Abstract
Background
Preterm infants are at high risk of infection and have distinct pathogen recognition responses. Suggested mechanisms include soluble mediators that enhance cellular levels of cAMP. The aim of this study was to assess the relationship between blood cAMP concentrations and TLR-mediated cytokine production in infants during the first month of life.
Methods
Cord and serial peripheral blood samples (days of life 1–28) were obtained from a cohort of very preterm (<30 weeks’ gestational age) and term human infants. Whole-blood concentrations of cAMP and FSL-1 and LPS in vitro stimulated cytokine concentrations were measured by ELISA and multiplex bead assay.
Results
cAMP concentrations were higher in cord than in peripheral blood, higher in cord blood of female preterm infants, and lower at Days 1 and 7 in infants exposed to chorioamnionitis, even after adjusting for leukocyte counts. TLR2 and TLR4-mediated TNF-α, IL-1β, IL-6, IL-12p70, and IL-10 production in vitro increased over the first month of life in preterm infants and were positively correlated with leukocyte-adjusted cAMP levels and reduced by exposure to chorioamnionitis.
Conclusions
The ontogeny of blood cAMP concentrations and associations with chorioamnionitis and TLR-mediated production of cytokines suggest that this secondary messenger helps shape distinct neonatal pathogen responses in early life.
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Introduction
Newborn infants, especially those born preterm are particularly susceptible to invasive infections; up to 60% of the most premature infants (<28 weeks’ gestational age (GA)) have at least one sepsis episode during their hospital admission.1 Immune responses in preterm infants are distinct from those of term infants, older children, and adults and contribute to the increased risk of invasive infection in this population.2 Importantly, dysregulated infection-related inflammation is associated with adverse long-term outcomes in preterm infants.3,4
The mechanisms sha** the ontogeny of early life immune responses, particularly in preterm infants, are incompletely understood. Gestational age-dependent maturation of responses to innate immune pattern recognition receptor (PRR) stimulation may be critical for susceptibility to invasive infections and associated outcomes. Prior studies have demonstrated gestational age-specific functional differences in the innate immune response to PRR stimulation.5 In vitro studies have implied a role for soluble mediators, as age-specific differences in response to stimulation were found to be dependent on the use of autologous or age-matched plasma in these experiments.6,7
Neonatal plasma contains multiple immunomodulating factors, including adenosine, that is present in markedly elevated concentrations compared to adults.8,9,10 Adenosine enhances production of cyclic adenosine mono-phosphate (cAMP), a key component of intracellular signaling pathways. Extracellular stimuli such as adenosine activate adenylate cyclase, which in turn generates cAMP and pyrophosphate.11,12 cAMP may modulate innate and inflammatory responses to whole microbes, microbial products, or vaccine adjuvants (e.g., certain Toll-like receptor (TLR) agonists) with implications for sepsis pathophysiology as well as adjuvanted vaccine design.9 Whether induced physiologically by adenosine or pharmacologically by phosphodieseterase inhibitors, cAMP inhibits production of pro-inflammatory cytokines (e.g., tumor necrosis factor (TNF), interferons) but preserves or enhances the production of acute-phase cytokines such as interleukin (IL)-6 and regulatory cytokines, such as IL-10.2,13,14,15
Most mechanistic studies of early-life immune ontogeny have focused exclusively on cord blood16; however, risk of infection persists throughout the neonatal period and in preterm infants is the highest between 10 and 14 days of age.17 We therefore evaluated the concentrations of circulating cAMP (cellular and extracellular) in the first month of life and their correlation with TLR2 and TLR4-mediated in vitro cytokine production in a prospective longitudinal study.
Methods
Study subjects
This longitudinal observational cohort study was approved by the institutional ethics committee at King Edward Memorial Hospital, Perth, Australia (1627/EW) and written informed consent was obtained from parents prior to study participation. One hundred and twenty-nine infants born at <30 weeks’ GA and 20 term infants (37–41 weeks’ GA) without major congenital abnormalities or chromosomal aberrations were recruited into this study. Serial blood samples were collected from recruited preterm infants from cord and peripheral blood on days of life (DOL) 1, 7, 14, 21, and 28. For ethical reasons, blood collection from recruited healthy term infants was limited to cord and peripheral blood on Days 1 and 28. Infants were determined to have an episode of confirmed late-onset sepsis (LOS; onset >72 h after birth) based on a positive blood culture and C-reactive protein (CRP) concentration >15 mg/dL during sepsis evaluation. Those with negative blood cultures but with CRP >15 were deemed to have clinical LOS. Table 1 describes the basic clinical characteristics of the study cohort.
Blood sampling and preparation
Infant cord and peripheral blood (800 μL) for whole-blood stimulation and white blood cell extended differential counts was collected by venipuncture or from an existing umbilical catheter (DOL 1 only) on Days 7, 14, 21, and 28 into lithium-heparin tubes (Becton Dickinson, North Ryde, Australia).
An additional 400 μL of infant blood was collected, as above, into lithium-heparin tubes containing 2 µL of 2 mM dipyridamole (in dimethyl sulfoxide; Sigma-Aldrich, Castle Hill, Australia) and 2 µL of 200 µM erythro-9-(2-hydroxy-3-nonyl) adenine hydrochloride (in water; Sigma-Aldrich). Samples were centrifuged at 6000 × g for 2 min and plasma was removed. Blood cell pellets were resuspended in 1 ml 0.1 M HCL and incubated at room temperature (RT) for 20 min. These samples were centrifuged at 1000 × g for 10 min and supernatant (blood lysate) was stored at −80 °C until cAMP measurement.
Placental histology
Placental histology was examined as part of routine clinical care from pregnancies delivering <30 weeks’ GA. Sections of the chorioamniotic membranes, umbilical cord, chorionic plate, and placenta were analyzed using an adaptation of a widely accepted semi-quantitative scoring system, as previously described.18,19
cAMP determination
cAMP in blood lysates was quantified using a cyclic AMP ELISA Kit in accordance with the manufacturer’s instructions (Cayman Chemical, Ann Arbor, MI; lower limit of detection, 0.3 pmol/mL).
Whole-blood stimulation
Twenty-five μL of whole blood was cultured in 75 μL RPMI 1640 GlutaMAX, supplemented with 0.01 M HEPES, 1 mM sodium pyruvate, and 5.5 μM beta-mercaptoethanol (all from Gibco, Life Technologies, Mulgrave, Australia), 24 h at 37 °C and 5% CO2 with either supplemented RPMI media, 10 ng/mL lipopolysaccharide (LPS) and 100 ng/mL fibroblast-stimulating lipopeptide-1 (FSL-1; both from Invivogen, San Diego, CA). Following overnight incubation, 100 μL of RPMI 1640 supplemented as above along with the addition of 5% fetal bovine serum (SAFC Biosciences, Lenexa, KS) was added and supernatants harvested and stored at −80 °C.
Multiplex cytokine assay
Cytokine production following stimulation was quantified using a validated in-house multiplex bead-based assay.20 Primary antibodies against IL-1β and IL-12p70 (R&D Systems, Minneapolis, MN) and IL-6, IL-10, and TNF-α (BD Biosciences, North Ryde, Australia) were covalently conjugated to carboxylated microspheres (Luminex Corporation, Austin, TX). Supernatants were diluted in phosphate-buffered saline (PBS) with 0.05% (v/v) Tween20 and 2% (v/v) newborn bovine serum (all from Sigma-Aldrich). Microspheres, at a concentration of 3500 per bead region, and diluted samples were transferred to MV Multiscreen plates (Merck-Millipore, Bayswater, Australia) and incubated at RT for 30 min on an orbital shaker (500 rpm), protected from light. Biotinylated secondary antibodies against IL-1β and IL-12p70 (R&D Systems) and IL-6, IL-10, and TNF-α (BD Biosciences) were then added, and the plate was incubated for another 30 min at RT (500 rpm, in the dark). Wells were washed with PBS containing 1% (w/v) bovine serum albumin, 0.25% (v/v) Tween20, and 0.001% (w/v) NaN3 vacuum filtration before a streptavidin–phycoerythrin (PE) conjugate (BD Biosciences) was added for 15 min with shaking. Wells were washed twice as above, and the fluorescence in each bead region was measured on a BioPlex 200 System (Bio-Rad, Gladesville, Australia). Data were acquired electronically in real time and analyzed using the BioPlex Manager 5.0 software. Data in pg/mL were generated from seven-point and four- or five-parameter logistic standard curves. All values below the lowest standard were assigned an arbitrary cut-off value of half the lowest detectable standard for analysis.
White blood cell enumeration by extended differential count
Whole-blood samples were surface stained with antibodies targeting common leukocyte markers used in the validated method by Faucher et al.21 In brief, 25 μL of whole blood was stained with a cocktail of the following monoclonal antibodies: PE-conjugated CD36 (CD36-PE, clone CD38, mouse anti-human), allophycocyanin (APC)-conjugated CD2 (CD2-APC, clone S5.2,9 mouse), Alexa Fluor 647 (AF647)-conjugated CD294 (AF647-CD294, clone BM16, rat anti-human), APC-H7-conjugated CD16 (APC-H7-CD16, clone 3G8, mouse anti-human), BD Horizon V450 (V450)-conjugated CD19 (V450-CD19, clone HIB19, mouse anti-human), AmCyan-conjugated CD45 (AmCyan-CD45, clone 2D15, mouse anti-human). Following 15-min incubation, red blood cells were lysed with 1 ml BD FACS Lysing Solution for 10 min in the dark at RT. Cells were then washed with FACS buffer (PBS, 2% w/v BSA, 0.01% w/v sodium azide from Sigma-Aldrich and 2% v/v fetal calf serum from SAFC Biosciences) and resuspended in BD Stabilizing Fixative with a known volume transferred to BD TruCOUNT Tubes, to allow for absolute counts of each cell type, and stored at 4 °C in the dark prior to analysis. Spectral compensation for each antibody was achieved using BD CompBeads. All antibody clones and flow cytometric reagents were obtained from BD Biosciences, unless otherwise stated.
White blood cells were analyzed using a three-laser, eight-color BD FACSCanto II flow cytometer and BD FACSDiva software (BD Biosciences). Prior to acquisition flow cytometer calibration was performed using SPHERO Ultra Rainbow Calibration beads (Spherotech, Lake Forest, IL), in addition to BD Cytometer Setup and Tracking beads (BD Biosciences) to monitor cytometer performance. Post-acquisition cell population analysis was performed using the FlowJo software version 8 (Tree Star Inc., Ashland, OR). Various leukocyte populations were identified using the validated gating strategy described by Faucher and colleagues.21 In brief, the following cell types were identified from the white blood cell count (WCC; CD45+) population: neutrophils (SSChigh/CD16+), non-cytotoxic T cells (SSClow/CD16− → CD2&CD294+/SSClow), classical monocytes (SSClow/CD16− → CD2&CD294− → CD19−/CD36+).
Statistical analysis
For longitudinal analysis of cAMP concentrations in blood lysates, values were log-transformed to satisfy distributional requirements and analyzed by fitting a mixed model with the Geisser–Greenhouse correction as implemented in GraphPad Prism version 8.0 (San Diego, CA). This mixed model uses a compound symmetry covariance matrix and is fit using Restricted Maximum Likelihood. In the presence of random missing values (as was the case in this study), the results can be interpreted as for repeated-measures analysis of variance. Correlations of cAMP and cell counts were determined using Spearman correlation test. We controlled for total cell counts when assessing cytokine responses by dividing the cytokine values by the total leukocyte counts and log-transformed this ratio, as well as the cAMP values, and calculated corresponding Spearman correlation coefficients. Comparison of the means between two groups was done using Mann–Whitney U test.
Results
cAMP concentrations after birth
The demographics of the study population are listed in Table 1. cAMP concentrations were significantly higher in cord blood than in peripheral blood in term infants but not in preterm infants (Fig. 1a). The concentration of cAMP in the cord blood of term infants (median 10.7 mmol/L, range 1.4–207.3, n = 16) was higher than that in preterm infant cord blood (median 2.4 mmol/L, range 0.4–40.05; n = 37, P = 0.0028) but was not different in peripheral blood on DOL1 (median 2.2 vs 2.8 mmol/L; n = 15 and 109, respectively) or DOL28 (median 2.5 vs 2.3 mmol/L; n = 11 and 102, respectively).
WCCs in cord blood and DOL1 peripheral blood were also higher in term infants compared to that in preterm infants (6.9 × 109 cells/L vs 3.4 × 109 cells/L, n = 15 and 32, P < 0.0001; and 10 × 109 cells/L vs 5.5 × 109 cells/L, n = 15 and 109, P = 0.0001, for cord and DOL1, respectively). This prompted us to examine the associations between cAMP concentrations and differential WCCs (Table 2). cAMP levels in cord blood were positively correlated with the absolute numbers of total white blood cells as well as with the counts for neutrophils, classical monocytes, and B cells. cAMP concentrations in peripheral blood showed positive correlations with total white blood cell, neutrophil, and inflammatory monocyte counts on DOL1 and DOL7 and with classical monocyte and B cell counts on DOL7. cAMP concentrations on DOL14 were negatively correlated with non-cytotoxic T cell counts.
Given the positive associations between cAMP concentrations and WCCs, we examined WCC-corrected cAMP concentrations (pmol/cell) in cord and peripheral blood samples (Fig. 1b). The cell corrected concentration of cAMP was still higher in term cord blood than in DOL1 peripheral blood but there was no longer a difference with DOL28 blood. However, the leukocyte-corrected concentration of cAMP in preterm infant cord blood was now higher than in peripheral blood throughout the 28-day postnatal period (P < 0.01). The cell-corrected concentrations of cAMP in cord, DOL1, and DOL28 did not differ between term and preterm infants.
cAMP correlates with TLR2- and TLR4-mediated cytokine production in preterm infants
To characterize innate immune responses in early life, cord and peripheral blood was stimulated in vitro with FSL-1 (TLR2/6 agonist) or LPS (TLR4 agonist) and cytokines measured in supernatant by multiplex assay (Fig. 2). The levels of LPS-induced TNF-α, IL-1β, IL-6, and IL-10 were higher in term infant peripheral blood than in the equivalent preterm infant blood samples (P < 0.05 for IL-10 at DOL28, P < 0.005 for remaining cytokines). Cord blood IL-1β, IL-6, and IL-10 levels were also higher in term infants than in preterm infants after LPS stimulation (P < 0.001). TNF-α, IL-1β, IL-6, and IL-10 levels were also higher in term infants than in preterm infants after FSL stimulation, and this was most marked for IL-6 and IL-10 in cord blood and DOL1 blood (P < 0.05), for TNF-α on DOL1 and DOL28 (P < 0.05), and for IL-1β on DOL1 (P < 0.0001). IL-12p70 levels did not differ between preterm and term infants. LPS consistently induced higher levels of all cytokines than FSL at each time point in both preterm and term infants.
LPS-stimulated cytokine levels in preterm infants were lower in peripheral blood on DOL1 than in cord blood and then increased over the first month of life (Fig. 2). The same pattern was seen for TNF-α and IL-6 after LPS stimulation and for IL-10 after FSL stimulation. IL-12p70 levels were higher in preterm infant cord blood than in peripheral blood on DOL1 after LPS and FSL stimulation, as was TNF-α after LPS stimulation.
We next assessed whether cAMP concentrations in cord and peripheral blood were associated with LPS- and FSL-induced cytokine production. Owing to the positive correlations of cAMP concentrations with WCCs, we assessed all associations using cytokine and cAMP values after correction of each for leukocyte count. Overall, cell-corrected cAMP levels in preterm infant peripheral blood showed a weak-to-moderate correlation with cell-corrected cytokine production from DOL1 onwards after FSL stimulation and DOL7 onwards with LPS stimulation (Table 3a, b). Consistent with our previously published studies of term newborns,9 LPS-induced TNF-α production in term cord blood was negatively correlated with cAMP, whereas DOL1 IL-10 responses were positively correlated. No other term LPS cytokine responses correlated with cAMP and term FSL-induced cytokine responses did not correlate with cAMP levels.
cAMP concentrations in preterm infants correlate with sex and chorioamnionitis
We next examined the potential effects of common immunologically relevant clinical parameters on cell-corrected preterm cAMP levels. cAMP concentrations in cord and peripheral blood showed no correlation with GA or birth weight. Further, there was no effect of mode of delivery, multiple birth status, or subsequent diagnosis of LOS (P > 0.05, data not shown). In contrast, cAMP levels were twofold higher in female compared to male preterm infant cord blood (median 1.15 vs 0.54 pmol/cell; ranges 0.27–3.73 vs 0.19–11.3 pmol/cell; P = 0.04, n = 14 and 18, respectively), but these differences were not observed in peripheral blood. cAMP levels were lower in peripheral blood on DOL1 and DOL7 in infants exposed to chorioamnionitis compared to unexposed infants (Fig. 3a). In kee** with the positive association between cell-corrected cAMP and cytokine production, LPS-induced cytokine levels were also lower on DOL1 and 7 in infants exposed to chorioamnionitis compared to those who were unexposed (Fig. 3b–f). The same pattern was also seen for TNF-α and IL-12p70 after FSL stimulation (data not shown).
Discussion
To our knowledge, this is the first study to determine total cAMP concentration in human preterm and term infant cord and peripheral blood during the neonatal period and to characterize the association with TLR2- and TLR4-mediated cytokine production. The second messenger cAMP is a key regulator of cellular functions, including metabolism, gene expression, and immune function.22,23 Increases in intracellular cAMP generally dampen production of pro-inflammatory/Th1-polarizing cytokines, but in vitro animal and human adult data may not reflect the effects in neonates, due to well-recognized age- and species-specific differences.13
In this unique large longitudinal cohort of preterm and term neonates, we found higher cAMP concentrations in term infant cord blood followed by significantly lower levels in peripheral blood on DOL1 and DOL28. We also observed that cAMP concentrations were positively correlated with WCCs, and following adjustment, cAMP concentrations in preterm infant cord blood were also higher than in peripheral blood at DOL1–28. This may reflect the dynamics of neonatal immune ontogeny of immunomodulatory molecules that induce cAMP production, including adenosine.8,9,14 Exposure to chorioamnionitis was associated with lower cell-corrected cAMP concentrations in peripheral blood at DOL1 and DOL7 and with lower TLR-induced cytokine concentrations, suggesting that cAMP may play a regulatory role in fetal and early postnatal life (Fig. 3). For example, intrauterine inflammation plays a key role in the initiation of preterm delivery and inadequately regulated inflammatory responses are associated with increased risk of common adverse prematurity-related outcomes.24
Of note, cell-corrected cAMP levels in cord blood were twofold higher in female than in male neonates. This is in line with emerging evidence that immune function is significantly influenced by sex, but little is known about relevance of sex-specific regulation of neonatal immunity.25,26 Several sex hormones impact key immune cell functions and the expression of X-linked immune genes contribute to sex-specific immune responses.25,27 While the mechanisms underlying sex differences in neonatal immunity are largely unknown, our observation of lower cAMP concentrations in male cord blood is consistent with distinct inflammatory responses that could contribute to poorer short- and long-term outcomes in male newborns.28,29,30
cAMP concentrations in preterms were positively correlated with peripheral blood TLR2- and TLR4-induced IL-1β, IL-6, IL-12p70, anti-inflammatory IL-10, and TNF-α levels. In contrast, in term newborns, cord blood cAMP was negatively correlated with TLR-4-induced TNF-α but positively correlated with IL-10, consistent with an inhibitory role of cAMP toward pro-inflammatory/Th1-polarizing cytokines in the term infant.9 This suggests that downstream cAMP signaling responses known to regulate TNF-α production in response to LPS, such as protein kinase A activation,31 may be differentially regulated in preterm infants. In addition, selective exposure to adenosine receptor-modulating substances, such as high-dose caffeine, may alter LPS responses in the peripheral blood of preterm infants.32 Alternatively, such differences between preterm and term infant blood responses could relate to GA-dependent variation in the regulation/maturation of TLR pathways themselves.16
The positive correlation of IL-6 and IL-10 with cAMP levels suggests that cAMP may have a role in the acute-phase response characteristic of the first DOL. This response mobilizes liver-derived anti-infective proteins to the bloodstream and maintains an anti-inflammatory milieu in the context of rapidly maturing pro-inflammatory capacity with increasing GA.2,33 The rapid fall in cAMP levels after birth may contribute to regulating the balance of postnatal inflammatory and anti-inflammatory responses to the ubiquitous microbial challenges encountered ex utero. Of note, even with the overall reduction of cAMP concentrations, values at a given DOL varied up to tenfold, suggesting that in addition to ontogeny, substantial inter-individual differences contribute to concentrations of this signaling metabolite. Differences in the concentrations of cAMP could have potential implications for the effectiveness of drugs that influence cAMP concentrations, such as the non-specific phosphodiesterase inhibitor, pentoxifylline, whose effects are enhanced in neonates and are dependent on an intact adenosine/cAMP pathway.34,35
The strengths of the study include the prospective longitudinal design throughout the first month of life, the sample size, and comprehensive analysis of cAMP levels, together with interrogation of immune cell number and capacity for cytokine production in whole blood (where extrinsic factors that may influence cAMP pathways are retained) following stimulation with defined TLR agonists. This study also had some unavoidable limitations: we were unable to determine the predominant source (i.e., intracellular vs extracellular or red blood cell vs white blood cell) of cAMP and its main inducers, due to the limited blood volumes available from preterm infants. We also did not account for maternal factors, such as maternal hypertension that can alter neonatal WCCs.36
In conclusion, cAMP was present in higher concentrations in cord than in peripheral blood in preterm and term neonates during the first month of life. Exposure to chorioamnionitis was associated with lower levels of cAMP and TLR-induced cytokine responses. The positive correlation of cAMP levels with TLR-mediated inflammatory and anti-inflammatory cytokine production raises the possibility that cAMP may contribute to sha** early-life TLR-mediated cytokine responses. Future studies should further explore the immunomodulatory properties of cAMP pathways in early life, whose distinct functional ontogeny may inform age-specific strategies for treatment or prevention of neonatal infection and inflammation.
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Acknowledgements
This project was supported by a National Health & Medical Research Council (NHMRC) of Australia project grant award (572548). S.S.S. was supported by a Max-Kade fellowship. D.B. is supported by an NHMRC Senior Research Fellowship (1046518). Research at the Murdoch Children’s Research Institute is supported by the Victorian Government’s Operational Infrastructure Program. Work in O.L.’s laboratory was supported by U.S. National Institutes of Health (NIH) National Institutes of Allergy and Infectious Diseases (NIAID) grants 1RO1AI00135-01, Human Immunology Project Consortium (HIPC) award 1U19AI118608-01A1 and U01AI12484-01, as well as Global Health (OPPGH5284) and Grand Challenges Explorations (OPP1035192) awards from the Bill & Melinda Gates Foundation. The Precision Vaccines Program is supported by an internal award from the Boston Children’s Hospital Department of Pediatrics.
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T.S., S.D.v.H., M.P., D.B., O.L., A.J.C. made substantial contributions to conception and design. T.S., S.D.v.H., J.H., M.P., A.J.C. made substantial contributions to data acquisition and analysis. All authors made contributions to interpretation of data and drafting/revising critically for important intellectual content. All authors approve the version to be published.
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Over the past 5 years, O.L.’s laboratory has received sponsored research support from MedImmune and Crucell (Johnson & Johnson) and reagent support from the Infectious Diseases Research Institute. The other authors declare no competing interests.
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Strunk, T., van Haren, S.D., Hibbert, J. et al. Cyclic AMP in human preterm infant blood is associated with increased TLR-mediated production of acute-phase and anti-inflammatory cytokines in vitro. Pediatr Res 88, 717–725 (2020). https://doi.org/10.1038/s41390-019-0586-2
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DOI: https://doi.org/10.1038/s41390-019-0586-2
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