Abstract
Human natural killer (NK) cells are cytotoxic effector cells that are increasingly harnessed in cancer immunotherapy. NKG2A/CD94 is an inhibitory receptor on NK cells that has established regulatory functions in the direct interaction with target cells when engaged with its ligand, the non-classical HLA class I molecule HLA-E. Here, we confirmed NKG2A as a checkpoint molecule in primary human NK cells and identified a novel role for NKG2A in maintaining NK cell expansion capacity by dampening both proliferative activity and excessive activation-induced cell death. Maintenance of NK cell expansion capacity might contribute to the preferential accumulation of human NKG2A+ NK cells after hematopoietic cell transplantation and enrichment of functionally impaired NK cells in human cancers. Functional silencing of NKG2A for cancer immunotherapy is highly attractive but will need to consider that this might also lead to a reduced survival by driving activation-induced cell death in targeted NK cells.
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Introduction
Human natural killer (NK) cells have received renewed attention in clinical immuno-oncology, especially for use in adoptive cell therapy1,2, most recently as engineered cytotoxic effector cells carrying chimeric antigen receptors for the treatment of hematologic cancers3. Advantages of targeting NK cells compared to T cells for cancer immunotherapy include their innate antitumor activity and, by demonstrating a remarkable safety profile3,4, their potential as off-the-shelf product. However, adoptive transfer of non-engineered NK cell products or singular targeting of inhibitory receptors on endogenous NK cells by means of antagonistic antibodies have not yet yielded substantial clinical benefit2. Therefore, a better understanding of NK cell biology seems critical to better harness and enhance the antitumor potential of these cytotoxic cells.
The surface molecule NKG2A complexed as a heterodimer with the non-signaling CD94 molecule is an invariant inhibitory NK cell receptor (hereafter referred to as NKG2A)5,6,7. NKG2A has established regulatory functions in the direct interaction of NK cells with target cells, limiting NK cell effector responses like cytotoxicity when engaged with its ligand, the non-classical HLA class I molecule HLA-E5. Importantly, overexpression of HLA-E has been reported in a wide range of human cancers8 and has been associated with worse prognosis in colorectal cancer, non-small cell lung carcinoma and gynecological cancers9,10,11,12,13. Blocking NKG2A or disruption of its ligand on cancer cells has been demonstrated to improve outcome of immunotherapy and thus, NKG2A has been considered an NK cell checkpoint8,14,15,16,17. Furthermore, NKG2A is involved in NK cell education18,19 rendering NKG2A+ NK cells more reactive towards transformed HLA class I negative target cells. Since in humans NKG2A is expressed by around half of blood NK cells20, NKG2A with its low genetic diversity makes it an abundant and attractive target molecule for engineering of NK cells.
Here, we disrupted NKG2A via CRISPR gene editing and expanded engineered NK cells, which is needed to reach large enough numbers for therapeutic infusions. We adopted an ex vivo NK cell expansion protocol that has been used safely in clinical trials3,21, based on a myeloid leukemic cell line expressing membrane bound IL-21 as irradiated feeder cells22. Although expression of NKG2A has been associated with an immature NK cell phenotype that correlates with increased proliferative capacity23, it remained unclear whether NKG2A is directly involved in NK cell expansion. By abrogating NKG2A at the genetic level, we validated the functional involvement of NKG2A in NK cell cytotoxicity and provide evidence suggesting that NKG2A is required to maintain NK cell expansion.
Methods
Primary cells and cell lines
Peripheral blood mononuclear cells (PBMCs) were isolated from healthy donors with density gradient centrifugation (Ficoll Paque Premium, GE Healthcare, 17-5442-03). For the expansion of NKG2A+ and NKG2A− NK cells, PBMCs were first depleted of T cells with anti-CD3 MicroBeads (Miltenyi, 130-050-101) and in a second step separated by using APC-conjugated anti-CD159a (Miltenyi, 130-113-563) and anti-APC MicroBeads (Miltenyi, 130-090-855) according to the manufacturer’s instructions. Primary human NK cells were isolated from PBMCs using the human NK cell Isolation Kit (Miltenyi, 130-092-657) for negative selection of NK cells and the autoMACS® Pro Separator according to manufacturer’s instructions. For expansion of NK cells, irradiated (130 Gy) K562mbIL21 feeder cells (kindly provided by Dr. Dean Lee, Nationwide Children’s Hospital, Columbus, United States) were added at a 1:2 ratio (lymphocyte to feeder cell ratio) on day 0 and at a 1:1 ratio every 7 days. Transformed autologous cells were manufactured from primary human B cells, isolated from PBMCs using anti-CD19 MicroBeads (Miltenyi, 130-050-301) according to the manufacturer’s protocol and infected with Epstein Barr Virus (EBV) B95-8 at an MOI of 0.1 for transformation, to generate lymphoblastoid cell lines (LCLs). Primary human NK cells were cultured in RPMI1640 medium (Gibco) supplemented with 10% fetal calf serum (FCS; Biochrom), 1% penicillin/streptomycin (1% P/S; Gibco) and 200 U/mL recombinant human IL-2 (PeproTech, 200-02). Medium was replaced every 2–3 days. K562 cells were obtained from ATCC. K562 cells, LCLs and K562mbIL21 cells were cultured in RPMI1640 medium supplemented with 10% FCS and 1% P/S and passaged twice per week. Viability of the cells was assessed using 0.4% trypan blue solution (Gibco) at a 1:10 dilution.
Editing of NK cells
The NKG2A knockout (KO) from bulk NKG2A+ NK cells and NKG2A+KIR− NK cells was performed 7 days after start of the expansion using CRISPR gene editing. The KLRC1 targeting crRNA (ACTGCAGAGATGGATAACCA) was designed in-house with CRISPOR24 and purchased from Integrated DNA Technologies (IDT) as was the non-targeting control crRNA, the tracrRNA (IDT, 1072533) and Cas9 (Streptococcus pyogenes) protein (IDT, 1081058). The formation of Cas9 ribonucleoproteins (RNPs) was performed as described by Roth et al.25 0.5 × 106 NK cells were electroporated per well of a Nucleostrip™ with RNPs using the P3 Primary Cell 4D-Nucleofector™ X kit S (Lonza, V4XP-3032) according to the manufacturer’s instructions and pulsed with the code DK-100 using the 4D-Nucleofector™ (Lonza). NKG2A KO efficiency was determined 72 h after electroporation by flow cytometry.
Flow cytometry
For the detection of surface markers cells were stained for 20 min at 4 °C in PBS with the appropriate antibodies. For the detection of intracellular or intranuclear markers after surface staining the cells were fixed with the BD Cytofix/Cytoperm™ Fixation/Permeabilization Kit (BD, 554714) according to the manufacturer’s instructions and stained with the appropriate antibodies for 30 min at 4 °C. For the detection of dead cells, the samples were stained with Zombie Aqua™ (Biolegend, 423101). Samples were acquired on BD LSRFortessa™ Flow Cytometer (BD Biosciences) or BD FACSymphony 5L (BD Biosciences). To evaluate apoptosis, cells were stained with the surface markers first, then washed and stained with Annexin V (IQ products, IQP-120F) according to the manufacturer’s instructions. Cells were defined as apoptotic when being Annexin V positive and negative for the live/dead marker. The data was analyzed using FlowJo software (Tree Star). The following antibodies were used: anti-CD56 (BV650, HCD56, Biolegend, 318344), anti-CD16 (BV605, 3G8, Biolegend, 302040), anti-CD3 (BV711, OKT3, Biolegend, 317328), anti-CD3 (PerCP-Cy5.5, UCHT1, Biolegend, 300430), anti-Ki67 (BV605, 16A8, Biolegend, 652413), anti-CD57 (PE-Dazzle-594, HNK1, Biolegend, 359620), anti-CD159a (FITC, REA110, Miltenyi, 130-113-565), anti-phosphorylated S6 ribosomal protein (PE-Cy7, Cell signaling, 34411S), anti-CD25 (APC-Cy7, BC96, Biolegend, 302614), anti-CD132 (PE, TUGh4, Biolegend, 338606), anti-CD158a,h (APC, EB6B, Beckmann Coulter, A22332), anti-CD158b1/b2,j (APC, GL183, Beckmann Coulter, A22333), anti-CD158e (APC, DX9, R&D, FAB1225A-100), anti-CD159a (PE, Z199, Beckmann Coulter, IM2391U), anti-LILRB1 (PE-Cy7, HP-F1, Invitrogen/eBioscience, 25-5129-42), anti-phospho-STAT5-Y694 (PerCP-eFluor710, SRBCZX, Invitrogen/eBioscience, 46-9010-42), anti-phospho-STAT3-Y705 (PE-Cy7, LUVNKLA, Invitrogen/eBioscience, 25-9033-42), anti-HLA-ABC (APC-Cy7, w6/32, Biolegend, 311426), anti-HLA-E (APC, 3D12, Biolegend, 342606). For staining of pSTAT3 and pSTAT5, cells were fixed with the BD Pharmingen Transcription Factor Phospho Buffer Set (BD, 565575) following the manufacturer’s instructions.
Cytotoxicity assays
For cytotoxicity assays K562 cells or LCLs were labeled with PKH67 green (Sigma, MINI67-1KT) or PKH26 red fluorescent cell linker (Sigma, MINI26-1KT) according to the manufacturer’s protocol. Labeled target cells and primary cells were cocultured at different target:effector ratios (1:1, 1:5, 1:10, 1:20) for 4 h. Viability of the labeled target cells was determined by the addition of TO-PRO™-3 iodide (Invitrogen, T3605) immediately before acquisition.
FACS sort
NK cells were stained for CD3, CD56, NKG2A, KIR2DL1/DS1, KIR2DL2/L3/S2, KIR3DL1 and live/dead as described above. After selection for viable CD3−CD56+ NK cells, subpopulations were sorted based on the expression of NKG2A (CD159a) and/or KIRs (KIR2DL1/DS1 (CD158a,h), KIR2DL2/L3/S2 (CD158b1/b2,j), KIR3DL1 (CD158e)) using a FACSAria III cell sorter with BD FACS Diva Software (BD Biosciences), nozzle size 100 µm. Purity of the populations was confirmed after sorting by flow cytometric analysis.
Statistical analysis
Statistical analysis was performed with GraphPad Prism Version 9.2.0 (283). Number of experimental repeats, donors and specific statistical tests are specified in the corresponding figure legends. p values of less than 0.05 were considered significant.
Ethics statement
All methods were carried out in accordance with relevant guidelines and regulations. Informed consent was obtained from all subjects. The use of blood from adult healthy donors was approved by and performed according to the cantonal ethical committee of Zürich, Switzerland (protocols KEK-StV-Nr. 19/08 and 2019-00837).
Results
Knockout of the NK cell checkpoint NKG2A increases killing of transformed autologous cells
To determine whether the cytotoxic capacity of human NK cells (Fig. S1 for gating strategy) could be increased by knocking out the inhibitory receptor NKG2A, PBMCs were isolated from healthy donors, depleted of T cells by magnetic-activated cell sorting (MACS), then separated by the expression of NKG2A and the NKG2A+ fraction selected (Fig. 1A). A crRNA targeting KLRC1, the gene encoding NKG2A located on chromosome 12 was designed in-house (Fig. S2A). Nucleofection of NKG2A+ cells with Cas9 ribonucleoprotein (RNP) complexes led to an average reduction of NKG2A protein expression by 78% as assessed by surface staining (Fig. 1B and Fig. S2B). Before performing cytotoxicity assays, no significant difference was found in the proportion of NK cells among NKG2A+ and NKG2AKO populations (Fig. 1C) and NKG2A was still significantly reduced on NKG2AKO NK cells after expansion (Fig. 1D and Fig. S2C). To determine the functional impact of the NKG2A knockout on NK cell cytotoxicity, expanded NKG2A+ or NKG2AKO NK cells were co-cultured for 4 h with HLA class I positive autologous Epstein Barr virus transformed B lymphoblastoid cells at different effector to target cell ratios. Addition of NKG2AKO NK cells resulted in significantly greater lysis of target cells than observed with addition NKG2A+ NK cells (Fig. 1E). In contrast, this increased killing capacity of NKG2AKO NK cells compared to NKG2A+ NK cells was not detectable against K562 cells, a myelogenous leukemic cell line that is mostly HLA class I deficient and thus lacks the ligand for NKG2A (Fig. 1F). Together, these results demonstrate at the genetic level that NKG2A functions as a checkpoint molecule in human NK cells with disruption of KLRC1 leading to increased cytotoxicity of engineered NKG2AKO NK cells.
NKG2A− NK cells show a decreased fold expansion in vitro as compared to NKG2A+ NK cells
In separate sets of experiments, NKG2A− NK cells were isolated in parallel to NKG2A+ NK cells (Fig. 2A). After selection by MACS, frequencies of CD3−CD56+ NK cells were not significantly different between the NKG2A+ subpopulation and the NKG2A− subpopulation (Fig. 2B). NKG2A expression on CD3−CD56+ NK cells was > 97% in the NKG2A+ subpopulation and below 50% within NK cells of the NKG2A− subpopulation (Fig. 2C). Furthermore, the percentages of CD56dimCD16+ NK cells among sorted NKG2A+ NK cells and NKG2A− NK cells (Fig. 2D) as well as the percentages of CD56brightCD16− NK cells did not differ significantly between the two NK cell fractions, although CD56brightCD16− NK cells were rare among NKG2A− NK cells (Fig. 2E). In contrast, the proportion of cells with KIR expression was almost threefold higher in NKG2A− NK cells than in NKG2A+ NK cells (Fig. 2F), while there was no significant difference in the expression of the inhibitory receptor LILRB1 (Fig. 2G) or the terminal differentiation marker CD57 (Fig. 2H). Compared to NKG2A+ NK cells, NKG2A− NK cells showed a significantly lower fold bulk expansion over the course of 3 weeks (Fig. 2I, mean difference on day 22: 18.8-fold). Because of low NK cell frequencies in the starting population after MACS enrichment, NK cells were FACS sorted to high purity. Notably, the difference in expansion capacity was maintained in FACS sorted NK cells comparing NK cells after knocking out NKG2A via Cas9 RNPs and NKG2A+ NK cells treated with nontargeting Cas9 RNPs (Fig. S2D). At the end of expansion, both NKG2A+ and NKG2A− MACS enriched subpopulations contained almost exclusively CD3−CD56+ NK cells (Fig. 2J). However, the percentage of NKG2A expression increased to 80% in the NKG2A− subpopulation, whereas it remained close to 100% in the NKG2A+ subpopulation (Fig. 2K). While discrimination between CD56dimCD16+ NK cells and CD56brightCD16− NK cells was no longer possible due to upregulation of CD56 during expansion, the percentage of CD16+ NK cells was similar in both NKG2A+ and NKG2A− NK cell fractions (Fig. 2L). In contrast, KIR expression in NKG2A+ and NKG2A− NK cells showed significant differences after expansion, which was higher in NKG2A− NK cells (Fig. 2M), similar to the differences at baseline (Fig. 2F). Interestingly, the percentage LILRB1+ NK cells and CD57+ NK cells decreased to below 1% in both NKG2A+ and NKG2A− NK cell fractions after expansion (Fig. 2N,O). Thus, NKG2A− NK cells display reduced expansion capacity when stimulated with IL-2 and irradiated myeloid leukemic K562 feeder cells with membrane-bound IL-21 and maintain high KIR expression.
NKG2A− NK cells lacking KIR expression exhibit the lowest expansion capacity
Indeed, aside from NKG2A, killer cell immunoglobulin-like receptors (KIRs) are main regulators of NK cell responsiveness including NK cell education and, like NKG2A interact with HLA class I molecules26. Importantly, expression of both HLA-E and HLA class I on feeder cells is strongly increased upon coculture with NK cells (Fig. S3). Since expanded NKG2A− NK cells upregulated NKG2A (Fig. 2K) but retained KIR expression (Fig. 2M) and to explore whether NK cell expansion is influenced by NKG2A depending on KIRs, NK cells were MACS isolated from PBMCs by negative selection, and four different subpopulations based on the expression of NKG2A and KIRs were sorted using flow cytometry: NKG2A+KIR−, NKG2A+KIR+, NKG2A−KIR+, NKG2A−KIR− (Fig. 3A and Fig. S4A). The proportion of the different subsets varied among individuals, but the frequencies of the individual subpopulations were not significantly different across donors (Fig. 3B). There was no obvious difference in the proportion of CD56dimCD16+ NK cells within the four subsets (Fig. 3C). However, whereas the NKG2A+KIR− cell subset contained more CD56brightCD16− NK cells than the NKG2A−KIR+ cell subset, of note, by comparison, CD56brightCD16− NK cells were at least equally abundant in the NKG2A−KIR− cell subset and were not depleted (Fig. 3D). The intensity of LILRB1 was higher in NK cell subsets lacking NKG2A (Fig. 3E). Notably, CD57+ NK cells were not enriched in the NKG2A−KIR− cell subset (Fig. 3F). The four subsets were then expanded separately over a course of 21 days. Compared to all other subsets, the double negative NKG2A−KIR− NK cell subset showed the lowest capacity of bulk expansion (Fig. 3G) with log-fold differences at day 21 compared to the NKG2A+KIR− subset (mean difference: 276.7-fold), the NKG2A+KIR+ subset (mean difference: 211.1-fold) and the NKG2A−KIR+ subset (mean difference: 311.5-fold). Likewise, expansion capacity with fold-expansion corresponding to initially sorted phenotype showed a similar deficit in the NKG2A−KIR− NK cell subset (Fig. S5A). No significant differences in LILRB1 intensity at day 13 (Fig. 3H) or day 20 (Fig. 3I) were observed between expanding NK cell subsets after sort, although intensity tended to be higher in NK cell subsets lacking NKG2A. Together, since expansion capacity of sorted NK cell subsets lacking NKG2A differed according to expression of KIR and NK cell subsets with NKG2A expression maintained robust expansion, these data suggest a role for NKG2A and KIR in sustaining expansion capacity of NK cells.
High frequency of CD57 expression does not mark NK cell subsets with diminished expansion capacity
CD57 is an established marker of a terminally differentiated subset of NK cells thought to harbor decreased proliferative potential23,27,28, however, heterogeneity within this subset has recently been described29. Expression of CD57 at steady state before the start of the expansion was highest on NKG2A+KIR+ NK cells and lower on double negative NKG2A−KIR− NK cells compared to NKG2A−KIR+ NK cells (Fig. 3F and Fig. S4B). However, on day 13 (Fig. 3J and Fig. S4C) and day 20 (Fig. 3K and Fig. S4D) of expansion after the sort, CD57 expression within populations gradually decreased in all subsets with no significant differences between the individual subsets. Thus, even though the terminal differentiation marker CD57 was initially expressed at equal or higher frequencies (highest on NKG2A−KIR+ NK cells that showed the greatest fold expansion, Fig. 3G), all of these NK cell subsets displayed log-fold higher expansion capacity compared to the NKG2A−KIR− NK cell subset that initially contained a majority of CD57− cells. Therefore, at least in the context of the expansion protocol used herein, expression of CD57 per se seems not to predict proliferative potential of a given NK cell population.
Expansion capacity of NKG2A+KIR− NK cells directly depends on NKG2A
To further investigate whether NKG2A is only a surrogate marker for more immature NK cells that possess increased proliferative potential or plays a direct role in KIR-independent expansion capacity of NK cells and because NKG2A−KIR− NK cells had the lowest expansion (Fig. 3G), NKG2A was knocked out using Cas9 RNPs in sorted NKG2A+KIR− NK cells (Fig. 4A), a subset that otherwise exhibits high expansion capacity (Fig. 3G). After the knockout, expression of NKG2A was efficiently abrogated in NKG2AKOKIR− NK cells (Fig. 4B). When comparing the expansion capacity to parental NKG2A+KIR− NK cells, the fold expansion of the NKG2AKOKIR− population was significantly lower than that of NKG2A+KIR− NK cells by day 7 (Fig. 4C, mean difference = 5.6) and day 14 (Fig. 4D, mean difference = 51.3) after knockout, closely resembling reduced expansion of NKG2A−KIR− NK cells. Expansion capacity in NKG2AKOKIR− and NKG2A−KIR− NK cells with fold expansion corresponding to engineered or initially sorted phenotype also showed similar deficits (Fig. S5B,C). NKG2A expression remained at reduced levels in NKG2AKOKIR− NK cells (Fig. 4E) but increased in NKG2A−KIR− NK cells (Fig. 4F), while in the NKG2A+KIR− population it was high and even increased slightly over the course of the expansion (Fig. 4G). Intensity of LILRB1 was not different on day 6 (Fig. 4H and Fig. S6A), but higher in both expanding NKG2AKOKIR− and NKG2A−KIR− NK cells on day 13 after knockout compared to NKG2A+KIR− NK cells (Fig. 4I) and mock edited NKG2A+KIR− NK cells (Fig. S6B). No significant differences were found in CD57 expression between expanding NKG2A+KIR−, NKG2AKOKIR− and NKG2A−KIR− NK cells on day 6 (Fig. 4J) and day 13 (Fig. 4K) after knockout or expanding mock edited NKG2A+KIR− NK cells (Fig. S6C,D). Taken together, these results suggest a direct and KIR-independent role for the inhibitory receptor NKG2A in maintaining the expansion capacity of NK cells.
Proliferation of NKG2AKOKIR− NK cells cannot compensate for higher apoptosis rate
To assess whether a difference in the expression of receptors for interleukins that are associated with the expansion of NK cells could be involved in the reduced expansion capacity of NKG2AKOKIR− NK cells, we investigated expression of unique and common interleukin receptor subunits by flow cytometry. An important interleukin for the activation and expansion of NK cells is interleukin-2 (IL-2), which we used in the expansion protocol alongside stimulation with membrane-bound IL-213,21,22. However, only low levels of the IL-2 receptor alpha chain (CD25) could be detected with no significant differences between expanding NKG2A+KIR− NK cells and NKG2AKOKIR− NK cells on day 6 (Fig. S7A) and day 13 (Fig. S7B) after knockout, but trending higher in NKG2AKOKIR− NK cells. Similarly, on day 6, no significant differences were observed for the expression of the common cytokine receptor gamma chain (CD132) which is the receptor subunit for multiple interleukins including IL-2, IL-15 and IL-21 (Fig. S7C). However, there was a slight decrease in CD132 intensity on expanding NKG2AKOKIR− NK cells by day 13 after knockout (Fig. S7D). Staining for the IL-21 receptor did not reveal distinct expression in NKG2A+KIR− NK cells from NKG2AKOKIR− NK cells (data not shown). To explore signaling downstream of receptor engagement upon IL-2 binding, phosphorylation of STAT5 was compared in expanding NKG2A+KIR− NK cells and NKG2AKOKIR− NK cells, showing a slight decrease in NKG2AKOKIR− NK cells at day 6 after knockout (Fig. S7E), but no differences at day 13 (Fig. S7F). Likewise, as a readout for signaling downstream of receptor engagement upon IL-21 binding, phosphorylation of STAT3 did not reveal any obvious differences in expanding NKG2A+KIR− NK cells and NKG2AKOKIR− NK cells (Fig. S7G,H). Therefore, these data indicate that differential expression of receptors for interleukins and associated downstream signaling relevant to NK cell activation and survival is not critically involved in the different expansion capacity of NKG2A+KIR− NK cells versus NKG2AKOKIR− cells.
The mTOR signaling pathway directs cellular growth and maintains cellular homeostasis30. The phosphorylated ribosomal protein S6 (p-S6) is a downstream target of mTORC1 and thus serves as a marker of mTORC1 activity31,32. To assess mTORC1 activity, expression of p-S6 was measured, but p-S6 was not differentially expressed in NKG2A+KIR− NK cells compared to NKG2AKOKIR− cells neither on day 6 (Fig. S7I) nor day 13 (Fig. S7J) of expansion. These data suggest that differences in mTORC1 activity are not the primary cause of the reduced expansion capacity of NKG2AKOKIR− cells.
When measuring proliferation and apoptosis after NKG2A knockout (Fig. 5A), the expression of the proliferation marker Ki-67 in NKG2AKOKIR− NK cells trended to be increased but not significantly higher than in NKG2A+KIR− cells NK on day 6 after knockout (Fig. 5B). Apoptotic cells were detected using Annexin V33 (Fig. S8A), and interestingly NKG2AKOKIR− NK cells showed a more than three-fold higher frequency of Annexin V binding as compared to NKG2A+KIR− NK cells (Fig. 5C). However, when comparing the ratio of proliferation to apoptosis, the proliferation rate of NKG2AKOKIR− NK cells could not compensate for the drastically higher apoptosis and thus the expansion index, i.e., the Ki-67+/Annexin V+ ratio, was significantly decreased for NKG2AKOKIR− NK cells (Fig. 5D and Fig. S8D). These results indicate that NKG2A buffers both proliferative activity and excessive activation-induced cell death to maintain expansion capacity of human NK cells.
Discussion
Our data demonstrate that primary human NK cells can be gene edited to efficiently abrogate NKG2A protein expression and confirm at the genetic level that NKG2A functions as an NK cell checkpoint molecule. A function of NKG2A in NK cell biology beyond its role in inhibiting immediate effector function and mediating NK cell education, however, has remained largely unexplored. Recently, NKG2A has been demonstrated to inhibit short-term NK cell proliferation34. In contrast, we here show that during expansion over a period of several weeks, NKG2A is essential for maintaining the expansion capacity of human NK cells. Our data suggest that NKG2A dependent expansion is achieved through regulation of proliferative activity and apoptosis to avoid activation-induced cell death. The results by Anton et al.34 and our current work do not need to be mutually exclusive, however, since the observed inhibition of proliferative activity is likely to precede the impact of activation-induced cell death on expansion. Thus, the NKG2A dependent reduction in proliferative activity in the initial phase of expansion described by Anton et al. may initially mask the increased expansion capacity we observed, which is also regulated by NKG2A but only becomes apparent later during expansion. We did not identify a major contribution of differences in IL-2 or IL-21 signal integration mediated by NKG2A in regulating NK cell expansion capacity. While other work has described downregulation of the IL-2 receptor subunit CD25 after abrogation of NKG2A surface expression8, we, like others35, only found low expression of CD25 without evidence of further decrease after genetic disruption of NKG2A. Furthermore, we found that the frequency of CD57 expression, a marker of terminal NK cell differentiation23,27,28, was unable to predict expansion capacity and decreased in expanding NKG2A+ NK cells. These data suggest that NKG2A can shield NK cells from apoptotic activation-induced cell death and terminal differentiation, leading to the depletion of CD57+ NK cells.
The myeloid K562 cells used in the expansion protocol may partially reflect the physiological interaction of NK cells and myeloid cells, which is particularly relevant in the tumor microenvironment36,37, providing signals like cytokines and ligands, e.g., the NKp30 ligand for NK cell activation38,39,40. Interestingly, reconstitution of NK cells in patients after hematopoietic cell transplantation (HCT) is dominated by NKG2A+ NK cells with reduced KIR expression41,42,43. Beside a transition from precursors, the role of NKG2A we identified in maintaining NK cell expansion capacity could help explain the overrepresentation of NKG2A+ over NKG2A− NK cell populations with an expansion advantage mediated by NKG2A in the post-HCT setting rich in cytokines that provide stimulatory signaling44,45. Likewise, NKG2A+ NK cells are preferentially found in the myeloid cell-rich46,47 tumor microenvironment of human cancers48,49,50, where functionally, intratumoral NK cells are generally described as hyporesponsive51.
While our work identified a key role for NKG2A in maintaining NK cell expansion, although not directly targeted, we also found that expression of KIRs is essential for expansion. Indeed, NKG2A−KIR− NK cells displayed the lowest expansion capacity although not being depleted of the immature CD56brightCD16− NK cell subset52, but having higher expression of the inhibitory receptor LILRB1 instead, that like NKG2A and KIR also interacts with HLA class I molecules53. Thus, studying the impact of KIR and LILRB1 on regulating NK cell expansion is warranted. Together, it is possible that inhibitory signaling is required more generally to avoid activation-induced cell death and thus sustain expansion of NK cells confronted with excessive stimulatory signals. Ultimately, this may represent part of the mechanisms for maintaining self-tolerance, by which the expansion of NK cells lacking essential inhibitory receptors like NKG2A for self-HLA class I is reduced to protect against autoimmunity and tissue damage in inflammatory settings. On the other hand, cancer may exploit this mechanism to evade NK cell mediated immune surveillance by upregulation of HLA-E9,10,11,12,13,40, leading to preferential expansion of NKG2A+ NK cells and thus depletion of potentially more responsive, uninhibited NK cells lacking NKG2A. This should be considered in cancer immunotherapy approaches targeting NKG2A on NK cells because this could drive activation-induced cell death leading to reduced survival of these cells, if not counter-balanced by signaling from inhibitory receptors like KIRs.
Data availability
The data generated in this study are available upon request from the corresponding author.
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Funding
This research was supported by Cancer Research Switzerland (KFS-4371-02-2018 to O. Chijioke). M. Kaulfuss was supported by a research fellowship from the German Research Foundation (project number 415801544). The study also benefitted from the CRPP ImmunoCure of the University of Zürich.
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M.K. and J.M. performed and analyzed experiments. A.F. helped with initial experiments. J.v.B helped with gene editing. M.K. and O.C. analyzed data and wrote the main manuscript text, with editorial input from all coauthors. C.M. cosupervised this work. O.C. supervised and coordinated all aspects of this work. All authors reviewed the manuscript.
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Kaulfuss, M., Mietz, J., Fabri, A. et al. The NK cell checkpoint NKG2A maintains expansion capacity of human NK cells. Sci Rep 13, 10555 (2023). https://doi.org/10.1038/s41598-023-37779-6
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DOI: https://doi.org/10.1038/s41598-023-37779-6
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