Evaluation of combining the PDX analogue AN-137B with oseltamivir in a mouse model of severe influenza A (H1N1) infection

Abstract

Severe influenza infections involve an exacerbation of the pro-inflammatory response, which is influenced by both viral and host factors. Protectins PD1 and PDX previously demonstrated anti-influenza activity as well as anti-inflammatory properties. We recently reported that the combination of AN-137B, a molecular analogue of PDX, with oseltamivir or baloxavir provided synergism/additive effects against influenza, in vitro. Herein, we investigated potential benefits of the AN-137B-oseltamivir combination in mice infected with influenza A/Puerto Rico/8/1934 (H1N1) virus. Untreated animals and those that received single oseltamivir or AN-137B treatment showed mortality rates of 80%, 100% and 100%, respectively, whereas only 40% of mice that received the oseltamivir-AN-137B combination had to be euthanized. Body weight loss was also lower in the group of the combination. In the latter group, the mean lung viral titre (LVT), as determined by plaque assay (2.53 ± 0.63 × 10⁵ PFU/mL) and by qRT-PCR (2.39 ± 1.3 × 10⁸ copies/mL), was significantly lower than that of the untreated group (4.76 ± 0.9 × 10⁵ PFU/mL and 3.75 ± 0.86 × 10⁸ copies/mL (p < .05), contrasting with LVTs of animals that received single therapies. These in vivo results reinforce the potential of AN-137B when combined to a potent anti-influenza agent against severe influenza.

Keywords

influenza protectin AN-137B oseltamivir combination therapy

Introduction

Seasonal influenza A viruses (IAVs) are transmissible pathogens responsible for acute respiratory infections that can lead to up to 650,000 deaths per year worldwide.¹ Young children, the elderly and people with chronic illnesses are at a higher risk of developing severe complications.² During severe IAV infection, the imbalance between pro-inflammatory and anti-inflammatory cytokines is associated with a deleterious clinical outcome. As a complement to annual immunization programs, antivirals targeting key viral enzymes, such as the neuraminidase (NA) and the polymerase acidic (PA) endonuclease, can play an important role in controlling seasonal influenza infections.³ However, antivirals alone have not been shown to provide a significant reduction in mortality rates for severe influenza.⁴ As the exacerbation of the inflammatory response could be influenced by host-related factors in addition to factors related to viral replication, the use of compounds with the potential to modulate the host immune response could provide important clinical benefits.

Previous reports showed that protectins D1 (PD1) and DX (PDX), pro-resolving mediators that are formed during the resolution phase of acute inflammation, contributed to enhance the return of inflamed/injured tissue to homoeostasis.⁵ These protectins were involved in the defence of the host against various viral infections, including those caused by herpes viruses,⁶ human respiratory syncytial virus⁷ and virulent human and avian influenza A (H1N1) and A (H5N1) strains.^8,9

In a previous study, we synthesized a series of structurally simplified PDX analogues¹⁰ and assessed their activity against influenza A (H1N1) viruses, in vitro. Interestingly, the PDX analogue AN-137B was found to reduce influenza A/Puerto Rico/8/1934 (H1N1) viral titres, in a dose-dependent manner in treated ST6-GalI-MDCK cells, and demonstrated synergistic and additive in vitro effects when combined to the NA inhibitor oseltamivir and the PA inhibitor baloxavir, respectively.¹¹ Similar antiviral activity (IC₅₀ of 23 µM) was obtained with AN-137B when tested against wild-type and oseltamivir-resistant A (H1N1) pdm09 viruses.¹¹ The aim of the present study was to evaluate the in vivo properties of AN-137B alone or in combination with oseltamivir in mice experimentally infected with the influenza A/Puerto Rico/8/1934 (H1N1) virus.

Materials and methods

Cell culture and virus stock preparation

Madin-Darby canine kidney cells overexpressing the ⍺2-6 sialic acid receptor (ST6-GalI-MDCK cells), kindly provided by Y. Kawaoka from the University of Wisconsin-Madison, WI),¹² were maintained in minimum essential medium (MEM) supplemented with 10% FBS and puromycin (7.5 µg/mL).

Influenza A/Puerto Rico/8/1934 (H1N1) virus stock was prepared by infecting ST6GalI-MDCK cells in MEM medium supplemented with 1 μg/mL tosyl phenylalanyl chloromethyl ketone (TPCK)-treated trypsin (Sigma, Oakville, ON, Canada). After 4 days of incubation, resulting into complete cytopathic effects, viral production was harvested, aliquoted and frozen at – 80°C. An aliquot was thawed and titrated by plaque assay using 12-well plates containing confluent ST6GalI-MDCK cells.

Compounds

Oseltamivir-phosphate (Tamiflu) was purchased from a local pharmacy (at the CHU de Québec, Québec, Qc, Canada), and the protectin DX analogue AN-137B was synthesized as previously described¹⁰ and stored at −80°C under nitrogen and protected from light. No detectable degradation was observed after 1 year of storage under these conditions, as confirmed by HPLC and 1 H proton nuclear magnetic resonance (¹H NMR) analyses. AN-137 B was resuspended in propylene glycol: dimethylsulfoxide (DMSO) (92: 8) immediately before injection to ensure compound stability and accurate dosing.

Mouse experimental infections

Animal studies were performed using groups of nine 6- to 8-week old female C57BL6 mice (Charles River, St-Constant, Canada) that included a group of untreated animals and three treatment groups consisting of oral oseltamivir and/or intraperitoneal AN-137B (1 mg/kg, once daily for 5 days). The dose of AN-137B and the route of administration were selected from preliminary experiments assessing the compound toxicity. In addition, given the fact that native protectin (PDX) and other analogues have demonstrated efficacy in several inflammatory and infectious models, we anticipated a measurable biological response of AN-137B at the selected dose. We also preliminary tested different oseltamivir doses and virus concentrations before selecting the parameters proposed in this study. Consequently, by using a PR8 inoculum of 200 PFU, we expected to obtain a 100% mortality rate in untreated animals and we also targeted a minor protection with 1 mg/kg of oseltamivir to better see eventual benefits of the combination. Animals were initially weighed and randomly assigned to different treatment groups. Treatments started 4 h before viral inoculation. Finally, a group of uninfected animals was used as control. Experimental viral infection was performed under isoflurane anaesthesia by intranasal inoculation of 35 µL of PBS containing 200 plaque forming units (PFUs) of influenza A/Puerto Rico/8/1934 (H1N1) virus. Mice were weighed daily for 14 days. Animals whose weight loss reached ≥20% from their initial weight were humanely euthanized. Four mice per group were sacrificed on day 5 post-infection (p.i.), and their lungs were aseptically removed and homogenized for determination of lung viral titres (LVTs) and cytokine levels (n = 4).

For the determination of LVTs, harvested lung tissues were homogenized in 1 mL of PBS containing 2 x antibiotic solution (penicillin, streptomycin and amphotericin B) using Omni Tip homogenizer (OMNI International, GA, USA). Cells were pelleted by centrifugation (600 g, 5 min) ,and supernatants were titrated by plaque assay on ST6GalI-MDCK cells. Supernatants of lung homogenates were also used for viral RNA (vRNA) extraction with the MagNA Pure LC system (Total nucleic acid isolation kit, Roche Molecular System, Laval, QC, Canada), followed by reverse transcription quantitative PCR (qRT-PCR) assay as previously described.¹¹ The assay was performed with the QuantiTect Virus + ROX Vial Kit (Qiagen, Toronto, ON, Canada) on a LightCycler 480 system (Roche Molecular System). The results are expressed as number of vRNA copies per mL.

Interleukin-6 (IL-6) and interleukin-1 beta (IL-1β) levels in lung homogenates from infected mice were determined using specific mouse Enzyme Linked Immunosorbent Assay (ELISA) kits in duplicate following the manufacturer’s instructions (Sigma-Aldrich).

Statistical analyses

All analyses were made using the PRISM software (GraphPad Inc, San Diego USA). Viral titres and cytokine levels in lung homogenates of mice were compared using the unpaired Student’s t test. Mouse body weight changes and survival rates were compared with one-way ANOVA and the Chi-square test, respectively.

Results

As expected, intranasal inoculation of mice with 200 PFUs of influenza A/Puerto Rico/8/1934 (H1N1) virus resulted in clinical signs of infection such as body weight loss, lethargy and mortality that were observed in the four infected groups of mice with no signs being observed in uninfected animals. As shown in Figure 1, 4/5 animals (80%) in untreated and infected animals and all animals (5/5; 100%) in groups that received single oseltamivir or AN-137B treatment were humanely euthanized or died between day 7 and day 9 p.i. Only, 2/5 animals (40%) of mice that received the combination of oseltamivir and AN-137B were humanely euthanized. Accordingly, important body weight losses, in particular during days 5–9 p.i., were observed in infected animals while no signs of infection were observed in the uninfected group (Figure 2). Of interest, body weight loss was remarkably lower in the group that received the combined oseltamivir and AN-137B treatment (Figure 2).

Figure 1.

Survival curve of mice. Kaplan–Meier survival curves of non-infected (NI) and infected mice with 200 PFUs of influenza A/Puerto Rico/8/1934 (H1N1) virus. Four groups of infected- mice included a group that received saline (untreated) and those that received single or combined therapy with oseltamivir (gavage) and AN-137B (intraperitoneal) (1 mg/kg, once daily for 5 days). Mortality was recorded in subgroups of 5 animals during 14 days post-inoculation and analysed using the log-rank (Mantel–Cox) test.

Figure 2.

Body weight losses of mice. Mean percent weight changes ± standard deviation (as compared to initial weights) of mice inoculated intranasally with 200 PFUs of influenza A/Puerto Rico/8/1934 (H1N1) virus were recorded daily until day 14 post-inoculation. Infected mice included a group that received saline (untreated) and those that received single or combined therapy with oseltamivir (gavage) and AN-137B (intraperitoneal) (1 mg/kg, once daily for 5 days). *p < .05; **p < .01; **p < .001 as compared to the uninfected group. NI = non-infected mice.

Mean LVTs determined on day 5 p.i. were comparable in the group of untreated mice and those of animals that received single oseltamivir or AN-137B treatment (4.76 ± 0.9 × 10⁵, 3.03 ± 0.83 × 10⁵ and 3.86 ± 0.68 × 10⁵ PFU/mL, respectively). By contrast, the group of mice that received the combined treatment had a mean LVT of 2.53 ± 0.63 × 10⁵, which was significantly lower than the untreated group (p < .05; Figure 3(A)). Quantification of viral RNA in lung samples by qRT-PCR revealed a significant reduction in the number of viral RNA copies in the group that received the oseltamivir-AN-137B combination compared to the untreated group (2.39 ± 1.3 × 10⁸ copies/mL vs 3.75 ± 0.86 × 10⁸ copies/mL, respectively (p < .05)) while the groups that received single oseltamivir and AN-137B treatments had vRNA copy numbers that were not significantly different compared to the untreated group (3.75 ± 1.3 × 10⁸ copies/mL and 4.86 ± 2.29 × 10⁸ copies/mL, respectively) (Figure 3(B)).

Figure 3.

Mouse lung viral titres. Mean lung viral titres ±standard deviation for 4 mice infected intranasally with 200 PFUs of influenza A/Puerto Rico/8/1934 (H1N1). Titres were determined on day 5 post-inoculation by using plaque assays in ST6-GalI-MDCK cells (a) and by quantification of vRNA by qRT-PCR (B). Data were analysed by using the one-way ANOVA test (GraphPad). *p = .026 and .037 for (a) and (b), respectively, as compared to the untreated group.

Levels of the pro-inflammatory cytokine IL-1β in lung samples were significantly lower in the groups that received oseltamivir alone or oseltamivir in combination with AN-137B, compared to the untreated group (135.40 ± 17.92 pg/mL, 128.55 ± 28.55 pg/mL and 160.42 ± 3.12 pg/mL, respectively) while IL-1β levels of the AN-137B group were not significantly reduced compared to the untreated group (141.65 ± 6.24 pg/mL (Figure 4(A)). A similar pattern was observed regarding IL-6 lung levels, that is, 565.00 ± 99.08 pg/mL, 501.20 pg/mL, 654.57 ± 13.98 pg/mL and 763.85 ± 102.35 pg/mL for the groups that received oseltamivir, oseltamivir + AN-137B, 137B and no treatment, respectively (Figure 4(A)).

Figure 4.

Cytokine levels in mouse lungs. Levels of IL-1-β (a) and IL-6 (b) were determined in lung homogenates of mice infected intranasally with 200 PFUs of influenza A/Puerto Rico/8/1934 (H1N1) virus by ELISA. Results are expressed as the mean of protein concentration in pg/mL ± standard deviation of 4 mice per group from two independent experiments. *, p-values when comparing the oseltamivir group and the combination group to the untreated group using the Chi-square test were 0.033 and 0.023, respectively, (a) and 0.017 and 0.031 (b).

Discussion

Influenza A strains, mainly from the H1N1 and H3N2 subtypes, circulate each winter season throughout the world causing serious public health and economic problems. In most people, seasonal influenza viruses replicate in the upper respiratory tract inducing a self-limited disease, whereas viral replication may progress towards the lower respiratory tract, potentially triggering secondary bacterial infections and pneumonia in the elderly, young children and immunocompromised patients.² Influenza vaccines have the potential to mitigate the impact of influenza epidemics and eventual pandemics; however, the protection afforded by influenza vaccines could be much lower in high-risk groups. Moreover, antigenic drifts, that occur at regular intervals in seasonal influenza A viruses, may result in a significant decrease in vaccine effectiveness.¹³ Antiviral agents, including neuraminidase inhibitors (oseltamivir, zanamivir, peramivir and laninamivir) and compounds targeting the viral polymerase complex, such as baloxavir marboxil, constitute another important means for the management of seasonal influenza and are expected to play a major role in the advent of influenza pandemics. However, as for other antivirals, such as amantadine and rimantadine (in the adamantanes class), the emergence of resistant viruses constitutes a serious threat that may compromise the clinical utility of these agents. Several in vitro and in vivo studies have shown that therapies combining compounds with different mechanisms of action may be clinically advantageous in the treatment of influenza infections, including the potential to delay the emergence of resistance.

The aim of this study was to investigate whether, in agreement with our recent in vitro findings,¹¹ combining the PDX analogue AN-137B with oseltamivir would also improve the outcome of influenza A (H1N1) infection in a lethal mouse model. Importantly, AN-137B possesses both moderate antiviral activity and potent anti-inflammatory properties.¹¹ Furthermore, in vitro studies have shown synergism for the combination of AN-137B and oseltamivir.¹¹ The treatment of mice with AN-137B alone did not significantly improve the outcome of infection, based on the mortality rate (all mice died) and on animal weight losses (Figures 1 and 2). Future studies will aim at increasing either the concentration, the frequency of administration and the mode of administration of AN-137B in order to improve its activity against influenza viruses. Treatment with oseltamivir alone was not optimal although we used a low dose of the drug (1 mg/kg/day) in order to detect a potential synergistic effect when combined with AN-137B. Indeed, the combination of AN-137B with oseltamivir significantly improved animal survival; furthermore, weight losses were also remarkably lower in the combination group of infected mice (Figures 1 and 2). Accordingly, there was also a significant reduction in LVT from mice that received the combination therapy when assessed by both plaque and qRT-PCR assays (Figure 3). Of note, NA gene sequencing from lung samples of mice that received oseltamivir treatment did not reveal any oseltamivir resistance mutation.^14–16

Due to our institutional animal care committee restrictions, we used a limited number of mice per group for survival (n = 5) and for lung removal (n = 4) that may have impacted the statistical power of our results. However, the trend appears clear and is consistent with predictions based on our in vitro results. Moreover, our findings are in agreement with a previous report that protectin PDX improved the survival and lung pathology induced by severe influenza A (H1N1) and A (H5N1) infections even under conditions where the NA inhibitor peramivir failed to protect mice from death.⁹

In vitro experiments previously showed that the natural protectin PDX affected the replication of influenza A viruses by interfering with the virus RNA nuclear export machinery.⁹ The same group further described PDX as an innate suppressor of influenza virus replication that protects against lethal influenza virus infection since PDX levels appeared to inversely correlate with the pathogenicity of influenza virus strains. Nevertheless, as they are autacoids, natural protectins are rapidly metabolized and inactivated in vivo⁹ notably through beta-oxidation of its polar head chain. In that regard, AN-137B could share with PDX similar in vitro and in vivo mechanisms of action while the former providing important advantageous features, including greater chemical, thermal and metabolic stability as well as a more rapid synthesis (10–12 steps for PDX analogue AN-137B vs 26 steps or more for natural).^10,17,18 In that regard, we are planning on performing structure–activity relationship studies (SAR) in order to improve the antiviral activity of AN-137B while preserving its immunomodulatory properties.

As AN-137B derives from the pro-resolving lipid mediator PDX, we expected that AN-137B would exhibit in vivo anti-inflammatory activity as previously suggested by our LPS-stimulated macrophage experiments.¹¹ We thus evaluated the levels of IL-1β and IL-6 by ELISA due to their important role in the cytokine cascade during severe influenza, where IL-1β is expressed during the early stages of infection, followed by increased IL-6 expression.¹⁹ Nevertheless, we recognize that other cytokines/chemokines such as TNF-α, α/β IFNs and IFN-γ would also have been interesting to evaluate. In the present study, levels of IL-1-β and IL-6 pro-inflammatory cytokines were significantly reduced in the group of mice that received AN-137B combined to oseltamivir or oseltamivir alone with a slight decrease of IL-1-β and IL-6 levels (although not statistically significant) in animals that received AN-137B monotherapy when compared to the untreated group of mice. In this regard, it is possible that a higher dose of AN-137B might be necessary to generate a greater effect of the monotherapy on the cytokine levels. Also, there is a possibility that other cytokines might be involved in that context.

Conclusion

In conclusion, these in vivo results reinforce the potential of the PDX analogue, notably AN-137B, as a new therapeutic option when combined to oseltamivir for the control of severe influenza infections.

Footnotes

ORCID iD

Yacine Abed

Ethical considerations

All animal procedures described in this article were approved by the Institutional Animal Care Committee of Laval University (protocol # 2023-1282) according to the guidelines of the Canadian Council on Animal Care.

Author contributions

YA, GB and AM contributed to the design of the study and the preparation of the manuscript. CR and NF performed animal studies. JC performed in vitro experiments. RM and DP synthesized the AN-137B protectin analogue.

Funding

The authors disclosed receipt of the following financial support for the research, authorship, and/or publication of this article: Guy Boivin is a holder of a Canadian Institutes of Health Research grant: #229733.

Declaration of conflicting interests

The authors declared no potential conflicts of interest with respect to the research, authorship, and/or publication of this article.

Data Availability Statement

Data can be shared by the corresponding author.*

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