Abstract
Severe influenza A virus (IAV) infections can result in hyper-inflammation, lung injury and acute respiratory distress syndrome1,2,3,4,5 (ARDS), for which there are no effective pharmacological therapies. Necroptosis is an attractive entry point for therapeutic intervention in ARDS and related inflammatory conditions because it drives pathogenic lung inflammation and lethality during severe IAV infection6,7,8 and can potentially be targeted by receptor interacting protein kinase 3 (RIPK3) inhibitors. Here we show that a newly developed RIPK3 inhibitor, UH15-38, potently and selectively blocked IAV-triggered necroptosis in alveolar epithelial cells in vivo. UH15-38 ameliorated lung inflammation and prevented mortality following infection with laboratory-adapted and pandemic strains of IAV, without compromising antiviral adaptive immune responses or impeding viral clearance. UH15-38 displayed robust therapeutic efficacy even when administered late in the course of infection, suggesting that RIPK3 blockade may provide clinical benefit in patients with IAV-driven ARDS and other hyper-inflammatory pathologies.
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Data availability
The single-cell RNA-sequencing datasets analysed during the current study are available in the NCBI Short Read Archive (SRA) under accession PRJNA612345. Other datasets generated during and/or analysed during the current study are PDB: 4M66, PDB: 4M69 and PDB: 7MX3. Source data are provided with this paper.
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Acknowledgements
We acknowledge M. Cameron, W. Childers, J. Wooltorton and K. Korzekwa for carrying out pharmacokinetic analyses of UH15-38, and L. Richey and J. Onufrak for toxicological assessment of this molecule. The authors thank J. Testa for the M29 cell line and R. Dunbrack for assistance with molecular modelling. We acknowledge The University of Texas at San Antonio Center for Innovative Drug Discovery for scale-up synthesis of UH15-38. This work was supported by NIH grants AI135025 and AI168087 to S.B.; AI144400 to S.B., G.D.C. and A.D.; AI161624 to S.B. and S.S.-C.; AI164003 to G.D.C. and A.D.; HL170121 to D.F.B. and S.B.; R01AI144828 and R35CA231620 to D.R.G.; Collaborative Influenza Vaccine Innovation Centers contract 75N93019C00052 and funds from the American Lebanese Syrian Associated Charities to S.S.-C.; HHS Contract 75N93021C00016 (St Jude Center of Excellence for Influenza Research and Surveillance) to S.S.-C. and P.G.T.; 75N93021C00018 (Center for Influenza Disease and Emergence Response) to P.G.T; and Deutsche Forschungsgemeinschaft grant SFB1160 to M. Schwemmle. Additional funds were provided by S10OD030332 to the UF Scripps Institute for Biomedical Innovation and Technology, by a Fox Chase Cancer Center Innovator Grant, and NIH Cancer Center Support Grant P30CA006927 to S.B.
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Contributions
A.G. and D.F.B. carried out most of the biological experiments, with assistance from T.Z., I.S., L.-A.V.d.V., J.G., V.M., B.T., D.A.R., C.Y., D.S., J.B., C.D., R.M.W., M. Shubina, B.L., D.Z. and J.C.C. RIPK3 constructs, pMLKL antibodies and Casp8−/−MlklFlag/Flag mice were generated by D.A.R. and D.R.G. Test compounds were prepared by S.N., R.B. and A.L.D. Molecular docking studies were carried out by S.L. Analyses of docking results and rendering of models was performed by M.D.A. Histological analyses of infected tissues was conducted by K.Q.C. and P.V. C.L., L.C.F., M. Schwemmle, S.S.-C., D.R.G., G.D.C., P.G.T., A.D. and S.B. designed experiments and analysed the data. A.G., D.F.B., A.D., G.D.C. and S.B. wrote the manuscript. All authors participated in editing the manuscript.
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S.N., G.D.C., A.D. and S.B. are listed as co-inventors on patent applications related to the UH15 series of compounds filed by Tufts University, the University of Houston and the Institute for Cancer Research, Fox Chase Cancer Center. L.C.F., G.D.C., A.D. and S.B. hold equity in Vaayu Therapeutics. G.D.C. holds equity in Denali Therapeutics and has received royalties from Brigham and Women’s Hospital. The other authors declare no competing interests.
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Extended data figures and tables
Extended Data Fig. 1 UH15-38 is a potent RIPK3 kinase inhibitor.
a, Immunoblot analysis of pMLKL and cleaved caspase 8 (CC8) in lysates obtained from Ripk3–/– MEFs stably expressing 2xFv-RIPK3 and treated with dimerizer (AP20187, 100 nM) in the presence of the pan-caspase inhibitor (IDN-6556, 20 μM) and UH15-38 (500 nM) for 12 h. b, Table comparing UH15-38 to GSK′872 in the indicated recombinant kinase assays. Kinase assays were performed using ADPGlo (Promega) and on the DiscoverX platform (Eurofins DiscoverX). ND = Not determined. c, Overview of docking of UH15-38 into human RIPK3. d, Docking of GSK′872 into mouse RIPK3. e, Docking of GSK′843 into mouse RIPK3. f, MEFs infected with PR8 (MOI = 2) were treated with indicated drugs in the presence of zVAD (50 μM) and cell viability was determined after 24 h. g, Cell survival kinetics of iBMDMs treated with LPS (10 ng/ml) and TAK1 inhibitor 5z7 (200 nM) following exposure to the indicated concentrations of the RIPK3 inhibitors UH15-38 and GSK′872 or the RIPK1 inhibitor GSK′547 for 6 h. h, Ripk3+/+ and Ripk3–/– MEFs were treated with TNF/5z7/IDN6556 and TNF/5z7, respectively, in the presence of the indicated concentrations of UH15-38, and viability was determined after 24 h. Ripk3–/– MEFs treated with UH15-38 alone were used as controls. i, Viability of Ripk3–/– MEFs treated with TNF/5z7 in the presence of DMSO or GSK′547 (10 μM). j, Immunoblot analysis of Gasdermin D (GSDMD) cleavage in primary BMDMs pre-treated with LPS (10 ng/ml) for 3 h followed by Nigericin (10 μM) or ATP (5 mM), along with DMSO or UH15-38 (500 nM), for an additional 1 h. k, Viability of primary BMDMs pre-treated with LPS (10 ng/ml for 3 h) followed by treatment with Nigericin (10 μM) and the indicated concentrations of UH15-38 for 1 h. Viability was determined by using CellTiter-Glo assay (as in g, h, k) or Trypan Blue exclusion assay (as in f). Error bars represent mean ± SD (n = 3). Data are from one of the at least two independent experiments. Groups were compared using ordinary one-way ANOVA (as in f, k) or the unpaired two-sided Student’s t test (as in i).
Extended Data Fig. 2 Pharmacological profiling of UH15-38.
a, Half-life (T1/2) and peak concentrations (Cmax) of UH15-38 in tissue samples collected from mice treated with four once-daily) doses of UH15-38 (30 mg/kg/day, i.p.). b, c, Immunofluorescence staining for phosphorylated-MLKL (pMLKL) (b) and quantification of pMLKL signal in lung, heart kidney and liver sections (c) obtained from Casp8–/–MlklFLAG/FLAG mice following i.p administration of either vehicle (n = 3 mice) or UH15-38 (30 mg/kg, once-daily, n = 4 mice) for four days. Six fields of each tissue section per mice were quantified. d, InVEST Safety Panel profile of UH15-38 showing percent inhibition of each target in the presence of 1μM compound. e, f, Immunohistochemistry for cleaved caspase 3 (CC3) (e) and quantification of cleaved caspase 3 signal (f) in lung, heart, kidney and liver sections (n = 4 mice) following i.p. administration of either vehicle or UH15-38 (30 mg/kg, once-daily) for seven days. IAV PR8-infected lung tissue (n = 4 mice) is shown as positive control in e and f (green). Groups were compared using the two-sided Mann-Whitney U test.
Extended Data Fig. 3 UH15-38 is a potent and specific inhibitor of necroptosis in murine and human cells.
a, Podoplanin (PDPN) staining demonstrates purity of primary Type I AECs. CD140a was used as control for fibroblastic (Fibs) contamination. b, Cell survival kinetics of Type I AECs treated with TCZ and exposed to the indicated concentrations of the RIPK3 kinase inhibitors UH15-38, GSK′843 or GSK′872). c, Cell survival kinetics of primary wild-type MEFs infected with PR8 (MOI = 2) and treated with the indicated RIPK3 kinase inhibitors in the presence or absence (DMSO) of zVAD. d, Immunoblot analysis of the indicated proteins in lysates prepared from primary MEFs infected with PR8 (MOI = 2) and treated with the indicated concentrations of UH15-38. Cell lysates were prepared 12 h after infection. e, Cell survival analysis following infection of MEFs with a panel of IAV and IBV strains and exposure to the indicated concentrations of UH15-38 in the presence or absence of zVAD (50 μM). f, Immunoblot analysis of the indicated proteins in cell lysates prepared from primary MEFs infected with a panel of IAV or IBV strains (MOI = 5) and treated with DMSO or UH15-38 (1 μM). Cell lysates were prepared 12 h after infection. g, Viability of primary Ripk1–/– MEFs infected with PR8 (MOI = 2) and treated with DMSO or UH15-38 (1 μM). h, Viability of primary MEFs after infection with PR8 (MOI = 2) and treatment with UH15-38 or CSLP37 (a RIPK2 inhibitor) in the presence of either DMSO or zVAD (50 μM). (zVAD is included in the assays to block apoptosis so that effects of the test compounds on necroptosis can be evaluated). i, Viability of primary MEFs after infection with PR8 (MOI = 2) and treatment with UH15-38 or imatinib (an ABL inhibitor) in the presence of either DMSO or zVAD (50 μM). j, k, Zbp1–/– MEFs stably expressing 2xFv-tagged murine ZBP1 were exposed to dimerizer (AP20187, 100 nM) in the presence of the indicated concentrations of UH15-38. Cell viability (j) and immunoblot analyses (k) of the indicated proteins (right) are shown. l, Viability of HeLa-RIPK3 cells treated with human TNFα (100 ng/mL) + cycloheximide (2.5 μg/mL) + zVAD (50 μM) (TCZ) in the presence or absence of UH15-38 (1 μM). m, HeLa-RIPK3 cells treated with TCZ and the indicated concentrations of UH15-38 were examined for pMLKL, total MLKL, and RIPK3 by immunoblot analysis 18 h after treatment. n, M29 cells infected with PR8 (MOI = 10) were treated with increasing concentrations of UH15-38 for 24 h and examined for the indicated proteins by immunoblot analysis. H1N1 influenza strains: A/Puerto Rico/8/1934 (PR8), A/California/04/2009 (Cal/09); H3N2 influenza strains: A/Brisbane/10/2007 (Bri/07), A/Singapore/INFIMN-16-0019/2016 (Sin/16); Influenza B virus strains B/Colorado/06/2017 (Col/17) and B/Florida/04/2006 (Flo/06). zVAD (50 μM) was used to prevent apoptosis in this experiment. Cell viability in all panels was determined at 24 h after infection, using the Trypan Blue exclusion assay. Error bars represent mean ± SD of n = 3 samples. All data are from one of at least two independent experiments with similar outcomes. Groups were compared using ordinary one-way ANOVA.
Extended Data Fig. 4 UH15-38 is a potent inhibitor of RIPK3 in cellulo.
a, Viability of MEFs following treatment with indicated concentrations of UH15-38. b, Immunoblot analysis of the lysates of MEFs treated with indicated concentrations of UH15-38 for the markers of apoptosis. CC8 = cleaved caspase 8, CC3 = cleaved caspase 3. c, Viability of wild-type MEFs treated with 100 x IC50 (5 μM) of UH15-38 in the presence of DMSO or zVAD (50 μM), as compared to the viability of Ripk3 −/− MEFs treated with 100x IC50 UH15-38. d, Viability of Type I AECs following treatment with indicated concentrations of UH15-38. e, Immunoblot analysis of the lysates of Type I AECs treated with indicated concentrations of UH15-38 for markers of apoptosis. Cell viability in all panels was determined using the Trypan Blue exclusion assay. Groups were compared using ordinary one-way ANOVA.Error bars are mean ± SD of n = 3 samples. Figures are representative of two (b, e) or three (a, c, d) independent experiments with similar outcomes.
Extended Data Fig. 5 UH15-38 prevents lethality in severe influenza.
a, Weight loss curves of mice infected with PR8 (6000 EID50; ~LD100) followed by i.p. administration of vehicle (n = 20) or the following doses of UH15-38: 50 mg/kg (n = 20), 30 mg/kg (n = 21), 15 mg/kg (n = 15), 7.5 mg/kg (n = 15). Vehicle or UH15-38 was administered once-daily per the dosing schedule shown above the graph. b, c, Survival graphs (b) and weight loss curves (c) of mice (n = 10) infected with PR8 (6000 EID50) and treated with vehicle (n = 12) or with UH15-38 (30 mg/kg, i.p.) for a shortened-, or delayed-dosing regimens, as indicated above panel b. d, e, Survival (d) and weight loss (e) curves of mice (n = 7) infected with PR8 (4500 EID50) and treated i.p. with vehicle or GSK′872 (30 mg/kg) as indicated above the graph. f, Weight loss analysis of mice infected with IAV H1N1 strain A/California/04/09 (600 EID50; ~LD60) and treated once-daily with either vehicle (n = 10) or UH15-38 (30 mg/kg, i.p., n = 13) per the dosing schedule shown above the graph. g, Weight loss curves of mice infected with PR8 (4500 EID50; ~LD60) and treated i.p. with UH15-38 (30 mg/kg, i.p.), per dosing regimens shown above the graph (drug treatment beginning at day 3 after infection, n = 9; all other groups, n = 10/group). h, Wild type mice or Mlkl –/– mice (n = 10) were infected with PR8 (2500 EID50). Wild type mice were treated with either vehicle (n = 10) or 30 mg/kg UH15-38 (n = 12) once daily for four days starting 24 h after infection. i, Wild type mice or Mlkl –/– mice (n = 15) were infected with PR8 (4500 EID50). Wild type mice were treated with either vehicle (n = 14) or 30 mg/kg UH15-38 (n = 13) once daily for four days starting 24 h after infection. Mice were observed until 21 days and survival curves were plotted. Wild-type (Mlkl+/+) mice in panels h and i were generated by intercrossing Mlkl+/– mice. Groups were compared using the Log-rank (Mantel-Cox) test.
Extended Data Fig. 6 UH15-38 prevents necroptosis, inflammation, and injury in IAV-infected lungs.
a, b, Immunofluorescence staining of cleaved caspase 3 (CC3) (a) and quantification of CC3 signal (b) in lung sections harvested on the indicated days post-infection from mice infected with PR8 (6000 EID50) and treated i.p. with either vehicle or UH15-38 (30 mg/kg once-daily), starting one day after infection, for up to four days. c, Primary Type I AECs were infected with PR8 (MOI = 2) and treated with DMSO or UH15-38 (1 μM). Supernatants were collected 12 h after infection and the indicated chemokines were analyzed on the Luminex platform. d, e, Morphometric images of Tenascin C stained lung sections showing Tenascin C positive area (red), inflamed tenascin C negative lung area (blue), larger airways (yellow) and normal lung area (green) (d) and proportion of Tenascin C positive area (e) in infected lungs (n = 5/group) nine days after infection, following i.p. administration of either vehicle or UH15-38 (30 mg/kg once-daily), starting one day after infection, for four days. f, Levels of IL-17 and CCL5 in BALF from infected mice (n = 4/group) measured on the Luminex platform three days after infection, following i.p. treatment with either vehicle or UH15-38 (30 mg/kg once-daily), starting one day after infection, for two days. g, Histological scores of lung sections obtained from mice (n = 5/group) three days (alveolar inflammation and interstitial inflammation) or nine days (septal thickening and epithelial metaplasia) following infection with PR8 (6000 EID50) and treated i.p. with either vehicle or UH15-38 (30 mg/kg once-daily), starting one day after infection, for up to four days. h, Primary BMDMs were infected with PR8 (MOI = 5) and treated with UH15-38 (1 μM) in the presence or absence of zVAD (50 μM). Supernatants were collected 24 h after infection and IL-1β and IL-18 levels were measured by ELISA. i, Airway resistance (RI) was measured in mice uninfected (Mock/Vehicle, n = 5; Mock/UH15-38, n = 4) or infected (PR8, 2500 EID50, n = 4/group) 10 days after infection following treatment with either vehicle or UH15-38 (30 mg/kg) intraperitoneally one dose daily for four days starting 24 h post infection. Data are presented as mean ± SD. (n = 6/group in b or n = 3/treatment condition in c, h). Comparison between groups was carried out by two sided Mann-Whitney U test (as in b, e, f, g) or by ordinary one-way ANOVA (as in c, h) or two-way ANOVA (as in i).
Extended Data Fig. 7 UH15-38 does not impede virus clearance or anti-IAV CD8+ T cell responses.
a,b, Lung morphometry showing virus spread (red areas) in lungs (a) and quantitation of percentage of viral antigen-positive lung area (b) at 6 days after infection. n = 5/group. c, Virus titers in lungs (day 3 and day 6, n = 10/group; day 9 and day 12, n = 5/group) at indicated time points as determined by plaque assay. d, Frequencies of IAV-specific CD8+ T cells nine days after infection with PR8 in BALF of vehicle- and UH15-38-treated mice using peptide:MHC tetramers incorporating PB1 residues 703-711 or PA residues 224-233 (n = 10/group). Comparison between groups was carried out by the two-sided Mann-Whitney U test (as in b, c, d), nd = not detected.
Extended Data Fig. 9 MLKL binding requires the displacement of the RIPK3 αC helix.
a,b, Structures of monomeric (a) and MLKL-bound (b) mRIPK3. N-terminal lobe is depicted in gold and the C-lobe in light green. The αC helix is shown in light blue, and the beginning of the activation loop, including the DFG motif, in salmon. The side chains of key active site residues are shown as sticks and labeled. c. Overlaying the monomeric and MLKL-bound conformations of mRIPK3 shows that the αC helix swivels (blue arrow) outwards in the MLKL-bound conformation, with the E61 residue now facing away from the active site. The dashed red lines indicate axes of the αC helices in inactive and active conformations.
Supplementary information
Supplementary Figure 1
Images of uncropped immunoblots
Supplementary Table 1
In vitro safety and kinome profiling of UH15-38. The first tab shows InVEST Safety Panel (Reaction Biology) results for inhibitory activity of UH15-38 (1 μM) against a panel of 50 critical enzymes. The second and third tabs depict results from screening UH15-38 (500 nM) against a panel of 90 non-mutant human kinases (KinomeScan, DiscoverX).
Supplementary Table 2
Toxicological assessment of UH15-38. The first tab depicts whole-mouse and organ weights at the end of a 7-day toxicology assessment of UH15-38, following intraperitoneal administration at 30 mg kg−1 day−1 for 7 days. The second tab shows cell composition and bloodwork at the end of the 7-day toxicology assessment. The third tab contains the Pathologist’s report.
Supplementary Table 3
Pharmacokinetic profile of UH15-38. The first tab shows key pharmacokinetic parameters of UH15-38 measured from plasma and lung levels of the compound in mice, following intraperitoneal administration of four once-daily 30 mg kg−1 doses of UH15-38. The second tab shows levels of serum biomarkers following intraperitoneal administration of four once-daily 30 mg kg−1 doses of UH15-38.
Supplementary Table 4
NMR spectra and HPLC chromatograms of UH15-38•HCl and UH15-38 Me.
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Gautam, A., Boyd, D.F., Nikhar, S. et al. Necroptosis blockade prevents lung injury in severe influenza. Nature 628, 835–843 (2024). https://doi.org/10.1038/s41586-024-07265-8
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DOI: https://doi.org/10.1038/s41586-024-07265-8
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Nature Reviews Drug Discovery (2024)
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Targeting necroptosis prevents viral-induced lung damage
Cell Death & Differentiation (2024)
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Blocking cell death limits lung damage and inflammation from influenza
Nature (2024)
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Need for standardization of Influenza A virus-induced cell death in vivo to improve consistency of inter-laboratory research findings
Cell Death Discovery (2024)