeed, nucleoplasmic RelA was evident within 1 h of F-DiA treatment and cells appeared dead within 3 h.

In response to specific stresses, nucleoplasmic NF-κB/RelA complexes have been shown to mediate apoptosis by repressing basal NF-κB-driven transcription (44). To examine this as a possible mechanism for the apoptotic effects of the diaspirin compounds, we next performed NF-κB reporter assays. We found that both DiA and F-DiA induced a significant decrease in basal levels of NF-κB transcriptional activity. This decrease was more pronounced than for aspirin, occurred in a time-dependent manner and was subsequent to nucleoplasmic accumulation of RelA (Fig. 5C and D). Furthermore, similar to depletion of cyclin D1, nucleoplasmic accumulation of RelA and the induction of apoptosis, we found that F-DiA had a more rapid and profound effect on NF-κB-driven transcription than DiA (Fig. 5E). These data suggest that, similar to aspirin, the diaspirin compounds stimulate the NF-κB pathway and mediate apoptosis through repression of NF-κB-driven transcription. However, they also suggest that the mechanism underlying this repression differs between aspirin and the related agents.

Taken together, the above data suggest that the diaspirin compounds, particularly F-Dia, have potent activity against CRC cells. To determine whether these effects translate into in vivo potency, we utilised the well characterised MAC13 syngeneic mouse model of CRC (38). In the cytotoxicity assays MAC13 cells cultured in vitro were more sensitive to DiA and F-DiA than aspirin (data not shown); in vivo, the mouse colon carcinoma cells were implanted subcutaneously into NMRI mice and treatment commenced 12 days after implantation. Low dose (1 mg/kg) DiA or F-DiA was administered every day for 10 days by intravenous injection. No overt side-effect was observed between the treatment and vehicle-treated control group, and food and water intake was unaffected. As shown in Fig. 6, treatment with DiA and F-DiA significantly inhibited the growth of the tumours, and almost complete suppression of growth was apparent in the mice treated with F-DiA.