Abstract
Background
There is substantial evidence that signaling through Toll-like receptor 4 (TLR4) contributes to the pathogenesis of necrotizing enterocolitis (NEC). Pregnane X receptor (PXR), a xenobiotic sensor and signaling intermediate for certain host-bacterial metabolites, has been shown to negatively regulate TLR4 signaling. Here we investigated the relationship between PXR and TLR4 in the developing murine intestine and explored the capacity of PXR to modulate inflammatory pathways involved in experimental NEC.
Methods
Wild-type and PXR−/− mice were studied at various time points of development in an experimental model of NEC. In addition, we studied the ability of the secondary bile acid lithocholic acid (LCA), a known PXR agonist in liver, to activate intestinal PXR and reduce NEC-related intestinal inflammation.
Results
We found a reciprocal relationship between the developmental expression of PXR and TLR4 in wild-type murine intestine, with PXR acting to reduce TLR4 expression by decreasing TLR4 mRNA stability. In addition, PXR−/− mice exhibited a remarkably heightened severity of disease in experimental NEC. Moreover, LCA attenuated intestinal proinflammatory responses in the early stages of experimental NEC.
Conclusion
These findings provide proactive insights into the regulation of TLR4 in the developing intestine. Targeting PXR may be a novel approach for NEC prevention.
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Main
Necrotizing enterocolitis (NEC) is the most common and lethal gastrointestinal emergency of premature infants, affecting ~5–10% of infants with a birth weight under 1,500 g (1). The mortality rate is between 20 and 30%, and survivors are at significant risk for neurodevelopmental delays and lifelong impairment in gut function (2). The exact etiology of NEC remains unknown; however, several lines of evidence suggest an interaction between luminal bacteria and pattern recognition receptors in the intestinal epithelium. Studies in animal models and surgically resected preterm intestine suggest that signaling through Toll-like receptor 4 (TLR4), which recognizes lipopolysaccharide (LPS) of Gram-negative bacteria, is critical to NEC pathogenesis (3, 4, 5). Excessive stimulation of TLR4 leads to decreased epithelial proliferation, induction of apoptosis, and reduced barrier integrity (5, 6, 7), which may allow for bacteria to translocate across the epithelium culminating in the severe (uncontrolled) innate inflammatory response characteristic of the disease (1). Thus, identifying mechanisms of TLR4 control as they relate to the maintenance of intestinal barrier function could help in the design of NEC prevention strategies.
Pregnane X receptor (PXR), a nuclear receptor and xenobiotic sensor that is highly expressed in intestine and liver (8), has recently been identified as a negative regulator of TLR4 signaling (9, 10). PXR is activated by a broad range of endogenous and exogenous ligands, including steroids, bile acids, dietary compounds, and host-bacterial metabolites (8, 9, 10, 11). In xenobiotic liver metabolism, PXR regulates the expression of genes encoding enzymatic pathways involved in detoxification and clearance, such as cytochrome P450s and multidrug resistance protein 1a (Mdr1a) (P-glycoprotein) (12, 13). It is interesting to note that there is mutual suppression between xenobiotic metabolism and NF-кB-mediated inflammation in the enterohepatic axis (14). Exposure to xenobiotic drugs that activate PXR can suppress inflammation (14); whereas, inflammation can reduce the expression of PXR-responsive genes (15). The ability of PXR to function as a signaling intermediate for certain host-bacterial metabolites and its opposing relationship to TLR4 and NF-KB activity has made it an attractive target for studying intestinal inflammatory disorders. As such, PXR has been identified as contributing to inflammatory bowel disease (IBD) in humans (16, 17) and animal models (18). To date, however, there have been no studies investigating the role of PXR in regulating intestinal inflammation in NEC.
Although no experimental model of NEC fully recapitulates the clinical condition, many of the signaling pathways involved in NEC pathogenesis have been elucidated through the use of such systems (19). Indeed, the importance of TLR4 and its associated molecules in NEC pathophysiology has been demonstrated using neonatal mice subjected to a model of intermittent hypoxia and formula feeds, or variations thereof (5, 6, 7, 20). Thus, to better understand the pathogenesis of NEC relative to TLR4-dependent signaling, and explore the capacity of PXR to regulate NEC-associated inflammatory pathways, wild-type (WT) and PXR−/− mice were studied at various time points of development and subjected to a well-established experimental model of NEC (5, 6, 7, 20, 21). In addition, we studied the ability of the secondary bile acid lithocholic acid (LCA), a known PXR agonist in liver, to activate intestinal PXR and reduce NEC-associated intestinal inflammation. Secondary bile acids, such as LCA, are produced by luminal bacteria via the deconjugation of primary bile acids and are reported to have variable effects on the intestinal epithelium (22, 23). We speculated that when used at concentrations comparable to those that may be found in the neonatal intestine (24) and at levels sufficient to activate PXR in liver (11), LCA would activate intestinal PXR and reduce signaling via proinflammatory pathways thought to contribute to NEC. We observed a reciprocal relationship between the developmental expression of intestinal PXR and TLR4 and that PXR−/− mice demonstrated a heightened inflammatory response during experimental NEC. Furthermore, activation of intestinal PXR through LCA reduced early proinflammatory responses that precede development of full-blown disease in the NEC model.
Methods
Reagents, Cell Culture, and Mice
Ultrapure LPS (Escherichia coli 0111:B4) from Invivogen (San Diego, CA) was reconstituted in sterile water. LCA was from Sigma-Aldrich (St. Louis, MO) and reconstituted in methanol or directly dissolved in NEC formula. The rat small-intestinal cell line, IEC-6, was obtained from the American Type Culture Collection (ATCC, Manassas, VA) and maintained as per ATCC recommendations. Mouse primary intestinal organoids were isolated according to STEMCELL Technologies’ (Cambridge, MA) mouse intestinal organoid isolation protocol and cultured in the mouse IntestiCult organoid growth medium (06005). C57BL/6 (WT) mice were from the Jackson Laboratory (Bar Harbor, ME). PXR−/− mice (11) were generously provided by Dr. Sridhar Mani (Albert Einstein College of Medicine) and backcrossed into a C57BL/6 background. All animal procedures were approved by the University of Connecticut Health Animal Care and Use Committee and performed in accordance with the recommendations in the Guide for the Care and Use of Laboratory Animals of the National Institutes of Health.
Quantitative Real-Time PCR
Total RNA was extracted from either cultured IEC-6 enterocytes or ileal tissues using the RNeasy mini kit (Qiagen, Valencia, CA) and reverse transcribed (1 μg of RNA) into cDNA using iScript reverse transcription supermix for RT-qPCR (Bio-Rad, Hercules, CA). The mRNAs for genes of interest were quantified by real-time PCR using the Bio-Rad CFX96 real-time system and primers obtained from Integrated DNA Technologies (Coralville, IA) (Predesigned qPCR Assays). All results were normalized to the housekeeping gene β-actin.
RNA Interference
ON-TARGETplus rat Nr1i2 siRNA SMARTpool (L-099761-02) and ON-TARGETplus non-targeting siRNA (D-001810-01) were purchased from Dharmacon (Lafayette, CO). Small interfering RNA was transfected into IEC-6 cells for 48 h using Lipofectamine 2000 transfection reagent (ThermoFisher, Waltham, MA), followed by treatment as indicated.
Induction of Experimental Mouse Necrotizing Enterocolitis
Experimental NEC was induced in 7-day-old mice (WT or PXR−/−) using a protocol similar to that previously reported (5, 6, 7, 20, 21). NEC formula (Similac (Abbott Nutrition, Columbus, OH) PM60/40 infant formula: Esbilac (PetAg, Hampshire, IL) canine milk replacer, 2:1) was supplemented with enteric bacteria made from a stock created from a stool specimen obtained from an infant with surgical NEC (12.5 μl stool slurry in 1 ml formula) and fed by oral gavage five times per day (50 μl per g mouse body weight). The mice also were exposed to hypoxia (5% O2, 95% N2) for 10 min twice daily for up to 4 days using a hypoxic chamber (Billups-Rothenberg, Del Mar, CA). Previous studies have demonstrated that this experimental NEC protocol induces intestinal inflammation and production of inflammatory cytokines that closely resembles human NEC (5, 6, 7, 20, 21). Control mice remained with their mothers and were breast-fed ad libitum. After killing, terminal ileums were harvested 1 cm proximal to the ileocecal valve and fixed in 10% formaldehyde for histologic assessment or frozen in liquid nitrogen for quantitative real-time PCR. The severity of disease was determined on histologic sections stained with hematoxylin and eosin by a blinded investigator based on a previously published NEC scoring system from 0 (normal) to 3 (severe) (5). Immunohistochemistry was performed essentially as described (25). Formalin-fixed paraffin-embedded sections of mouse small intestine underwent antigen retrieval at pH 6 in Dako target retrieval solution (Dako, Carpinteria, CA) and incubated with a 1:200 dilution (1 μg/ml) of polyclonal rabbit anti-mouse PXR (Cloud Clone, Houston, TX). This primary antibody was detected with EnVision+ System-HRP anti-rabbit reagent (Dako) and visualized with a DAB substrate kit (Cell Marque, Rocklin, CA). PXR staining intensity was determined by scanning slides on the 3DHistec Pannoramic 250 Flash II slide scanner (SIG #1S10OD019961-01) in the Analytical Imaging Facility at Albert Einstein College of Medicine.
Isolation of Nuclei and Nuclear Run-On Assay
These assays were performed according to the methods previously published (26) with minor modifications. Nuclei were isolated from cultured LS174T cells and immediately stored at −80 °C until analysis. For nuclear run-on assay, identical number of LS174T nuclei was used for preparation of nascent transcripts. To perform the nuclear run-on transcription, 5 × 106 nuclei were incubated in a reaction buffer (5 mM Tris-HCl, pH 8.0, 2.5 mM MgCl2, 150 mM KCl, 1.0 mM each of ATP, GTP, CTP) and 0.5 mM biotin-16-UTP at 30 °C for 45 min in a final volume of 25 μl. The reaction was stopped by the addition of 60 U RNase-free DNase and incubated further for 10 min at 37 °C. The nuclei were then lysed by the addition of lysis buffer containing 10 mM Tris-HCl, 1% SDS, 5 mM EDTA. The reaction mixtures were treated with 20 μl of proteinase K (10 mg/ml). RNA was extracted with TRIzol Reagent, ethanol-precipitated, and resuspended in 50 μl RNase-free water. Biotinylated RNA was purified by adding streptavidin beads, followed by 2 h incubation at 25 °C on a shaker. Beads were separated by centrifugation at 2,000 rpm for 5 min, and washed once with 2 × SSC-15% formamide for 10 min and twice with 2 × SSC alone for 5 min. Finally, beads were resuspended in 30 μl DEPC-treated water. The biotinylated RNA solution was used for reverse-transcriptase cDNA synthesis and further real-time qPCR for the quantitative mRNA assay.
Actinomycin D Chase
LS174T cells were plated into six-well tissue culture dishes and treated with rifampicin for 48 h. After rifampicin treatment, 20 μg/ml of Actinomycin D, dissolved in DMSO was added in each well and RNA isolated at different time points starting at t=0 after actinomycin D exposure. RNA was subsequently used for reverse transcription and real-time qPCR analysis.
Statistical Analysis
Statistical analysis was performed using Prism 7 software (GraphPad, La Jolla, CA). Data are expressed in mean±SEM as indicated. Two-tailed unpaired t-test was used for comparisons between two groups. Ordinary one-way analysis of variance (ANOVA) with Tukey’s post-test was used when comparing fold changes between multiple groups, whereas Kruskal–Wallis one-way ANOVA with Dunn’s post-test was used for multiple comparisons to a control group. Statistical significance was defined as a P value⩽0.05. The half-life of TLR4 mRNA was calculated according to the formula: t1/2=0.693/κ, where κ=ln(N0/Nt)t, with N0 being TLR4 mRNA expression at t=0 and Nt being TLR4 mRNA expressions at various time points.
Results
Reciprocal Relationship Between PXR and TLR4 in the Developing Murine Intestine
We first sought to characterize the relationship between expression of PXR and TLR4 in the developing intestine. To do so, ileal-jejunal tissues were harvested from prenatal (E16, E18) or postnatal (P1, P3, P7) WT mice, out to a time when mice are susceptible to experimental NEC (20, 21), to determine PXR and TLR4 transcript levels by quantitative real-time PCR (qRT-PCR). As shown in Figure 1a, intestinal TLR4 expression was highest during the early prenatal period and decreased following delivery. In contrast, PXR expression was lowest during the early prenatal period and increased robustly around the time of delivery. PXR target genes (Mdr1a and Cyp3a11) demonstrated a similar pattern of expression (Figure 1bi). These observations suggest a reciprocal relationship between the developmental expression of PXR and TLR4 in murine intestine.
To further explore this relationship, ileal-jejunal tissues were harvested from WT and PXR−/− mice from E18 to postnatal day 7 and analyzed for TLR4 expression. There were no differences in intestinal TLR4 expression between PXR−/− and WT mice at any of the time points evaluated (Figure 1c). Thus, despite the reciprocal relationship between expression of PXR and TLR4 in WT mice, the absence of PXR did not significantly impact baseline TLR4 expression during the prenatal or early postnatal periods.
PXR Negatively Regulates the TLR4 Pathway by Decreasing TLR4 mRNA Stability
Given the observed inverse relationship between expression of PXR and TLR4 in the developing intestine, we next sought to better define the mechanism(s) by which PXR regulates the TLR4 pathway. To determine whether PXR regulates TLR4 at the transcriptional level, we performed nuclear run-on analysis using human colon epithelial LS174T cells treated with the human PXR agonist rifampicin (27). As shown in Figure 2a, upon activation of PXR with rifampicin, we observed a steady increase in MDR-1 gene transcription but no change in TLR4 transcription (Figure 2a). We then considered the possibility that PXR acts post-transcriptionally to attenuate expression of TLR4. To this end, we conducted Actinomycin D chase experiments and found that rifampicin treatment decreased the half-life of TLR4 mRNA by ~47% compared to untreated cells (Figure 2b). Together, these observations show that the effect of PXR activation by rifampicin on TLR4 gene expression in not a direct transcriptional event, but instead it is due to a PXR-mediated post-transcriptional effect on TLR4 mRNA stability.
WT Mice Demonstrate Reduced PXR Protein Expression and PXR-Deficient Mice Demonstrate a Heightened Inflammatory Response During Experimental NEC
It is known that there is mutual repression between the TLR4 and PXR signaling pathways (14, 15). Given the critical involvement of TLR4 signaling to NEC pathogenesis, we next sought to determine whether exposure to NEC-associated intestinal inflammation would alter PXR expression and whether the absence of PXR would increase susceptibility to NEC. Experimental NEC was induced in WT and PXR−/− pups using a well-characterized model that involves gavage feeding with formula and exposure to twice-daily hypoxia (5, 6, 7, 20, 21). In this model, WT mice demonstrate severe intestinal inflammation by day 4; thus we killed some mice at earlier time points to clarify the inflammatory processes that underlie the development of full-blown disease. We first examined intestinal tissues from WT control (breastfed) and WT NEC mice that were immunostained for PXR. As shown in Figure 3a, at an early stage (day 2) of the NEC protocol, WT control mice demonstrated PXR-positive stain intensity that was almost two-fold higher than that found in WT NEC mice (31.52% vs. 17.27%).
We next compared WT NEC mice to PXR−/− NEC mice at a similar early stage of the NEC protocol. As shown in Figure 3b–d, by gross inspection and histopathological assessment, the gut injury was more severe in the PXR−/− mice. Experimental NEC also induced a profound increase in transcripts for the proinflammatory cytokine IL-6, which was ~10-fold greater in intestinal tissues obtained from PXR−/− mice as compared to WT mice. Exposure to the NEC protocol also resulted in a significant increase in TLR4 expression in WT mice, which was markedly exacerbated in the absence of PXR (Figure 3ei). These observations indicate that intestinal proinflammatory cascades progress faster in the absence of PXR and further suggest, consistent with other studies (9, 10, 14), that PXR suppresses TLR4 signaling in NEC-associated inflammation. Additionally, markers of intestinal barrier function were more notably disrupted in PXR−/− mice. Experimental NEC resulted in reduced levels of MUC2, a predominant secretory mucin produced by goblet cells, in PXR−/− mice as compared to WT mice (Figure 3eiii). At baseline, connexin-43 (Cx43), the major connexin involved in maintaining gap-junctional intercellular communication, was lower in PXR−/− control mice vs. WT controls, but then dramatically increased in PXR−/− mice subjected to experimental NEC (Figure 3eiv), which could indicate gap-junction disassembly with accumulation of dysfunctional isoforms (28).
LCA Activates Intestinal PXR and Suppresses LPS-Induced Proinflammatory Cytokine Expression In Vitro
To study the physiological function of intestinal PXR in vitro, we treated IEC-6 enterocytes with the secondary bile acid LCA, a known PXR agonist in liver (11). (Figure 4ai) shows that LCA stimulated the transcription of PXR and Mdr1a, a major gene target of PXR, in a dose-dependent manner, indicating that LCA treatment promotes activation of PXR in intestinal epithelial cells. Evidence of developing toxicity was observed when LCA concentrations exceeded >200 μM, thus for subsequent in vitro experiments, LCA was used at concentrations below this threshold. To examine the potential of PXR to suppress TLR4 signaling cascades, we pretreated IEC-6 cells with LCA prior to the stimulation with LPS. (Figure 4bi) shows that LCA pretreatment reduced the LPS-induced transcription of both IL-6 and TNFα by ~50% (P<0.05 and P<0.01, respectively).
LCA Suppresses LPS-Induced IL-6 Transcription in a PXR-Dependent Manner
It is known that LCA can activate intestinal receptors other than PXR, such as the vitamin D receptor (29). Therefore, we next sought direct evidence that the ability of LCA to suppress LPS-induced proinflammatory responses in intestinal tissues was PXR-dependent. To do so, we knocked down PXR in IEC-6 enterocytes using PXR-specific siRNA. Following the knockdown, IEC-6 cells exposed to LCA demonstrated a three-fold reduction in PXR mRNA as compared to those treated with scrambled siRNA (data not shown). Under conditions of reduced PXR expression, LCA pretreatment no longer suppressed LPS-induced transcription of IL-6; instead, an enhancement in the levels of IL-6 transcripts was observed (Figure 5ai). In contrast, LCA still suppressed the LPS-induced transcription of TNFα (Figure 5aii), suggesting that IL-6 and TNFα are differentially regulated downstream of TLR4 signaling cascades. In this series of experiments, the induction of proinflammatory transcripts following stimulation of IEC-6 cells with LPS was less pronounced than in Figure 4b; however, the results were suggestive that LCA may diminish the LPS-induced transcription of IL-6 in intestinal tissues via PXR.
To further investigate this possibility, we isolated primary intestinal organoids (30) from WT and PXR−/− mice, and exposed them to LPS following pretreatment or not with LCA. As shown in Figure 5bi, LCA pretreatment of WT intestinal organoids reduced LPS-induced transcription of IL-6 by over 90%. In contrast, LCA pretreatment did not alter LPS-induced transcription of IL-6 in intestinal organoids generated from PXR−/− mice (Figure 5bii). This result strongly suggests that LCA suppression of LPS-induced IL-6 expression in intestinal tissues is PXR-dependent. LCA did not alter LPS-induced transcription of TNFα in WT intestinal organoids (Figure 5biii), providing additional evidence that transcription of this cytokine is regulated downstream of TLR4 signaling in a PXR-independent manner and potentially by an LCA receptor that is present in rat IEC-6 cells but absent in murine intestinal organoids.
LCA Reduces Intestinal Transcription of IL-6 and TLR4 at an Early Stage of Experimental NEC in a PXR-Dependent Manner
In the next series of experiments, we sought to determine whether LCA could protect against NEC-associated inflammation in a PXR-dependent manner. WT and PXR−/− mice were subjected to the NEC protocol described previously (5, 6, 7, 20, 21); however, in this series, formula mixtures administered by oral gavage were supplemented or not with 0.5% LCA. At an early stage (day 2) following initiation of the NEC protocol, the transcription of IL-6 and TLR4 in the terminal ileums of WT mice receiving LCA was reduced compared to WT mice not given LCA, indicating that LCA protected against the upregulation of these proinflammatory markers (Figure 6ai). In contrast, LCA failed to reduce these proinflammatory markers in the terminal ileums of PXR−/− mice (Figure 6bi). This observation suggests that during early stages of NEC-associated inflammation, LCA-mediated reduction in IL-6 and TLR4 is PXR-dependent. Despite these reductions, there was no difference in histologic grading of NEC severity (Figure 6c). Furthermore, as NEC progressed to late stage (day 4), the levels of transcripts for IL-6 and TLR4 were comparable between LCA and non-LCA fed WT mice (Figure 6di).
Discussion
Excessive stimulation of TLR4 within the intestinal epithelium is speculated to serve as a prequel to NEC by initiating signaling cascades that result in intestinal barrier breakdown (5, 6, 7). Subsequently, bacterial translocation and propagation of the profound inflammatory response to infiltrating bacteria leads to intestinal necrosis and the systemic manifestations that are characteristic of this disease (1). Inhibition of TLR4 signaling in the intestinal epithelium has been shown to enhance enterocyte proliferation and limit enterocyte apoptosis (6, 21, 31), and could therefore be utilized as a potential route for NEC prevention (21). In this study, we evaluated the capacity of PXR, a xenobiotic sensor and negative regulator of TLR4 signaling (9, 10), to limit NEC-associated inflammatory pathways. We show that a reciprocal relationship exists between the developmental expression of intestinal PXR and TLR4, PXR protein levels are reduced in WT mice subjected to experimental NEC, and that PXR-deficient mice exhibit a remarkably heightened inflammatory response following exposure to the NEC protocol. Moreover, we provide evidence that the secondary bile acid and commensal byproduct, LCA, reduces NEC-associated intestinal inflammatory responses in a PXR-dependent manner. Taken together, these findings suggest that targeting intestinal PXR may be a novel approach to reduce intestinal injury in conditions, such as NEC, that are attributed to excessive TLR4 stimulation. It is known that following ligand binding, PXR heterodimerizes with retinoid X receptor (RXR) to form a PXR/RXR complex, which directly interacts with the p65 subunit of NF-κB thereby limiting TLR4 signaling cascades (8, 32). Here we provide evidence that at least one additional mechanism for PXR to limit NEC-related inflammatory responses is via the regulation of TLR4 mRNA stability.
In both humans (4) and mice (33), intestinal expression of TLR4 is higher early in gestation compared to later time points, which suggests a developing role for TLR4 in epithelial differentiation. The possibility exists that elevated expression of TLR4 in the preterm intestine is the normal state and that pathology arises from a combination of premature delivery and postnatal microbial colonization. Nevertheless, only ~5–10% of the most susceptible infants develop NEC (1), which suggests that protective mechanisms exist to suppress the deleterious effects of TLR4 activation. Our data support the notion that PXR is a central regulator of TLR4-mediated control of intestinal barrier function (9) and expand the spectrum of intestinal disorders in which PXR may play a protective role to include NEC (9, 16, 17, 18). In WT intestinal tissues, the robust increase in PXR transcripts, and PXR-target genes Mdr1a and Cyp3a11, noted shortly after delivery coincided with a reduction in TLR4. Our discovery that PXR regulates TLR4 mRNA stability further suggests that accumulation of xenobiotic PXR agonists in the postnatal intestine may serve as a switch to limit TLR4 expression after birth. Additionally, in the absence of PXR, mice subjected to NEC had a marked increase in TLR4 expression compared to WT mice and demonstrated increased susceptibility to intestinal injury.
Prior to the induction of experimental NEC, we compared baseline levels of transcripts for proteins associated with intestinal inflammation or barrier homeostasis in PXR−/− vs. WT mice, as an indicator of their vulnerability to intestinal injury during the perinatal period. We observed no elevation in baseline levels of TLR4 transcripts in prenatal or early postnatal PXR−/− mice compared to age-matched WT controls. This is in contrast to a recent report that utilized adult PXR−/− mice, in which the absence of PXR was associated with increased baseline enterocyte TLR4 expression (9). It is possible that insufficient levels of commensal microbiota were present during the perinatal period to induce TLR4 expression over WT mice. Additional mechanisms of early postnatal intestinal TLR4 control, such as epidermal growth factor (EGF) ingested with the breast milk may also be involved (21). Nevertheless, because our model includes gavage feeding with enteric bacteria isolated from a preterm infant with NEC, the observed increase in TLR4 mRNA following initiation of the NEC protocol strongly suggests that microbiota-derived signals play a major role in regulating TLR4 expression, particularly in the setting of reduced PXR activity.
The possibility that intestinal dysbiosis contributes to NEC susceptibility is supported by several studies demonstrating that the fecal microbiome of infants that develop NEC is dominated by LPS-containing Proteobacteria (34, 35). Alternatively, an abundance of strict anaerobes is negatively associated with NEC, which suggests that these bacteria and/or their products may trigger protective mechanisms (35). In our study, we used the secondary bile acid and known liver PXR agonist, LCA, to evaluate its ability to dampen NEC-associated intestinal inflammation. LCA is produced from the conversion of primary bile acids by commensal bacteria possessing 7α-dehydroxylase activity (36); of the various bacteria inhabiting the human intestine, several strains of Clostridium (36, 37) and Bacteroides (38) possess 7α-dehydroxylase activity. Both ex vivo experiments and analysis of intestinal tissues obtained from early NEC show that LCA diminishes intestinal proinflammatory responses in a PXR-dependent manner. Conversely, LCA did not reduce histologic severity or alter intestinal proinflammatory responses at later time points. This likely reflects the nature of the model, which involves repeated, combined insults to the intestine, surpassing LCA’s protective effects. Alternatively, the reduction in PXR expression following initiation of the NEC protocol may account for decreased responsiveness to LCA. It is conceivable that providing higher doses of LCA would result in greater levels of protection; however, high doses of LCA are also associated with liver toxicity (11). In future studies, additional PXR ligands with greater activating potential or lower levels of systemic toxicity should be evaluated for their capacity to protect against NEC. It was recently demonstrated that tryptophan metabolites (e.g., Indole 3-propionic acid) produced by intestinal commensals regulate intestinal barrier function through PXR (9, 39). The combined influence of microbial small molecule output on NEC susceptibility is an intriguing area of investigation.
Interestingly, Cx43 mRNA was significantly reduced in PXR−/− mice as compared to WT controls, but then demonstrated a profound increase upon the induction of experimental NEC. Cx43 is the most abundant connexin regulating gap junction communication between enterocytes, and protein levels are reported to be reduced in experimental NEC and patients with IBD (40). It is known that Mdr1a-deficient mice, which develop spontaneous colitis, have accumulation of differentially phosphorylated isoforms of Cx43 representing a marker of gap junction disruption during intestinal injury (28). Thus, under conditions of cellular stress, the absence of PXR, which regulates Mdr1a activity, may also result in the accumulation of dysfunctional isoforms of Cx43. This possibility remains to be determined but could account for the large increase in Cx43 transcripts measured by RT-PCR. There were no differences in baseline levels of IL-6 or MUC2 transcripts between PXR−/− and WT mice; however, their pattern of expression following the induction of NEC were consistent with greater levels of intestinal damage in the PXR−/− mice.
Despite the established association between reduced PXR expression and IBD (16, 17), there have been no studies evaluating the contribution of PXR in human NEC. It is interesting to note that while PXR agonists can protect against DSS-induced colitis, PXR-deficient mice do not show increased susceptibility to this model of distal colonic injury (18). In contrast, in animal models, small intestinal disease appears to be enhanced in the absence of PXR (9, 14). This suggests that the large intestine, as compared to the small intestine, may have compensatory mechanisms in place that can be activated in the absence of PXR (18). NEC involves the small bowel and ileocecal junction more often than the large bowel, supporting the notion that PXR may play a regulatory role in NEC pathophysiology at these anatomic sites. Furthermore, compensatory mechanisms may not be fully established in the preterm infant, in which case the protective effect of PXR signaling may be more critical in the large bowel.
In summary, we have now expanded the role of PXR as a central regulator of TLR4 signaling to include suppression of inflammatory pathways in the early phase of experimental NEC. Further studies will determine if PXR plays a similar regulatory role in human NEC and explore the potential utility of microbiome-, pharmacologic- or dietary-related PXR agonists as novel approaches for preventing this devastating condition of prematurity.
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Acknowledgements
We gratefully acknowledge David Hackam and his laboratory staff, Johns Hopkins Children’s Center, for their advice in performing the NEC model; and Justin Radolf, University of Connecticut School of Medicine, for his mentorship and review of the manuscript.
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The authors declare no competing financial interests.
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STATEMENT OF FINANCIAL SUPPORT:
This work was supported by funds made available through a Connecticut Children’s Medical Center Young Investigator Award (A.P.M.), NCI P30CA013330 (Analytical Imaging Facility at the Albert Einstein College of Medicine, V.D., S.M.), SIG#1S10OD019961-01 (Analytical Imaging Facility, V.D.), Broad Medical Research Program (#362520; S.M.), R01 CA161879 (S.M.) and Department of Defense Grant# PR160167 (K.M.K., S.M.).
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US patent application # PCT/US2013/072709 filed by Albert Einstein College of Medicine on behalf of S.M. and S.M. (https://www.google.com/patents/WO2014088982A1?cl=en).
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Huang, K., Mukherjee, S., DesMarais, V. et al. Targeting the PXR–TLR4 signaling pathway to reduce intestinal inflammation in an experimental model of necrotizing enterocolitis. Pediatr Res 83, 1031–1040 (2018). https://doi.org/10.1038/pr.2018.14
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DOI: https://doi.org/10.1038/pr.2018.14
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