The five-gene knockout cell line (5GKO, GGTA1/CMAH/β4galNT2/SLA-I α chain/β-2 microglobulin) was generated from ipLDEC, as previously described (36). The 5GKO cell line served as the parental cell line to express HLA-E and/or HLA-G molecules.

HLA-G is a heterodimer protein consisting of a heavy chain and β-2 microglobulin (B2M) subunits encoded by two genes located on different chromosomes. A single chain gene was designed by linking the HLA-G heavy chain (NCBI reference number: NM_001363567.2) and B2M (NCBI reference number: NM_004048.4) genes with self-cleaving peptide P2A DNA fragment, synthesized by Integrated DNA Technologies (IDT, Coralville, IA), and inserted downstream of the CMV promoter in an expression vector derived from pEGFP-N1, which had EGFP gene removed ( Figure 1A ). This recombinant plasmid was delivered into 5GKO ipLDEC by electroporation using the Neon Transfection System (Thermo Fisher Scientific, Waltham, MA). The transfected cells were cultured in selective media containing G418 at 200 ng/mL for 10 days. HLA-G expression was verified by flow cytometry using PE-conjugated mouse anti-HLA-G antibody (Clone 87G, BioLegend, San Diego, CA). 5GKO cells were used as a control ( Figure 1B ). 5GKO.HLA-G cells were isolated by a BD FACSAria Fusion cell sorter (BD Biosciences, San Jose, CA) ( Figure 1C ).

The HLA-E molecule is a trimeric complex, consisting of a heavy chain, B2M, and a signal peptide derived from other HLA class I molecules (30). To ensure HLA-E expression in porcine cells, the HLA-E heavy chain gene (HLA-E*010301 allele, NCBI reference number: NM_005516.6) was modified by replacing its original signal peptide DNA sequence with HLA-B*07:02 signal peptide (VMAPRTVLL, NCBI Reference Sequence: NM_005514.8) DNA sequence, then linked to B2M gene with P2A DNA fragment. This single-chain HLA-E gene was synthesized by IDT and subsequently cloned to the downstream of the CMV promoter in an expression vector derived from pEGFP-N1 ( Figure 1A ). This plasmid was delivered into 5GKO and 5GKO.HLA-G cells by electroporation, respectively. The transfected cells were cultured in selective media containing G418 at 200 ng/mL for 10 days. HLA-E expression was confirmed by flow cytometry using APC-conjugated mouse anti-HLA-E antibody (Clone 3D12, BioLegend). 5GKO.HLA-E and 5GKO.HLA-E.HLA-G cells were isolated by a BD FACSAria Fusion cell sorter (BD Biosciences) using APC-conjugated mouse anti-HLA-E antibody and PE-conjugated mouse anti-HLA-G antibody (BioLegend) ( Figures 1D, E ). Both HLA-E antibody and HLA-G antibody are specific. Cross-reactivity of HLA-E antibody to HLA-G molecules or HLA-G antibody to HLA-E molecules has not been observed.

HLA-E and HLA-G surface expression on 5GKO cells were examined four times for three weeks after flow sorting. 5GKO.HLA-E, 5GKO.HLA-G, and 5GKO.HLA-E.HLA-G were stained with APC-conjugated mouse anti-HLA-E antibody and PE-conjugated mouse anti-HLA-G antibody (BioLegend), as described above. HLA-E and HLA-G expression were measured by the percentage of positive cells as well as the mean fluorescence of intensity (MFI). The percentage of HLA-E or HLA-G positive cells was compared between 5GKO.HLA-E and 5GKO.HLA-E.HLA-G cells or between 5GKO.HLA-G and 5GKO.HLA-E.HLA-G cells at each time point. HLA-E MFI was compared between 5GKO.HLA-E and 5GKO.HLA-E.HLA-G cells while HLA-G MFI was compared between 5GKO.HLA-G and 5GKO.HLA-E.HLA-G cells.

HLA-G VL9 peptide (VMAPRTLFL) was synthesized at purity of 95.1% by GenScript Biotech (Piscataway, NJ). 5GKO.HLA-E cells were incubated with HLA-G peptides at final concentrations of 25 µM, 50 µM, and 100 µM in a CO₂ incubator at 37°C overnight. 5GKO.HLA-E cells alone were used as a control. HLA-E expression on pig cells was measured by APC-conjugated mouse anti-HLA-E antibody staining and analyzed by an LSRFortessa flow cytometer (BD Biosciences). Experiments were repeated three times with similar results.

NK cell degranulation assay was performed in a similar fashion as previously described (36, 38). CD107a is a functional marker and widely used for identification of NK cell activity (37, 39, 40). Commercially available buffy coats were acquired from Versiti Indiana Blood Center. Fresh whole blood was drawn from two human donors following the guidelines of the Institutional Review Board (IRB) of Indiana University, IRB#11013. Human peripheral blood mononuclear cells (PBMCs) were isolated from buffy coat and fresh whole blood using Ficoll-Paque Plus (GE-Healthcare, Pittsburgh, PA) and Lymphoprep (STEMCELL Technologies, Vancouver, Canada) gradient centrifugation, respectively, for a total of 5 human donors. PBMCs from 5 donors were cultured in RPMI1640 with 10% FBS, 1% penicillin/streptomycin, and 20 ng/mL recombinant human IL-2 (rhIL-2) (BioLegend) at 37°C in a 5% CO₂ incubator for 5 days. 5GKO, 5GKO.HLA-E, 5GKO.HLA-G, and 5GKO.HLA-E.HLA-G cells were plated at 5 ×10⁴ per well in a Biocoat collagen I-coated 48-well plate (Corning Incorporated, Corning, NY) one day prior to co-culture. PBMCs were added to porcine cells at 5 ×10⁵ per well and co-cultured for 2 hours at 37°C in a CO₂ incubator. Cultured cells were then collected and stained with fixable viability dye eFluor 780 (Thermo Fisher Scientific) and fluorochrome-conjugated antibodies against human CD45, CD3, CD56, and CD107a (BioLegend). Cells were fixed with 2% PFA for 15 minutes at room temperature and subsequently analyzed using an LSRFortessa flow cytometer (BD Biosciences). 70,000 - 80,000 events were acquired in lymphocyte gate. After pre-gating on CD45⁺ live singlets, NK cell degranulation activity was assessed by the percentage of CD107a positive cells in a CD3^-CD56⁺ cell population. Flow data were analyzed using FlowJo v10 software (BD Biosciences). The experiment was repeated three times to obtain technical replicates.

Human antibody binding to porcine endothelial cells was examined, as previously described (36). Briefly, 2×10⁵ porcine cells (5GKO, 5GKO.HLA-E, 5GKO.HLA-G, and 5GKO.HLA-E.HLA-G) were washed and incubated with 25% heat-inactivated human serum in EX-CELL 610-HSF serum-free medium (Sigma, St. Louis, MO) with 0.1% sodium azide for 1 hour at 4°C. Human sera were obtained from patients on the kidney transplant waitlist, 10 sera with high panel reactive antibody (PRA) and 10 sera with low PRA, for a total of 20 samples (n = 20). Each pig cell line was washed three times with EX-CELL 610-HSF serum-free medium and stained with goat anti-human IgG Alexa Fluor 488 or donkey anti-human IgM Alexa Fluor 647 (Jackson ImmunoResearch Laboratories Inc., West Grove, PA) for 30 minutes at 4°C, respectively. Cells were washed, fixed with 2% PFA for 15 minutes at room temperature, and subsequently analyzed using an LSRFortessa flow cytometer (BD Biosciences). Flow data were analyzed using FlowJo v10 software (BD Biosciences). Each pig cell line stained with goat anti-human IgG Alexa Fluor 488 or donkey anti-human IgM Alexa Fluor 647 was used as background and subtracted from each corresponding sera binding group. Human IgG and IgM bindings to pig cells were analyzed by stratification into low PRA and high PRA sera groups. The difference between low PRA and high PRA sera binding to each individual modified cell line was also compared.

Statistical analyses were performed using GraphPad Prism 9 software (GraphPad Software, San Diego, CA). A normality test was used to assess data distribution. An ordinary one-way ANOVA multiple comparisons test with Šídák’s correction was used to analyze the differences among multiple groups. Student’s t-test was used to analyze the differences between the two groups. A p-value less than 0.05 was considered statistically significant.

Three porcine cell lines expressing HLA-E, HLA-G, and co-expressing HLA-E and HLA-G were successfully established ( Figures 1C–E ). Stability of HLA-E and HLA-G molecules on porcine cells was examined. During the three-week culture, HLA-E expression on 5GKO.HLA-E.HLA-G was much more stable compared to HLA-E on 5GKO.HLA-E cells as indicated by the percentage of HLA-E positive cells ( Figure 2A ). In addition, 5GKO.HLA-E.HLA-G cells exhibited significantly higher HLA-E expression than 5GKO.HLA-E cells (p < 0.05) ( Figure 2C ). HLA-G expression was comparable between 5GKO.HLA-G and 5GKO.HLA-E.HLA-G cells ( Figures 2B, D ). These results indicate that HLA-E molecules are stable and more highly expressed on 5GKO.HLA-E.HLA-G cells than on 5GKO.HLA-E cells. All cells were examined by flow cytometry to ensure HLA-E or HLA-G expression prior to being used in the functional assays.

A recent study indicated that HLA class I signal peptide polymorphism influences surface HLA-E expression as well as NKG2A-HLA-E engagement (41). Surface HLA-E is unstable and is rapidly internalized (42). In 5GKO.HLA-E.HLA-G cells, HLA-E can bind to either HLA-B*07:02 VL9 or HLA-G VL9 peptides. In 5GKO.HLA-E cells, HLA-E can only bind HLA-B*07:02 VL9 peptides. To understand the mechanism by which 5GKO.HLA-E.HLA-G cells exhibited much higher HLA-E expression than 5GKO.HLA-E cells, we determined whether HLA-G VL9 peptide could enhance HLA-E expression on 5GKO.HLA-E cells. 5GKO.HLA-E cells were pulsed with HLA-G VL9 peptides at 25 µM, 50 µM, or 100 µM, and incubated overnight. HLA-E surface expression by flow cytometric analysis revealed that exogenous HLA-G VL9 peptides could significantly increase HLA-E expression on 5GKO.HLA-E cells in a dose dependent manner ( Figure 3 ). This result suggests that HLA-G VL9 peptides can stabilize HLA-E molecules and enhance HLA-E expression on 5GKO.HLA-E cells.

Human NK cell response to pig cell stimulation was examined by CD107a expression on NK cells. Our previous study demonstrated that 5GKO cells, like WT and TKO (triple-gene knockout, GGTA1/CMAH/β4galNT2) cells, could activate human NK cell. Despite the elimination of four xenoantigens (aGal, Neu5Gc, Sda, and SLA-I), 5GKO cells maintained the capability to trigger human NK cell degranulation (36). 5GKO cells were used as a control in this study. The gating strategy to identify the NK cell population (CD3^-CD56⁺) was shown in Figure 4A . Representative flow plots showing human NK cell degranulation in response to stimulation by each modified cell line as assessed by the percentage of CD107a positive cells in CD3^-CD56⁺ population were shown in Figure 4B . Ordinary one-way ANOVA multiple comparisons indicated that co-expression of HLA-E and HLA-G on 5GKO cells significantly inhibited CD107a expression on human NK cell compared to 5GKO (p < 0.0001), 5GKO.HLA-E (p < 0.001), and 5GKO.HLA-G (p < 0.01) ( Figure 4C ). Further Student’s t-test indicated that HLA-G expression on 5GKO cells significantly inhibited CD107a expression on NK cells compared to 5GKO cells (p <0.05) while HLA-E expression on 5GKO failed to inhibit CD107a expression on NK cells compared to 5GKO cells (p = 0.1853).

To test whether non-classical HLA class I molecules HLA-E and HLA-G could react to pre-existing HLA class I antibodies, human antibody (IgG and IgM) binding to 5GKO, 5GKO.HLA-E, 5GKO.HLA-G, and 5GKO.HLA-E.HLA-G cells was examined. A total of twenty human sera samples including ten high PRA sera and ten low PRA sera from the patients on the kidney transplant waitlist were used in this experiment. No statistically significant differences in human IgG or IgM binding among groups were observed: IgG with low PRA sera (p = 0.66), IgG with high PRA sera (p = 0.88), IgM with low PRA sera (p = 0.88), and IgM with high PRA sera (p = 0.75) ( Figures 5A–D ). No statistically significant difference was observed among groups in human IgG or IgM binding with the combination of the high PRA and low PRA sera (data not shown). In addition, there were no significant differences between low PRA sera and high PRA sera in IgG binding to 5GKO (p = 0.65), 5GKO.HLA-E (p = 0.67), 5GKO.HLA-G (p = 0.56), 5GKO.HLA-E.HLA-G (p = 0.53) ( Figure 5E ) as well as IgM binding to 5GKO (p = 0.48), 5GKO.HLA-E (p = 0.37), 5GKO.HLA-G (p = 0.28), 5GKO.HLA-E.HLA-G (p = 0.43) ( Figure 5F ). These results indicate that HLA-E and HLA-G on porcine cells do not react to existing antibodies in human sera, even from highly sensitized individuals.