Sepsis is characterized by a systemic inflammatory response syndrome (Kaukonen et al., 2015) driven by host cells following systemic bacterial (Ramachandran, 2014) and viral infections. The excessive inflammatory response can derail into septic shock resulting in multiple organ failure, the leading cause of death in intensive care units. Inflammasome activation, which downstream pathways cause the release of proinflammatory cytokines and the induction of an inflammatory cell death termed pyroptosis (Kumar, 2018), has been pointed out as the major driver of septic shock. Hereby, a two-armed lipopolysaccharide (LPS)-derived induction of the NLRP3-canonical inflammasome, the major source of IL-1β and IL-18 cytokine production (Lopez-Castejon and Brough, 2011) and the caspase-11-mediated non-canonical inflammasome leading to pyroptosis in monocytes (Yi, 2017), was determined as the underlying mechanism. Mechanistically, caspase-11 acts as a pattern recognition receptor for intracellular bacteria (Ding and Shao, 2017) that cleaves gasdermin D (GSDMD), a membrane pore-forming protein subsequently inducing pyroptotic cell death (Shi et al., 2015). The NLRP3-canonical inflammasome in turn was found to be indispensable (Man et al., 2017) for septic shock-induced death. However, cross-activation through caspase-11 promoting cytokine release has been described (Kayagaki et al., 2015; Kayagaki et al., 2011; Yang et al., 2015a), assigning the non-canonical inflammasome a cardinal role (Kayagaki et al., 2013).

Recent approaches such as anti-proinflammatory cytokine strategies blocking downstream targets of inflammasomes have been ineffective (Angus and van der Poll, 2013) while inhibiting inflammatory key regulators such as NF-κB may promote adverse side-effects (Fraser, 2006). Hence, contemporary clinical therapy of septic shock is based on symptomatic treatment rather than curative approaches that clear the cause of the disease itself.

In our previous studies, we have underscored the immunosuppressive properties of NAD⁺ in autoimmune diseases and allo-immunity via the regulation of CD4⁺ T cell fate (Tullius et al., 2014; Elkhal et al., 2016). More recently, we have shown that NAD⁺ administration protected mice from lethal doses of Listeria monocytogenes (L. m.) via mast cells (MCs) exclusively and independently of major antigen presenting cells (APCs) (Rodriguez Cetina Biefer et al., 2018). However, the underlying mechanism that allows NAD⁺, to concomitantly protect against autoimmune diseases, via its immunosuppressive properties (Tullius et al., 2014; Elkhal et al., 2016), and against lethal bacterial infection remains unclear.

Therefore, in the current study we investigated whether NAD⁺ protects against bacterial infection by dampening the systemic inflammatory response associated with sepsis or through enhanced bacterial clearance. Although, wild type (WT) mice subjected to NAD⁺ or PBS and lethal doses of pathogenic Escherichia coli (E. coli) exhibited similar bacterial load in various tissues, mice treated with NAD⁺ displayed a robust survival. Moreover, NAD⁺ protected against LPS-induced death that was associated with a dramatic decrease of systemic IL-1β and IL-18 levels, two major cytokines involved in the inflammasome signaling machinery. More importantly, we show that NAD⁺ protected from LPS-induced death by targeting specifically the non-canonical inflammasome via a blockade of the STAT1/IFN-β signaling pathway. Moreover, NAD⁺ treatment rendered not only caspase-11 knockout (KO) but WT mice fully resistant to poly(I:C)+LPS-induced septic shock, via an inflammasome-independent pathway mediated by a systemic IL-10 cytokine production.

Previously, we have delineated the protective role of NAD⁺ in the context of L. m. infection, a gram-positive bacterium (Rodriguez Cetina Biefer et al., 2018). However, it remained unclear whether NAD⁺ conveyed resistance toward L. m. by an augmented bacterial clearance or rather through its immunosuppressive effects dampening pathological systemic inflammation. Although the cell membrane of L. m. has been shown to bear lipoteichoic acids, which resemble the endotoxin LPS from gram-negative bacteria in both, structure and function, it is widely considered as an intracellular bacterium (Farber and Peterkin, 1991). In our current study, we administered a lethal dose of pathogenic E. coli, that is well known to promote septic shock, and showed that NAD⁺ also protected toward a lethal dose of this gram-negative bacterium. More importantly, we demonstrate that NAD⁺ conveys protection toward septic shock by specifically inhibiting the non-canonical inflammasome but not via bacterial clearance. Mechanistically, NAD⁺ impedes pro-casp-11 and casp-11 expression in macrophages blocking non-canonical-derived GSDMD cleavage and NLRP3 inflammasome activation, thus inhibiting pyroptotic cell death and proinflammatory cytokine release. The resistance of NAD⁺-treated WT mice against E. coli and LPS-induced septic shock reflected the robust inhibitory effect observed in vitro of NAD⁺ on the non-canonical inflammasome signaling machinery.

Until now, the exact mechanism how pro-casp-11 expression and its maturation to casp-11 is regulated remains unclear. Given the low basal expression of both pro-casp-11 and casp-11 (Schauvliege et al., 2002), a priming signal is required for initiating the non-canonical inflammasome pathway and macrophage sensing of intracellular LPS (Yang et al., 2015b). Previous work has demonstrated that transcriptional induction of the pro-casp-11 isoforms p42 and p38 in macrophages requires type I IFN stimulation (Schauvliege et al., 2002; Yen and Ganea, 2009) while IFN-β has been shown to promote transcriptional induction and processing of caspase-11 (Rathinam et al., 2012). In line with these findings, CTB treatment of macrophages primed with Pam3csk4 failed to elicit IL1-β release compared to LPS primed controls while exogenous administration of IFN-β in turn restored CTB-induced IL-1β production (Rathinam et al., 2012) underscoring the transcriptional role of type I IFN. Our RNA-sequencing results indicated a dampened cellular response toward IFN-β while western blotting revealed a significant downregulation of both, pro-casp-11 and casp-11, suggesting a transcriptional downregulation of both enzymes. Consistently, NAD⁺ decreased STAT-1 expression and phosphorylation, which constitutes the mechanistic link between extracellular type I IFN stimulation and transcriptional effects through translocation of phosphorylated STAT-1 to the nucleus inducing ISGs (Ivashkiv and Donlin, 2014). Thus, treatment of stimulated macrophages subjected to NAD⁺ with recombinant IFN-β restored STAT-1 signaling, caspase-11 expression, and GSDM cleavage which translated into reconstituted IL-1β production and LDH release. Collectively, NAD⁺ mitigates the intracellular response to IFN-β that leads to non-canonical inflammasome induction by suppressing macrophage-derived STAT-1 expression and phosphorylation. Furthermore, we showed that NAD⁺ treatment improved resistance of casp-11 KO mice toward poly I:C primed septic shock. More importantly, WT mice treated with NAD⁺ exhibited 100% survival while casp-11 KO mice treated with PBS exhibited a modest 40% survival, suggesting that NAD⁺ promotes survival beyond non-canonical inflammasome blockade. Our previous studies have delineated the effects of NAD⁺ on various immune cells such as dendritic cells and CD4⁺ T cells including Th1, Th17, regulatory type 1 (Tr1), and Treg cells communicated exclusively through MCs (Tullius et al., 2014; Elkhal et al., 2016; Rodriguez Cetina Biefer et al., 2018). Thereby, NAD⁺ treatment promoted MC-derived induction of TR1 cells that resulted into increased systemic levels of IL-10. Latter one was found to play a cardinal feature during bacterial infection as MC^-/- mice were more susceptible to L. m. infection than WT animals when treated with NAD⁺. Here, we found a direct effect of NAD⁺ on macrophages by specifically inhibiting the non-canonical inflammasome and promoting IL-10 production. Polymorphisms in the IL-10 locus or IL-10R deficiencies have been linked to severe intestinal inflammatory diseases in both, human and mice (Franke et al., 2008; Franke et al., 2010; Kühn et al., 1993; Begue et al., 2011). More importantly, mice deficient for IL-10 have been shown to display elevated inflammasome activation and IL-1β production resulting in severe colitis (Zhang et al., 2014) or Ag-induced arthritis (Greenhill et al., 2014). When inhibiting the autocrine pathway for IL-10 through combined receptor antagonization and IL-10 neutralization, we found a pronounced increase of IL-1β production of NAD⁺-treated macrophages stimulated with CTB and LPS (Figure 4D). This is consistent with previous reports showing that autocrine IL-10 signaling interferes with the transcription of pro-IL-1β (Sun et al., 2019). LDH release, in turn, was only restored partly possibly due to missing effects of second party leucocytes secreting IL-10 in vivo such as Tr1 cells which have been shown to inhibit the transcription of IL-1β and inflammasome-mediated activation of caspase-1 (Yao et al., 2015). More recently, casp-8, that plays a central role in apoptosis, has been reported as an important mediator of endotoxemia resistance and LPS-driven systemic inflammation. Since our RNA-sequencing results revealed a dramatically attenuated cellular response toward type I IFN with downregulation of various interferon regulatory factors, that have been reported as major regulators of casp-8 (Apelbaum et al., 2013; Newton et al., 2019), it is possible that NAD⁺ may exert protection against septic shock by altering caspase-8 expression as well. Although we have previously reported the protective effect of NAD⁺ against apoptosis of activated CD4⁺ T cells (Tullius et al., 2014), it remains yet to be determined how NAD⁺ impacts executioner proteins of other cell death processes such as apoptosis and necroptosis.

Notably, both casp-8 and casp-11 have been found dispensable in the hematopoietic compartment that produces the proinflammatory cytokines necessary to initiate shock (Mandal et al., 2018). Thus, NAD⁺ treatment may improve resistance of casp-11 KO mice to septic shock by also dampening the initiating proinflammatory cytokine cascade via its systemic IL-10 cytokine production. Importantly, while inhibiting macrophage-derived inflammasome function, NAD⁺ does not interfere with NF-κB signaling which has been shown to promote various inflammatory and autoimmune diseases when dysregulated (Liu et al., 2017). Taken together, we dissected the dichotomous capacity of NAD⁺ to dampen auto- and allo-immunity while concomitantly protecting toward severe bacterial infection, outlining its unique effects in the context of septic shock.

All data generated or analysed during this study are included in the manuscript as source data files for each figure. Data generated from RNA sequencing of BMDMs have been made publicly available in Dryad (https://doi.org/10.5061/dryad.zw3r228fj).

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Author details

1. Jasper Iske

   1. Division of Transplant Surgery, Department of Surgery, Brigham and Women’s Hospital, Harvard Medical School, Boston, United States
   2. Department of Cardiothoracic and Vascular Surgery, Germany Heart Center Berlin, Berlin, Germany

   Contribution

   Conceptualization, Data curation, Formal analysis, Validation, Investigation, Visualization, Writing - original draft, Writing – review and editing

   Contributed equally with

   Rachid El Fatimy and Yeqi Nian

   Competing interests

   No competing interests declared

   "This ORCID iD identifies the author of this article:" 0000-0001-8647-3092

2. Rachid El Fatimy

   1. Department of Neurology, Ann Romney Center for Neurologic Diseases, Brigham and Women's Hospital, Harvard Medical School, Boston, United States
   2. Institute of Biological Sciences (ISSB-P), Mohammed VI Polytechnic University, Benguerir, Morocco

   Contribution

   Data curation, Formal analysis, Validation, Investigation, Visualization, Methodology, Writing - original draft

   Contributed equally with

   Jasper Iske and Yeqi Nian

   Competing interests

   No competing interests declared

3. Yeqi Nian

   Institute of Transplant Medicine, Tianjin First Central Hospital, Nankai University, Tianjin, China

   Contribution

   Data curation, Formal analysis, Validation, Investigation, Visualization, Methodology, Writing - original draft

   Contributed equally with

   Jasper Iske and Rachid El Fatimy

   Competing interests

   No competing interests declared

4. Amina Ghouzlani

   NAD⁶ Immunology Laboratory, Huntington Medical Research Institutes, Pasadena, United States

   Contribution

   Formal analysis, Investigation, Visualization, Writing – review and editing

   Competing interests

   No competing interests declared

5. Siawosh K Eskandari

   Department of Internal Medicine, University of Groningen, Groningen, Netherlands

   Contribution

   Data curation, Formal analysis, Investigation

   Competing interests

   No competing interests declared

6. Hector Rodriguez Cetina Biefer

   1. Division of Transplant Surgery, Department of Surgery, Brigham and Women’s Hospital, Harvard Medical School, Boston, United States
   2. Department of Cardiac Surgery, Stadtspital Zurich Triemli, Zurich, Switzerland

   Contribution

   Investigation, Writing – review and editing

   Competing interests

   No competing interests declared

7. Anju Vasudevan

   Department of Neurosciences, Angiogenesis and Brain Development Laboratory, Huntington Medical Research Institutes, Pasadena, United States

   Contribution

   Supervision, Investigation, Methodology, Writing – review and editing

   Competing interests

   No competing interests declared

   "This ORCID iD identifies the author of this article:" 0000-0001-9814-2389

8. Abdallah Elkhal

   1. Division of Transplant Surgery, Department of Surgery, Brigham and Women’s Hospital, Harvard Medical School, Boston, United States
   2. NAD⁶ Immunology Laboratory, Huntington Medical Research Institutes, Pasadena, United States

   Contribution

   Conceptualization, Resources, Data curation, Software, Formal analysis, Supervision, Validation, Investigation, Visualization, Methodology, Writing - original draft, Project administration, Writing – review and editing

   For correspondence

   Abdala.Elkhal@hmri.org

   Competing interests

   No competing interests declared

   "This ORCID iD identifies the author of this article:" 0000-0002-8320-7722

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