The human renal proximal TEC line (HK-2) was purchased from American Type Culture Collection (Manassas, VA, USA) and cultured in Dulbecco's modified Eagle medium (Invitrogen, Carlsbad, CA, USA) with non-essential amino acids, 0.05 mg/ml bovine pituitary extract, 50 ng/ml human recombinant epidermal growth factor, 100 U/ml penicillin, 100 µg/ml streptomycin and 10% fetal bovine serum (FBS) under a 5% CO₂ atmosphere at 37°C. NK92-MI cells were cultured in α-modification of Eagle's Minimum Essential medium supplemented with 2 mM L-glutamine, 0.2 mM inositol, 20 mM folic acid, 12.5% FBS and 12.5% horse serum. Anti-NKG2D antibodies (#FAB139A) and anti-NKG2D ligand antibodies (#MAB13001, #MAB1380, #MAB1298, #MAB1517) were purchased from R&D Systems (Minneapolis, MN, USA).

Peripheral blood lymphocytes (PBLs) from buffy coats of healthy donors were prepared by Ficoll-Hypaque density gradient centrifugation (GE Healthcare, Little Chalfont, UK). The study was approved by the Institutional Bioethics Review Board at the Medical College of Inje University (Busan, Korea), and all the donors provided informed written consent prior to their participation in the study. Cells were stimulated with human interleukin (IL)-2 (500 U/ml; a quantity commonly used to stimulate primary NK cells) for cytokine production (32).

Surface antigen fluorescence-activated cell sorting (FACS) analysis was performed to detect NKG2D ligands on HK-2 cells. Cells were washed twice with ice-cold phosphate-buffered saline (PBS), and incubated with mouse anti-MICA antibody (#MAB13001) or anti-human ULBP monoclonal antibodies [anti-ULBP1 (#MAB1380), anti-ULBP2 (#MAB1298) and anti-ULBP3 (#MAB1517); R&D Systems} for 30 min on ice. After 2 washes, cells were incubated with an appropriate fluorescein isothiocyanate (FITC)-conjugated secondary antibody diluted in PBS for 30 min on ice and analyzed using a FACSCalibur flow cytometer.

Intracellular FACS analysis was performed to detect intracellular NKG2D ligand protein levels in HK-2 cells. Cells were washed twice with ice-cold PBS containing 0.05% bovine serum albumin (BSA) and 0.02% sodium azide (PBS-BSA), and were fixed in 2% paraformaldehyde in PBS for 15 min on ice. The cells were subsequently washed once in cold PBS-BSA, and resuspended in PBS containing 0.1% saponin and 0.05% sodium azide (permeabilization buffer) for 15 min, followed by incubation with anti-MICA and anti-ULBPs antibodies for 30 min on ice. Following 2 washes, cells were incubated with an appropriate FITC-conjugated secondary antibody in permeabilization buffer for 30 min on ice. Samples were analyzed using a FACSCalibur flow cytometer (BD Biosciences, Franklin. Lakes, NJ, USA).

RNA was isolated from HK-2 cells using RNeasy (Qiagen, Valencia, CA, USA), according to the manufacturer's instructions, and reverse transcribed into cDNA. The following primers were used for PCR amplification: TGF-β sense, 5′-GCC CTG GAC ACC AAC TAT TGC-3′ and antisense, 5′-GCT GCA CTT GCA GGA GCG CAC-3′; and MICA sense, 5′-TGC TTC TGG CTG GCA TCT TC-3′ and antisense, 5′-TAG TTC CTG CAG GCA GTC TG-3′. Cycling conditions for MICA and TGF-β were 1 min at 94°C, 1 min at 60°C and 1 min at 72°C for 32 cycles. β-actin was amplified as a control using a sense, 5′-GTG GGG CGC CCC AGG CAC CA-3′ and antisense primer, 5′-CTC CTT AAT GTC ACG CAC GAT TTC-3′; in the RT-PCR experiments. Cycling conditions for β-actin were 1 min at 94°C, 1 min at 55°C and 1 min at 72°C for 25 cycles. The PCR products were analyzed by ethidium bromide-stained 1.2% agarose gel electrophoresis

TGF-β expression was blocked by siRNA. Cell transfection was performed using Lipofectamine 2000 (Invitrogen) for 48 h. The siRNA sequences were as follows: TGF-β siRNA sense, 5′-CAG AGU ACA CAC AGC AUA U-dTdT-3′ and antisense, 5′-AUA UGC UGU GUG UAC UCU G-dTdT-3′; and non-related control siRNA (GL3-luciferase) for TGF-β siRNA transfection sense, 5′-AGG GAU ACA UAC GUG CAC G-dTdT-3′ and antisense, 5′-CGU GCA CGU AUG UAU CCC U-dTdT-3′. RT-PCR was performed to determine the level of silencing following transfection.

NK cell cytotoxic activity was determined by calcein-AM assays, as previously described (33). Briefly, target cells were washed twice with PBS and incubated with 5 mM calcein-AM (Molecular Probes, Eugene, OR, USA) in serum-free RPMI-1640 medium for 10 min at 37°C. Labeled target cells were distributed into U-bottom microtiter plates at a concentration of 2×10⁴ cells/well. Effector cells (PBL or the NK92MI NK cell line) were added at various effector to target ratios in quadruplicate. Target cells (HK-2 cells) in complete RPMI-1640 medium alone were used to determine spontaneous calcein-AM retention. Maximal lysis was determined by solubilizing 3 wells of the target cells in lysis buffer (0.1% Triton X-100). After incubation for 5 h, the assays were analyzed using a fluorescence reader. The percentage of specific cytotoxicity was calculated as follows: % specific release = [(retention of experimental well - retention of spontaneous well)/(retention of maximal lysis well - retention of spontaneous well)] ×100.

The concentrations of TGF-β and soluble MICA in culture supernatants were determined using human TGF-β and MICA ELISA kits (R&D Systems) following the manufacturer's instructions. Briefly, cell culture supernatant was added to microplate wells coated with either anti-TGF-β or anti-MICA antibody. After incubation with the cultured supernatant for 2 h, the wells were washed 4 times with washing buffer. Horseradish peroxidase-conjugated detection antibodies were added for 2 h, followed by the addition of the substrate solution for 30 min. Samples were read at 450 nm with an ELISA reader (Molecular Devices, Sunnyvale, CA, USA).

Statistical analysis was performed using GraphPad Prism (GraphPad Software, La Jolla, CA, USA). Student's t-test was used for assessing statistical significance for comparisons between two groups. Intergroup differences were assessed by one-way analysis of variance. P<0.05 was considered to indicate a statistically significant difference.

To evaluate NKG2D ligand expression in human renal proximal tubular epithelial (HK-2) cells, surface and intracellular expression of MICA and ULBP was analyzed. HK-2 cells expressed MICA, ULBP2 and ULBP3, but not ULBP1, on the cell surface. However, all these NKG2D ligands were detected intracellularly (Fig. 1A).

Several studies have reported TGF-β expression in renal proximal TECs (30), and in general, TGF-β has been shown to inhibit NK cell function via downregulation of NKG2D (24–25,34). To investigate the association between expression of NKG2D ligands and TGF-β in renal IRI, NKG2D ligand expression was measured using FACS analysis following treatment with exogenous TGF-β. Treatment with exogenous TGF-β induced the intracellular expression of MICA and ULBP2 in HK-2 cells; however, it did not induce the intracellular expression of other NKG2D ligands (Fig. 1B). Notably, treatment with TGF-β induced MICA surface expression in HK-2 cells, but induced little or no surface expression of ULBP2.

To confirm these findings, the effects of different concentrations of TGF-β on MICA expression in HK-2 cells were evaluated. TGF-β treatment significantly induced surface and intracellular expressions of MICA in a dose-dependent manner (Fig. 2A). Time-course experiments revealed that 48 h of incubation in the presence of TGF-β was optimal for the maximum induction of intracellular and surface expression of MICA in HK-2 cells (Fig. 2B). These results show that MICA expression increases in HK-2 cells following treatment with TGF-β in a dose- and time-dependent manner. Taken together, these data suggest that TGF-β is a regulator of MICA expression in human TECs.

Several studies in various cell types have revealed that NKG2D ligand expression is primarily controlled by the ATM and ATR protein kinase pathway (35,36). Kirshner et al (37) reported that TGF-β is involved in the ATM/ATR kinase pathway in response to genotoxic stress. To determine which pathway mediates the upregulation of MICA in HK-2 cells, an ATM/ATR kinase inhibitor was tested for its ability to block MICA expression following treatment with TGF-β. The ATM/ATR kinase inhibitor caffeine significantly blocked the expression of MICA induced by TGF-β (Fig. 3A). Additionally, ATM/ATR kinase activity and ATR kinase phosphorylation were markedly increased in HK-2 cells following treatment with TGF-β (Fig. 3B). These results suggest that the ATM/ATR pathway has a critical role in controlling the expression of MICA following TGF-β treatment.

To examine whether membrane-bound MICA expression on HK-2 cells influences cytotoxic function in primary NK cells, the cytotoxicity of PBL, isolated from healthy individuals, against HK-2 cells treated with or without TGF-β was evaluated. IL-2-activated effector cells exhibited significantly higher cytotoxicity against HK-2 cells treated with TGF-β compared with the naïve HK-2 cells (Fig. 4A). Subsequently, whether the observed TGF-β-mediated increase in the susceptibility of HK-2 cells to NK cell cytotoxicity directly involves NKG2D was examined. Neutralizing NKG2D with an anti-NKG2D antibody moderately reduced PBL cytotoxicity against TGF-β-treated HK-2 target cells, while treatment with anti-Fas or isotype control antibodies did not (Fig. 4B). These results suggest that TGF-β enhances NK cell cytotoxicity via an NKG2D-mediated pathway.

As MICA is expressed on the cell surface and released by metalloproteases (38,39), the effect of metalloprotease treatment on TGF-β-induced MICA surface expression was evaluated. ELISA analysis of culture supernatants revealed that the shedding of MICA from TGF-β-treated HK-2 cells was significantly enhanced at 72 h compared to that of the cells treated with media alone (Fig. 4C).

To determine the function of soluble MICA released from TGF-β-treated HK-2 cells, whether co-culture of TGF-β-treated HK-2 cells and NK cells affected the cytotoxicity of NK cells was evaluated using a Transwell system. Co-cultivation of NK cells with TGF-β-treated HK-2 cells resulted in significantly lower NK cell cytotoxicity compared with the TGF-β-untreated HK-2 cells (Fig. 4D). Additionally, NK cells co-cultured with TGF-β-treated HK-2 cells, in contrast to the NK cells that were not co-cultured, showed reduced NK activity against TGF-β-untreated HK-2 target cells. These results suggest that soluble MICA released from TGF-β-treated HK-2 cells can reduce NK cell cytotoxicity via downregulation of NKG2D expression.

To confirm that the secreted soluble MICA observed in the HK-2 cell culture supernatant was due to hypoxia-induced TGF-β expression, a hypoxia-mimetic chemical [200 µM cobalt chloride (CoCl₂)] was added to the HK-2 cells (40). CoCl₂ enhanced expression of TGF-β and MICA, as well as the release of soluble MICA from HK-2 cells (Fig. 5A and B). To elucidate the direct effect of TGF-β on soluble MICA secretion, TGF-β gene silencing was performed using siRNA transfection (Fig. 5C) and confirmed by RT-PCR. Soluble MICA secretion corresponded with the level of TGF-β silencing and was lower in TGF-β siRNA transfected cells compared to the control and negative control siRNA-transfected cells (Fig. 5D). This result indicated that hypoxia-enhanced TGF-β expression causes an increase in soluble MICA secretion, which in turn directly regulates IRI.