Peripheral blood mononuclear cells (PBMCs) were isolated from blood bank donor buffy coats using a Ficoll-Paque gradient (Cytiva, Marlborough, MA) and frozen in 10% DMSO (ThermoFisher, Waltham, MA) in fetal bovine serum (FBS) at -80° C (45). PBMCs were thawed and washed twice using growth media [RPMI 1640 supplemented with 10% FBS, 3 mM L-glutamine, and 100 U/ml penicillin/streptomycin (Gibco, Waltham, MA)] and cultured overnight at 37°C, 5% CO₂ and 100% relative humidity. Naïve CD4⁺ T cells were sorted using the human Naïve CD4⁺ T cell Isolation Kit II and LS MACS sorting columns (Miltenyi Biotec, Auburn, CA) following the manufacturer’s protocol. Naïve CD4⁺ T cells were then activated and differentiated by plating at a density of 2 x 10⁵ cells in 100 ul (2x10⁶/ml) per well on coated anti-CD3 (5 μg/ml; catalog # 16-0037-81; ThermoFisher) 96 well flat-bottom plates (Costar, Washington DC, MD) in the presence of soluble anti-CD28 (2.5 μg/ml; catalog # 16-0289-81; ThermoFisher) and IL-12 (25 ng/ml; catalog #573002; Biolegend, San Diego, CA) for 3 days in 37°C incubators with 5% CO₂ with and without 50 mM ethanol. IL-12 was added to growth media (ThermoFisher) to promote both Th1 and Treg differentiation (DIFF). There was no difference in promotion of FOXP3 expression with either IL-12 or TGF-beta and IL-2 stimulated CD4⁺ T cells (Supplementary Figure 1). Growth media with no IL-12, was referred to as control media (Act). Naïve CD4⁺ T cells that were not activated and differentiated were plated (density of 2x10⁶/ml per well) in growth media without anti-CD3 and anti-CD28. Water pans containing 75 mM ethanol were changed daily to maintain the 50 mM ethanol concentration in the incubator atmosphere as previously described (26). Both 25 mM and 50 mM ethanol were used in preliminary studies, but 25 mM had no significant effect on CD4⁺ T cell differentiation (data not shown), hence all subsequent experiments were performed with 50 mM. Experimental groups for this study are defined as:

CD4⁺ T cells were immunostained with antibodies purchased from Biolegend unless otherwise specified using the following panel (CD4⁺ differentiation panel): CD4-APC (clone: A161A1), CD45RA-BV570 (clone: HI100), CD38-AF700 (clone: HIT2), CD25-BV650 (clone: BC96), CD3-PE-Cy7 (clone: OKT3), CD28-BV605 (clone: CD28.2), FOXP3-PE-CY5 (clone: PCH101) (ThermoFisher, MA, USA), Tbet-PE (clone: 4B10), GATA3-BV421 (clone: 16E10A23), RORγt -PE-CF594 (clone: Q31-378) (BD Biosciences, Franklin Lake, NJ), Live/Dead – eFluor780 (Invitrogen, Waltham, MA). The staining was performed in two steps. The gating strategy for the CD4 differentiation panel is shown as Supplementary Figure 2. Cells were incubated with antibodies (1 μg) targeting CD4, CD45RA, CD38, CD25, and Live/Dead at 4°C for 30 minutes. Cells were then fixed for 30 minutes at room temperature in the dark using the Foxp3/Transcription Factor Staining Buffer Set (catalog #: 00-5523-00; ThermoFisher) according to the manufacturer’s protocol. Following permeabilization, cells were stained with antibodies targeting CD3, CD28, FOXP3, Tbet, GATA3, and RORγt at 4°C overnight for 16-18 hours. GLUT1 expression was assessed using a separate panel, and included CD3, CD4, Tbet, and FOXP3 from the CD4⁺ differentiation panel. GLUT1 (R&D Systems; clone: MAB1418) was conjugated with FITC in the laboratory using the Lighting-Link FITC conjugation kit (catalog #: 707-0010; Novus Biologicals, CO, USA). Samples were analyzed using an 18-color BD LSRII flow cytometer and FACSDiva software (ver. 8.0.1, Becton, Dickinson, Franklin Lakes, NJ). Flow cytometry gates were defined based on fluorescence minus one (FMO) controls.

The differentiated CD4⁺ T cells were sorted to Tbet- and FOXP3-enriched CD4⁺ T cell subsets using the human CD4⁺CD25⁺ regulatory T cell isolation kit (catalog #: 130-091-301; Miltenyi Biotec, Auburn, CA). After sorting, flow cytometry, using the CD4 Differentiation Panel, confirmed that 29% of CD4⁺CD25⁺ T cells expressed FOXP3 and 21% expressed Tbet. Flow through containing CD4⁺CD25^- CD4⁺ T cells were enriched in Tbet-expressing CD4⁺ T cells (18% Tbet and 4% FOXP3; Supplementary Figure 3). These sorted populations were defined as either CD4+CD25+ “Enriched Treg” or CD4+CD25- “Enriched Th1”.

Mitochondrial oxygen consumption rate (OCR) was measured using a Mito Stress Test (31) and Seahorse XFe96 technology (Agilent Technologies, Santa Clara, CA). Naïve and IL-12-differentiated CD4⁺ T cells were seeded on Cell-Tak (Corning, Corning, NY)-coated 96-well Seahorse plates in triplicate at a density of 3 x 10⁵ cells/well within 200 ul, at a concentration of 1.5 million cells/ml, and maintained under standard cell culture conditions (5% CO₂, 37⁰C). Cells were incubated in XF Assay Medium (pH 7.4) with sodium pyruvate (1 mM), L-glutamine (2 mM), and glucose (10 mM) at 37°C without CO₂ for 1 hr before measuring T cell OCR with an XFe96 Extracellular Flux Analyzer (Agilent Technologies, Santa Clara, CA) according to manufacturer’s instructions. Respiratory parameters were assessed by the sequential addition of oligomycin (1 μM), carbonyl cyanide‐p‐trifluoromethoxyphenylhydrazone (FCCP; 2 μM), and rotenone/antimycin A (0.5 μM). OCR measurements were normalized to cell count obtained by staining nuclei with Hoescht dye (2 μM; ThermoFisher Scientific) and visualizing on a BioTek Cytation 1 cell imaging multi-mode reader (BioTek, Winooski, VT).

A Glycolysis Stress Test (31) was performed in naïve and IL-12-differentiated CD4⁺ T cells seeded as described above. Cells were incubated at 37°C without CO₂ for 1 hr in glucose-free XF Assay Medium (pH 7.4) with L-glutamine (2 mM) before measuring CD4⁺ T cell extracellular acidification rate (ECAR) at baseline and after the sequential addition of glucose (10 mM), oligomycin (1 μM), and 2-deoxyglucose (2-DG; 50 mM). ECAR measurements were normalized to cell count as described for the Mito Stress Test.

T cell mitochondrial content was quantified with MitoTracker Deep Red FM probes (Thermofisher) (46, 47). Naïve and IL-12-differentiated CD4⁺ T cells were incubated in growth media containing MitoTracker Deep Red FM (17 nM) under standard cell culture conditions for one hour. An unstained control sample was simultaneously incubated in growth media without MitoTracker. Cells were pelleted, washed with phosphate-buffered saline (PBS; Gibco) and fixed for flow cytometry using the PerFix-nc Kit (Beckman Coulter, Brea, CA) according to manufacturer instructions. Samples were analyzed on a BD FACSCanto II flow cytometer (Becton, Dickinson and Company). The gating strategy for the Mitotracker Deep Red assay is shown as Supplementary Figure 4. Mean fluorescent intensities (MFI) were calculated using BD FACSDiva software (ver 8.0.1).

Glucose uptake was measured with 2-Deoxy-2-[(7-nitro-2,1,3-benzoxadiazol-4-yl) amino]-D-glucose (2-NBDG) (Sigma-Aldrich, St. Louis USA). Briefly, CD4⁺ T cells were washed with PBS and incubated in glucose-free RPMI 1640 supplemented with 10% FBS, 3 mM L-glutamine, and 100 U/ml penicillin/streptomycin (Gibco, Waltham, MA) for 1 hour. After incubation, 2-NBDG was added to culture wells to a final concentration of 150 μM for 30 minutes at 37°C and 5% CO₂. CD4⁺ T cells were washed twice with PBS and analyzed using the 533 nm wavelength channel on a BD FACSCanto II flow cytometer (Becton, Dickinson and Company). The gating strategy for the 2-NBDG uptake assay is shown as Supplementary Figure 5. Mean fluorescent intensities (MFI) were calculated using BD DIVA software (ver 8.0.1).

Naïve CD4⁺ T cells were activated and allowed to differentiate using the in vitro differentiation protocol above, and on day 2 of the 3-day culture, 2-DG (0.5 mM) was added for 24 h. After incubation with 2-DG, cells were stained and assessed by flow cytometry using the CD4⁺ differentiation panel as described above.

Total RNA was extracted from naïve and IL-12-differentiated CD4⁺ T cells after 3 days in the presence and absence of 50 mM ethanol using the miRNeasy Mini Kit (Qiagen, Valencia, CA) according to manufacturer’s instructions. cDNA was synthesized using the Qiagen RT² First Strand synthesis kit (Qiagen, Valencia, CA) and qPCR performed using custom RT² qPCR profiler arrays (Qiagen: CAPA9632-12:CLAH42284). qPCR reactions were carried out in duplicate using a CFX96 thermal cycler (Bio-Rad, Hercules, CA) with Beta-2-Microglobulin (B2M) as the endogenous control. Data were then analyzed using the 2^-ΔΔCt method. All genes analyzed are summarized in Table 1.

Data were checked for assumption of normality using the Shapiro-Wilk test. The alpha level set for all statistical analysis was a p value < 0.05. CD4⁺ differentiation, glycolysis, MitoTracker, and RT² profiler array data were analyzed using a 2 (differentiation) x 2 (ethanol) analysis of variance (ANOVA) with repeated measures on both factors. 2-DG data were analyzed using a 2 (differentiation) x 2 (ethanol) x 2 (2-DG) ANOVA with repeated measures on all factors. When appropriate, post hoc pairwise comparisons were conducted and p-values adjusted using Tukey’s HSD for 2-way ANOVA and Sidak for 3-way ANOVA. To analyze the effect of IL-12 on CD4⁺ differentiation, and of ethanol on Tbet-FOXP3-expressing CD4⁺ T cells, paired T tests were performed. Paired T tests were also performed to assess the effect of ethanol on CD4⁺ T cell mitochondrial function and to analyze the MitoTracker data within Treg and Th1 CD4⁺ subsets. The Treg OCR-linked proton leak data did not pass normality or lognormality tests and therefore a Wilcoxon test was used to analyze significance. All analyses except 3-way ANOVA were performed using GraphPad prism 9.2.0 (San Diego, CA). 3-way ANOVA analyses were conducted using SPSS (Version 25, IBM Corporation, Armonk, NY).

IL-12 was used to direct differentiation of CD4⁺ T cells. IL-12 preferentially directed differentiation of Tbet- (Th1; p = 0.006; Figures 1A, B) and had no effect on FOXP3- (Treg; Figures 1C, D) expressing CD4⁺ T cells, while decreasing the expression of GATA3 (Th2; p < 0.001; Figures 1E, F) and RORγt (Th17; p < 0.01; Figures 1G, H).

To test the impact of alcohol on CD4⁺ T cell differentiation, naïve CD4⁺ T cells were differentiated in the presence of 50 mM ethanol under Th1-promoting conditions. There was a significant interaction observed between DIFF and EtOH on both Tbet (p < 0.05) and FOXP3-expressing (p < 0.01) CD4⁺ T cells. Post hoc pairwise comparisons indicated that differentiation of CD4⁺ T cells significantly increased Tbet-expressing CD4⁺ T cells compared to undifferentiated naïve CD4⁺ T cells (p < 0.0001) and ethanol increased expression of Tbet within differentiated CD4⁺ T cells (p = 0.001; Figures 2A, B). Also, post hoc pairwise comparisons indicated that differentiation significantly increased FOXP3-expressing CD4⁺ T cells compared to undifferentiated naïve CD4⁺ T cells (p < 0.0001) and ethanol decreased expression of FOXP3 in differentiated CD4⁺ T cells (p = 0.001; Figures 2C, D). Ethanol increased the Tbet : FOXP3 ratio (p = 0.004; Figure 2E) in differentiated CD4⁺ T cells. No significant differences were detected between undifferentiated Naïve and EtOH-treated groups.

Glycolysis was assessed to understand if metabolism played a role in the ethanol-mediated increase of Tbet-expressing CD4⁺ T cells. There was a significant interaction observed between DIFF and EtOH on CD4⁺ T cell GLUT1 expression (p < 0.01), 2-NBDG uptake (p < 0.05), glycolysis (p < 0.0001) and glycolytic capacity (p < 0.0001). Post hoc pairwise comparisons indicated that differentiation of CD4⁺ T cells significantly increased GLUT1 expression (p < 0.0001; Figures 3A, B), glucose uptake (2-NBDG; p = 0.0002; Figures 3C, D), glycolysis (p < 0.0001; Figures 3E, F) and glycolytic capacity (p < 0.0001; Figure 3G) compared to undifferentiated naïve CD4⁺ T cells. Also, post hoc pairwise comparisons indicated that ethanol increased GLUT1 expression (p = 0.005; Figure 3B), glucose uptake (p = 0.014; Figure 3D), glycolysis (p = 0.005; Figure 3F) and glycolytic capacity (p < 0.0001; Figure 3G) within differentiated CD4⁺ T cells. No significant differences were detected between undifferentiated naïve and naïve EtOH groups.

To further understand the importance of glycolysis on the ethanol-mediated increase of Tbet-expressing CD4⁺ T cells, CD4⁺ T cells were exposed with ethanol in the presence of the glycolytic inhibitor 2-deoxyglucose (2-DG). The was a significant interaction observed between DIFF, EtOH, and 2-DG on Tbet-expressing CD4⁺ T cells (p < 0.05) and a significant interaction observed between DIFF and EtOH on FOXP3-expressing CD4⁺ T cells (p < 0.05). Post hoc pairwise comparisons indicated that differentiation increased Tbet (p < 0.0001; Figures 4A, B) and FOXP3-expressing (p < 0.0001; Figures 4C, D) CD4⁺ T cells compared to undifferentiated naïve CD4⁺ T cells. Ethanol increased Tbet-expression within differentiated CD4⁺ T cells (p = 0.002; Figures 4A,B). 2-DG prevented the ethanol-induced increase in Tbet-expression in differentiated CD4⁺ T cells (Figures 4A, B). Ethanol decreased CD4⁺ T cell FOXP3 expression within differentiated CD4⁺ T cells (p = 0.024; Figures 4C, D) irrespective of 2-DG treatment (p = 0.012; Figures 4C, D). No significant differences were detected between undifferentiated naïve and naïve EtOH groups.

In order to understand the ethanol-mediated decrease in FOXP3-expressing CD4⁺ T cells, mitochondrial parameters were assessed using the Mitostress test. Ethanol decreased maximal respiration (p = 0.049; Figures 5A, B) and increased OCR-linked proton leak within the differentiated CD4⁺ T cells (p = 0.022; Figure 5C). Ethanol decreased coupling efficiency (p = 0.036; Figure 5D), and OCR-linked ATP production (p = 0.014; Figure 5E) within the differentiated CD4⁺ T cells. Ethanol decreased Bioenergetic Health Index (BHI; p = 0.04; Figure 5F) and decreased the OCR/ECAR ratio (p = 0.01; Figure 5G) within differentiated CD4⁺ T cells.

To further understand the ethanol-mediated decrease in mitochondrial function within CD4⁺ T cells, cells were sorted with the human CD4+CD25+ regulatory T cell isolation kit to enrich Treg (CD4+CD25+ T cells) and negatively select CD4+CD25- Th1-enriched T cells. Ethanol increased OCR-linked proton leak in enriched Treg cells (p = 0.0313; Figures 6A, B). Ethanol decreased coupling efficiency (p = 0.0031; Figure 6C) and OCR-linked ATP production (p = 0.044; Figure 6D) in enriched Treg cells. There were no observed significant effects of ethanol on mitochondrial parameters within enriched Th1 cells. There were no differences for BHI or OCR/ECAR ratio observed between the enriched populations (Supplementary Figure 6)

Since mitochondrial function was impaired within ethanol-treated CD4⁺ T cells, mitochondrial content was assessed to determine any further potential ethanol-mediated dysfunction. There was a significant interaction observed between DIFF and EtOH on CD4⁺ T cell mitochondrial content (p < 0.01). Post hoc pairwise comparisons indicated that differentiation increased mean fluorescence intensity (MFI) of MitoTracker Deep Red within CD4⁺ T cells compared to undifferentiated naïve cells (p < 0.0001; Figures 7A, B) and ethanol increased MitoTracker MFI within differentiated CD4⁺ T cells (p = 0.004; Figures 7A, B). To determine if both Th1 and Treg cells are contributing to this ethanol-mediated increase in mitochondrial content, enriched CD4⁺ subsets were stained. Ethanol increased MitoTracker MFI in enriched Treg cells (p = 0.038; Figures 7C, D), with no observed significant increase in enriched Th1 cells (p = 0.062; Figures 7E, F).

Gene expression important for mitochondrial repair and mitophagy were assessed to determine the potential impact of ethanol on CD4⁺ T cell mitochondrial homeostasis. There was a main effect of DIFF to increase gene expression important for autophagosome formation (ATG5, p = 0.01; ATG13, p = 0.04; MAP1LC3B, p = 0.01; BECN1, p = 0.01; BNIP3L, p = 0.05; ULK1, p = 0.002; Figure 8), mitochondrial biogenesis (TFAM, p = 0.03; Figure 8), and mitochondrial fission (MFF, p = 0.02; Figure 8), and decrease PPARGC1B (p = 0.005; Figure 8) expression. There was a main effect of DIFF and a main effect of EtOH to increase gene expression important for mitochondrial fusion (MFN2, DIFF: p = 0.001, EtOH: p = 0.01; OPA1: DIFF: p = 0.003, EtOH: p = 0.03; Figure 8). There was a main effect of EtOH to increase gene expression important for mitophagy (PINK1, p = 0.01; Figure 8) and decrease expression important for autophagosome formation (ATG7, p = 0.04; Figure 8). (Summarized in Figure 9). No significant interaction effects were observed.