Fluorescence-guided development of a tricistronic vector encoding bimodal optical and nuclear genetic reporters for in vivo cellular imaging

All cell culture medium and supplements were obtained from Lonza BioWhittaker (Walkersville, USA) unless otherwise stated. A human T cell lymphoblastic lymphoma-derived cell line (SupT1) was obtained from the American Type Culture Collection (ATCC, University Boulevard Manassas, USA) and cultured in RPMI 1640 media (St. Louis, USA) supplemented with 10% foetal bovine serum (FBS) and GlutaMAX (Gibco, Grand Island, USA). Cell lines were maintained at 37°C in a humidified 5% CO₂ atmosphere. Three SupT1 cell populations were engineered, each with a different expression cassette; (1) an IRES-based bisictronic vector encoding for hNET and a cell surface marker CD34 (vector 1: SupT1/hNET.I.CD34), (2) a 2A peptide-linked tricistronic vector encoding for hNET, red-shifted codon optimised FLuc [25] and a highly compact marker/suicide gene RQR8 [22] with 2A linkage at the N-terminus of hNET (vector 2: SupT1/FLuc.2A.RQR8.2A.hNET) and (3) at the C-terminus hNET (vector 3: SupT1/hNET.2A.FLuc.2A.RQR8). Moloney murine leukaemia virus (Mo-MuLV) long terminal repeat (LTR) promoter was used. SupT1 cells were transduced with RD114 pseudotyped supernatant generated from transfection of HEK-293T cells with the expression plasmids supplying Gagpol (gift from Elio Vanin, Baylor College of Medicine), RD114 envelope (gift from Mary Collins, University College London) PeqPam-env and each of the three hNET encoding vectors above. Transduction efficiency was determined by flow cytometry with αCD34-APC staining for vector 1 and QBEnd10 staining as previously described [22] for vectors 2 and 3.

SupT1 cells (1 × 10⁶) transduced with hNET vector 1 were incubated at 37°C with varying concentrations of ASP⁺ (1 × 10⁻³, 5 × 10⁻³, 1 × 10⁻², 5 × 10⁻², 0.1, 0.5, 1 μM) for 10, 30, 60, 120 and 240 min. The cells were washed once with fluorescence activate cell sorting (FACS) buffer containing 1% FBS, phosphate saline buffer (PBS) and 50 mg/mL Normocin (InvivoGen, San Diego, USA). The supernatant was discarded and cells were re-suspended in 500 μL of FACS buffer. Flow cytometry was performed using Beckman Coulter Cyan instrument (Beckman Coulter, Brea, USA).

Optimal ASP⁺ staining conditions determined above were used for ASP⁺-guided flow sorting of SupT1 cell lines expressing the three hNET vector constructs. Cells were prepared as described above. ASP⁺ mean fluorescence intensities (MFI) were determined pre- and post-FACS (Beckman Coulter MoFlo-XDP) using areas under the curve and subtracting any non-specific signal from non-transduced SupT1 (SupT1/NT) cell populations. Measurements were acquired in triplicates for each cell line and statistical significance of differences between mean values was obtained with IBM SPSS software using the one-way ANOVA and the Tukey’s HSD test.

SupT1 cells expressing vectors 1 and 2 were further characterised by radiosubstrate uptake studies. 1 × 10⁶ SupT1/hNET.I.CD34, SupT1/FLuc.2A.RQR8.2A.hNET and SupT1/NT cells were incubated for 30 min at 37°C with [¹²⁵I]-MIBG (7.4 kBq). The cells were rapidly washed twice with 500 μL ice-cold PBS and the supernatant collected. Cell pellets were resuspended in 1 mL PBS. Radioactive uptake was determined by gamma counting (WIZARD, PerkinElmer, Beaconsfield, UK) of the resuspended cells and corresponding supernatants. Percentage [¹²⁵I]-MIBG cell uptake was calculated by dividing the counts in the cell pellet by the total counts (counts in cell pellet + counts in supernatant). All experiments were performed in triplicates. The one-way ANOVA and the Tukey’s HSD test were used to determine the significance of differences between mean values.

All animal procedures were carried out in accordance with the UK Animals (Scientific Procedures) 1986 Act and institutional ethics regulation. SupT1/FLuc.2A.RQR8.2A.hNET cells (5 × 10⁶) or non-transduced SupT1 cells (5 × 10⁶) were injected into the subcutaneous space of the right flank of NOD/SCID mice (n = 3 in each group). Seven days later, BLI images (Biospace photon imager Optima system, Paris, France) were acquired 15 min post-intraperitoneal administration of 200 μL of D-Luciferin (10 mg/mL) using a 50 mm CCD lens with a sensitivity of 37 photons/s/sr/cm². Images were analysed using Biospace M3 Vision software. 15 MBq (150 μL) of [¹²³I]-MIBG (Mallinckrodt, Northampton, UK) was subsequently administered to animals via tail vein followed by whole body SPECT/CT imaging (nanoSPECT silver upgrade, Mediso, Budapest, Hungary) at 1 h, 4 h and 24 h post injection. Images were reconstructed using HiSPECT software (InviCRO, Boston, USA) followed by image processing and analysis using VivoQuant Software (InviCRO, Boston, USA).