Preclinical Evaluation of Invariant Natural Killer T Cells Modified with CD38 or BCMA Chimeric Antigen Receptors for Multiple Myeloma

iNKT cells were isolated from healthy donor peripheral blood mononuclear cells (PBMCs) by Vα24⁺ selection using magnetic cell sorting. Directly after cell sorting the iNKT cell purity was ~30–70% with an iNKT cell content of 50.000–200.000 cells based on the double positive expression of Vα24 paired with Vβ11, as shown in Figure 1A. After one week of stimulation with α-galactosylceramide (α-GalCer) pulsed PBMCs, the cells expanded with a median of 11.7-fold (range 3–18), the purity increased up to 90%, and the cells were transduced with the affinity-optimized CD38B1-CARs containing three different co-stimulatory domains or with the BCMA-CAR, as schematically depicted in Figure 1B. The low-affinity nerve growth factor (LNGFR), dsRed, or 4–1BBL, which were co-expressed in the three different CD38-CAR constructs, were used to determine transduction efficiency, and used as a surrogate for CAR expression, as previously validated [43]. The BCMA-CAR expression was determined via direct CAR expression as measured by a goat-anti-mouse F(ab’)2 binding to the murine scFv sequence. The mean transduction efficacy of CAR-iNKT cells was ~50% (range: 20–90%, n = 8), as shown in Figure 1C, similar to transduction efficacies of conventional T cells in our earlier studies [42,43].

CAR-transduced iNKT cells were tested for their cytotoxic activity through the CAR-specific targeting of CD38 or BCMA expressed on multiple myeloma (MM) cell line UM9, as shown in Figure 2A. As expected, the UM9 cells were completely eradicated by the iNKT cells expressing the high affinity BCMA-CAR. Since the expression of CD38 on UM9 cells is intermediate, as shown in Figure 2A, left panel, a lysis up to 60% was observed for the affinity tuned CD38-CAR iNKTs, with no noteworthy distinction between CARs containing different costimulatory domains. Mock-transduced iNKT cells did not lyse UM9 cells.

To determine their cytotoxic activity via the CD1d-restriced invariant TCR, CD38-CAR, BCMA-CAR, and mock-transduced iNKT cells were tested against the CD1d intermediate positive MM1.s cells and against its CD1d-transduced variant with high levels of CD1d expression, as shown in Figure 2B. Since MM1.s cells express high levels of CD38 and BCMA, they were completely eliminated by both CD38- and BCMA-CAR iNKT cells even at low effector to target (E/T) ratios, whereas the lysis by mock-transduced iNKT cells was very low. Suggesting the intact signaling from the invariant TCR against MM cells, the mock-transduced cells killed the MM1.s cells up to 50% at high E/T ratios, in agreement with the intermediate CD1d expression detected on MM1.s, as shown in Figure 2C, left panel. Importantly, the CD1d-transduced MM1.s cells were completely eradicated, not only by CAR-transduced, but also mock-transduced iNKT cells even at low E/T ratios, suggesting the full functional activity of the endogenous CD1d restricted invariant TCR, as shown in Figure 2C, right panel.

To study the effect of CAR iNKT cells on primary MM cells, we conducted flow-based cytotoxicity assays on eight randomly selected bone marrow mononuclear cells (BM-MNC) from MM patients. These samples contained 10–40% malignant plasma cells (MM-PC) identified as cells expressing CD38^highCD138⁺, as shown in Figure 3A,B. Since the BM-MNCs contain both malignant MM cells and non-malignant hematopoietic cells, this flow-based assay system allows us to simultaneously determine the on-tumor and off-tumor cytotoxic activity of CAR-transduced cells [41,42]. As illustrated in Figure 3C, all primary MM cells were effectively lysed by CD38-CAR as well as BCMA-CAR-transduced iNKT cells, with no influence of the costimulatory domain. Since BCMA is expressed only on PCs, BCMA-CAR iNKTs did not lyse CD138 negative non-malignant hematopoietic cells. Importantly, and consistent with all our previous studies [41,42,43], the cytotoxic activities of affinity optimized CD38-CAR iNKTs were also exclusively directed against CD38^highCD138⁺ MM cells, while CD38^int/high CD138^– non-malignant cells were largely ignored, as shown in Figure 3A. Of note, in seven out of the eight samples there was little or no CD1d⁺ expression MM cells. Consequently, there was no mock-reactivity against these MM cells, as shown in Figure 3C, panel Mock. In the only sample that contained CD1d⁺ MM plasma cells there was significantly elevated levels of lysis by mock-transduced cells, again indicating the functional activity of the endogenous TCR, as shown in Supplementary Figure S1.

To further study the relevant functions of CAR iNKT cells, we analyzed the CAR-dependent cytokine production profile in response to one of the primary MM samples, as shown in Figure 4. A typical Th1 profile with very high levels of the proinflammatory cytokines IFN-γ and TNF but low or no production of Th2 cytokines IL-4 and IL-10 was found only for CD38-CARs carrying the 4-1BB costimulatory domain. Although other CAR iNKT cells also produced somewhat higher levels of IFN-γ as compared to IL-4, the IFN-γ to IL-4 ratios were in general lower than 10, suggesting a Th1/Th0 cytokine profile. Interestingly though, IL-2 was not detected above the levels observed from mock-transduced iNKT cells. A typical Th17 profile was not found in CAR iNKT cells. Furthermore, as expected, none of the CAR iNKT cells or mock-transduced iNKT cells produced significant levels of IL-6, one of the important cytokines associated with cytokine release syndrome.

We next evaluated the ex vivo expandability of the CAR iNKT cells. Since the costimulatory domain could influence the proliferative capacity, we focused on CD38-CAR iNKT cells and expanded them in a CAR-dependent manner by weekly stimulation with irradiated UM9 cells, as shown in Figure 5. The CD38-BBz-CAR iNKT cells vigorously proliferated upon stimulation with UM9, until the end of the experiment (Week 6), with total CAR⁺ iNKT cell yields around 10⁷ cells. The growth of CD38-CARs carrying the CD28 costimulatory domain stagnated after Week 4, as shown in Figure 5A. Mock-transduced cells proliferated to a lower extent as compared to CD38-BBz-CAR iNKT cells, revealing the contribution of CD38-specific stimulation in the exponential growth of CD38-CAR iNKT cells. Moreover, supporting this conclusion, at the end of the cultures, the percentage of CAR⁺iNKT cells in cultures transduced with CD38-BBz-CAR markedly increased from 30% to 70% and maintained their CAR-dependent cytotoxic activities, as shown in Figure 5C. iNKT cells transduced with the CD38-CAR carrying the 4-1BB costimulatory domain expressed little or low levels of PD-1 during the whole culture period. In contrast, CD38-CAR iNKT cells containing the CD28 costimulatory domain expressed high levels of PD-1, as shown in Figure 5D, left panel. In addition, the CD57 molecule, which is associated with exhaustion/senescence [46,47,48,49] was virtually absent in all CAR-transduced iNKT cells in contrast to mock-transduced cells, as shown in Figure 5D, middle panel. Reversely, the CD39 molecule, which is thought to regulate activation of iNKT cells [50,51], was positive on all CAR-transduced, but not on mock-transduced iNKT cells, as shown in Figure 5E, right panel. Taken together, these results indicated that 4-1BB provided the most suitable costimulatory signals for CAR-iNKT cells.

In further analyses, we evaluated whether the CAR iNKT cells could be stimulated and expanded by mature monocyte dendritic cells (moDC) loaded with α-GalCer. Since moDCs also express CD38, CD38-CAR iNKT cells would receive both CAR- and TCR-mediated signals, while BCMA-CARs would receive only signals from the invariant TCR. Therefore, we first studied the stimulation of BCMA-CARs in a series of experiments with four different donors, as shown in Figure 6A. BCMA-CAR iNKT cells vigorously proliferated upon stimulation with α-GalCer loaded DCs. Although their expansion rates were not as good as that of the mock-transduced iNKT cells, we achieved 1000-fold expansion of CAR⁺ iNKT cells in five weeks of time, as shown in Figure 6A, middle panel. As expected, the CAR iNKT percentages remained unchanged and BCMA CAR iNKT cells maintained their CAR-dependent cytotoxic activities at the end of the expansion period, as shown in Figure 6B.

Unlike the UM9 stimulated CD38-CARs, the BCMA-CARs stimulated with α-GalCer loaded DCs were largely positive for the PD-1 molecule during the whole culture period (data not shown). Therefore, in an independent setting we compared the growth of the iNKT cells transduced with BCMA-CARs and the most optimal CD38-BBz-CAR upon stimulation with α-GalCer loaded DCs, as shown in Figure 6C, and observed that the expansion rates of BCMA-CAR and CD38-CAR cells were somewhat lower (300–500-fold) but similar. Nonetheless, while the percentages of BCMA-CAR⁺ iNKT cells remained the same over time, the percentage of CD38-CAR⁺ iNKT cells diminished, as shown in Figure 6C, right panel. Furthermore, unlike CAR-dependent stimulations, CD38-CAR iNKT cells also expressed PD-1 after stimulation with α-GalCer loaded DCs. The checkpoint molecules Lag3 and Tim3 were also positive on both BCMA- and CD38-CAR iNKT cells.

Finally, we questioned whether CAR iNKT cells that have already been stimulated for several rounds with tumor cells in a CAR-dependent fashion could be further stimulated with α-GalCer loaded DCs. As illustrated in Figure 7, it was still possible to expand fully cytotoxic CD38-CAR iNKT cells by stimulation with α-GalCer loaded DCs, even if they had been stimulated for 6 weeks only with tumor cells.

CD38B1-CAR (in short CD38-CAR) constructs containing different costimulatory domains were previously described in detail [42,43]. The BCMA-CAR contained the 4-1BB costimulatory domain and was constructed using the published murine scFv sequence derived from BCMA02 CAR (product name bb2121, WO 2016/094304 A2) [55]. In the SFG retroviral construct, the scFv was followed by a CD8a transmembrane domain and the 4-1BB and CD3ζ signaling domains or a CD28 transmembrane domain and intracellular sequence as described in Zhao et al. [45]. The CAR sequences were linked by a P2A sequence [56] to a truncated low-affinity nerve growth factor (LNGFR), dsRed, or 4-1BBL sequence, as depicted in Figure 1A. The 4-1BBL sequence, which was obtained form EBV-LCL cell line 10850, was integrated in CD38B1-CAR vectors as described previously [43].

Phoenix-Ampho packaging cells were transfected with 10 μg CAR constructs + 5 μg gag-pol (pHIT60), and 5 μg envelope (pCOLT-GALV) vectors (Roche, Basel, Switserland) using calcium phosphate precipitation. Next, 16 h post-transfection medium was replaced with complete Dulbecco’s modified Eagle medium (DMEM) + 10% fetal bovine serum (FBS, and two and three days after transfection, cell free supernatants containing retroviral particles were collected and directly used for transduction of iNKT cells.

Healthy donor blood peripheral mononuclear blood cells (PBMCs) were isolated from buffy coats (Sanquin, Amsterdam, The Netherlands) through Ficoll-Paque (GE Healthcare Life Sciences, Hoevelaken, The Netherlands) density centrifugation. iNKT cells were purified using a Vα24 specific iNKT isolation kit (Miltenyi Biotec, Leiden, The Netherlands). Isolated iNKT cells were cultured in RPMI-1640 (Life Technologies, Bleiswijk, The Netherlands) supplemented with 10% FCS (Invitrogen, Bleiswijk, The Netherlands), penicillin (100 U/mL) and streptomycin (100 µg/mL), and 5.5 mM beta-mercaptoethanol (Gibco, Bleiswijk, The Netherlands). After isolation, the iNKTs were stimulated with the negative PBMC fraction irradiated (25 Gray) in a 1:1 ratio, supplemented with 100 ng/mL α-galactosylceramide (α-GalCer) (KRN7000 Funakoshi, Tokyo, Japan). The culture was supplemented with rhIL-2 (50 U/mL) (R&D, Minneapolis, MN, USA), rhIL-7 (10 ng/mL), and rhIL-15 (10 ng/mL) (PeproTech, London, UK) twice a week until retroviral transductions, which were performed in a RetroNectin-coated (15 µg/mL) (Takara, Saint-Germain-en-Laye, France) non-tissue treated 24-well plate (Corning, Amsterdam, The Netherlands) at a density of 5–10 × 10⁵ cells/mL in the presence of 1.0 mL virus per well followed by spinoculation (3000 rpm, 1 h at room temperature) in the presence of 4 µg/mL Polybrene (Sigma, Zwijndrecht, The Netherlands). A second transduction was conducted after 16 h, replacing 2/3 of the cell supernatant with freshly obtained virus. Then, 6–8 h after the second hit, half of the cell supernatant was replaced by fresh complete culture medium (RPMI-1640) (Life Technologies, Bleiswijk, The Netherlands) with the cytokine mix as previously described. Transduction efficiency was determined after 72 h as described in the flow cytometry section. iNKT cells were cultured in 48 or 24 well plates and were split 1:2 once a cell density of 1.5–2 × 10⁶ cells per/mL was reached. Every 7–10 days, irradiated (25 Gray) α-GalCer pulsed dendritic cells (DC) were added at E/T ratio 1:1 and the cultures were supplemented with the cytokine mix described earlier.

CD14⁺ cells were isolated from PBMCs using CD14 MicroBeads (Miltenyi Biotec, Leiden, The Netherlands) and were cultured in RPMI-1640 (Life Technologies, Bleiswijk, The Netherlands) supplemented with 10% FCS (Invitrogen, Bleiswijk, The Netherlands), penicillin (100 U/mL), and streptomycin (100 µg/mL) supplemented with 580 U/mL IL-4 and 1000 U/mL granulocyte/macrophage colony-stimulating factor (GM-CSF). After 5 days, 100 ng/mL α-GalCer and 1000 ng/mL Lipopolysacharide (LPS) were added. At Day 7, the mature, α-GalCer loaded moDCs with high expression of CD80, CD83, CD86, and HLA-DR were harvested and used to stimulate iNKT cells [57].

Bone marrow mononuclear cells (BM-MNCs) from MM patients containing ~10–40% malignant plasma cells (determined as CD38⁺/CD56^+/−/CD138⁺ cells by flow cytometry) were isolated from bone marrow aspirates through Ficoll-Paque (GE Healthcare Life Sciences, Hoevelaken, The Netherlands) density centrifugation. Isolated cells were directly used in cytotoxicity assays or cryopreserved in liquid nitrogen until use. All primary samples were obtained after informed consent and according to the code of conduct for medical research developed by The Council of the Federation of Medical Scientific Societies (FEDERA https://www.federa.org/codes-conduct↗).

Luciferase-transduced or unmodified human MM cell lines UM9, MM1.s, and MM1.s-CD1d were previously described [41,58,59]. The MM cell lines were cultured in RPMI-1640 ((Life Technologies, Bleiswijk, The Netherlands)) with 10% HyClone FCS (Fisher Scientific, Amsterdam, The Netherlands) and antibiotics (penicillin; 100 U/mL, streptomycin; 100 µg/mL). Phoenix Ampho cells were cultured in Dulbecco’s modified Eagle medium (DMEM) + GlutaMAX ((Life Technologies, Bleiswijk, The Netherlands)) with 10% FCS (Invitrogen, Bleiswijk, The Netherlands) and penicillin (10,000 U/mL) and streptomycin (10,000 µg/mL).

Flow cytometry was performed on an LSR Fortessa instrument (BD). Viable cells were determined with live/dead cell marker (LIVE/DEAD^® Fixable Near-IR; Life Technologies, Life Technologies, Bleiswijk, The Netherlands). Transduction efficiency via associated CAR expression was measured with an APC-conjugated antibody towards low-affinity nerve growth factor (LNGFR CD271), 4-1BBL (CD137L) (Biolegend, London, UK), or with F(ab’)2-Goat anti-Mouse (eBioscience, Bleiswijk, The Netherlands) in case of the murine-based BCMA sequence. CAR-28z-dsRed was measured in the PE-CF594 channel to detect dsRed. Additional antibodies used for iNKT phenotyping were: CD3, CD4, and CD8 (BD Bioscience, San Jose, CA, USA), Vα24, Vβ11 (Beckman Coulter, Woerden, The Netherlands), PD-1, CD57, CD39, Tim3, LAG3, CD62L (Biolegend, London, UK). In cytotoxicity assays antibodies against CD1d, CD3, CD19, CD38, CD56, and CD138 (BD Bioscience, San Jose, CA, USA) were used. Flow cytometry data were analyzed using FCS Express (Pasadena, CA, USA) V6 software.

Serial dilutions of mock- or CAR-transduced iNKT cells were incubated with target cells for 16–24 h. To distinguish the two cell types, target cells or effector cells were pre-stained with 0.5 µM Violet tracer (Thermo Fisher, Bleiswijk, The Netherlands). After the incubation period, Flow-Count™ Fluorospheres (Beckman Coulter, Woerden, The Netherlands) were added and the cells were harvested and stained for different CD markers (see) to identify different cell subsets. Viable cells were then quantitatively analyzed through Flow-Count-equalized measurements. Percentage cell lysis was calculated as follows and only if the analyzed target cell population contained > 500 viable cells in the untreated samples. % lysis cells = (1 − ((#viable target cells in treated wells/#of beads)/(#viable target cells in untreated wells/#of beads))) × 100%. Section 4.6

CAR iNKT cells were stimulated with relevant target cells for 16 h. The cytokines (IL-2, IL-4, IL-6, IL-10, IL17A, TNF, and IFN-γ) released in the culture supernatants were quantified using a Cytokine Bead Array (CBA) Human Th1/Th2/Th17 cytokine kit (BD, San Jose, CA, USA) according to the manufacturers’ protocol.

Statistical analyses were performed using GraphPad Prism software version 7.0 (GraphPad, San Diego, CA, USA). For normal distributions, parametric student’s t-tests were used. In analyses where multiple groups were compared, either a parametric ANOVA with Bonferroni post hoc test or nonparametric Kruskal–Wallis test were used with subsequent multiple comparison. A p value < 0.05 was considered significant.