Study outline
Ethical approval was obtained from RNSH human ethics committee (RESP/16/255).
Following provision of information on the study, DRESS patients gave informed written consent to have their blood collected for the study. For initial assay optimisation, blood was collected from healthy volunteers prior to being validated in DRESS and AGEP patients.
Blood collection and PBMC isolation
Fresh heparinised blood was collected for all experiments and PBMCs were collected using our previously published method(8). After collection off interface, PBMCs were washed with PBS and counted using a haemocytometer. Nine out of ten patients were in the recovery phase at time of blood collection and testing. Patient 7 was on low dose prednisone (under 10mg) at the time of testing.
Proliferation Assay evaluation
After PBMC collection and counting, cells were added to wells of a 96 well plate at a concentration of 200,000 cells per well in triplicate. Phytohaemagglutinin (PHA) at 5µg/ml (Sigma) and T-Cell Transact ™ beads (Miltenyi Biotec) at a 1:200 dilution, were used as positive controls. Negative control wells contained cells in culture media alone (RPMI + 10% FCS). Samples were incubated 37°C/5% CO2 for 6 days to allow for cell-stimulant interaction. At day 6, bromodeoxyuridine (BRDU), CyQUANT™, tetrazolium salt (3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (MTT) and tetrazolium salt (sodium 3´-[1- (phenylaminocarbonyl)- 3,4- tetrazolium]-bis (4-methoxy6-nitro) benzene sulfonic acid hydrate (XTT) proliferation detection assays were evaluated to determine which was most sensitive for determining cell proliferation in a non-radiolabelled LTT assay.
Briefly BRDU detection was performed using the Merck/Millipore Cell Proliferation ELISA, BrdU (colorimetric) assay (Catalogue number 2752) according to the manufacturer’s instructions. The CyQUANT™ NF cell proliferation assay kit (C35006) was performed as per manufacturer’s protocol. MTT (Sigma/Merck, Catalogue number M2128) at a stock concentration of 5mg/ml was added to each well for a final concentration of 0.5mg/ml (20µl per well) and incubated for 4hrs at 37°C. As T cells are not adherent, plates were spun at 1400 rpm for 10 minutes and supernatants carefully removed before addition of DMSO as a solvent to dissolve formazan crystals in the cells and plate read at 590nm. Absorbance was then read at 570nm. For XTT detection the (Roche/Sigma) cell proliferation kit II (XTT) was performed directly as per manufacturer’s instructions and read at 4, 6 and 24hrs at 492 and 690nm.
Other modifications tested
Once XTT had been shown to be the most sensitive and practical of the proliferation detection methods, other modifications to the assay were tested. The addition of autologous serum (AS) was tested to see the effect of proliferation on PHA and CD3+/CD28+ stimulated cells. AS is used in LTT assays particularly for Nickel allergies and reported to improve sensitivity. PBMCs were collected from three healthy controls. Briefly, RPMI media with 10% FCS was compared to RPMI with 10% FCS + 5% AS, or RPMI + 5% AS on PHA and CD3+/CD28+ stimulated cells over 6 days.
Regulatory T cell (T-reg) depletion by flow cytometric sorting was also tested. T-Regs may supress T cell, activation so depletion was tested to see if this improved the XTT-LTT assays sensitivity. Purified PBMCs from three healthy controls were stained with an anti-CD25 antibody (BD Biosciences) for 15 minutes at room temperature before CD25+ positive and negative PBMC’s were sorted using a BD FACSAria™. CD25+ positive and negative cell populations were spun at 1400 rpm for 5 minutes and washed in PBS prior to being counted and plated at 100,000 to 200,000 cells per well for testing in LTT assay. T-reg depleted (sorted) and unsorted PBMC’s +/- 5% AS were compared after stimulation with PHA and CD3+/CD28+ beads for 6 days. Positively sorted CD25+ve T-regs were also tested for proliferation levels to PHA and CD3+/CD28+ stimulation after 6 days with and without the addition of 5% AS.
Patient LTT
After XTT-modified LTT (XTT-LTT) assay optimisation, 8 patients diagnosed with DRESS and 2 with AGEP were tested with the XTT-LTT against implicated drugs and metabolites in some cases. A further 6 age and gender matched controls with no history of reactivity to any implicated drug were also added to the study. These drugs included vancomycin, piperacillin/tazobactam (Tazocin), sulfasalazine, allopurinol, apixaban, sulfapyridine, sulfamethoxazole, sulfamethoxazole + trimethoprim, amoxicillin/clavulanic acid, ceftriaxone, ceftotaxime, cefazolin, ceftazidime, benzylpenicillin, amoxicillin. All drugs were tested at 100µg/ml, 50µg/ml, 25µg/ml, 12.5µg/ml, 6.25µg/ml and 3.1µg/ml in duplicate or triplicate depending on the amount of patient cells available. The drugs allopurinol, oxypurinol, sulfapyridine and sulfamethoxazole had to be solubilized in DMSO prior to testing. PHA (Sigma) 5µg/ml and T-Cell Transact ™ beads (Miltenyi Biotec) at a 1:200 dilution, were used as positive controls. Negative control wells contained cells in RPMI media + 10% FCS alone. Drug-Cell interaction was carried out for 6 days at 37°C/5% CO2. At Day 6, 50µl of XTT solution was added to each well and read at 492 and 690nm at 4, 6 and 24hrs. All plates were frozen post 24hr read at -80°C for future cytokine analysis.
Cytokine Analysis
Ninety-six well plates stored at -80°C were removed and allowed to thaw at room temperature. Implicated drug-positive wells for each patient, along with PHA, T-Cell Transact ™ bead positive controls and negative controls were screened for interleukin-2 (IL-2), interleukin-4 (IL-4) and interleukin-5 (IL-5) levels by ELISA according to the manufacturers’ instructions (R and D Systems).
Data Analysis
One-way ANOVA
Data collected from each XTT-LTT patient or control were analysed using one-way ANOVA’ with Tukey’s multiple comparison post-test. All data was analysed with Prism 5.0 (Graph pad, La Jolla, CA).
Stimulation Index (SI) Calculation
Stimulation Index (SI) was calculated by dividing the XTT signal (492nm-690nm) of drug stimulated samples with the XTT signal of unstimulated samples with no drug added (negative control). A SI value of ≥ 2 was considered a positive result.