Research ArticlePediatric Rheumatology

Serologic Evidence of Gut-driven Systemic Inflammation in Juvenile Idiopathic Arthritis

Lampros Fotis, Nurmohammad Shaikh, Kevin W. Baszis, Charles M. Samson, Raffi Lev-Tzion, Anthony R. French and Phillip I. Tarr
The Journal of Rheumatology November 2017, 44 (11) 1624-1631; DOI: https://doi.org/10.3899/jrheum.161589

Abstract

Objective. Accumulating evidence links juvenile idiopathic arthritis (JIA) to nonhost factors such as gut microbes. We hypothesize that children with new-onset JIA have increased intestinal bacterial translocation and circulating lipopolysaccharide (LPS).

Methods. We studied systemic treatment-naive patients with JIA [polyarticular JIA, n = 22, oligoarticular JIA, n = 31, and spondyloarthropathies (SpA), n = 16], patients with established inflammatory bowel disease–related arthritis (IBD-RA, n = 11), and 34 healthy controls. We determined circulating IgG reactivity against LPS, LPS-binding protein (LBP), α-1-acid glycoprotein (α-1AGP), and C-reactive protein (CRP) in plasma or serum from these patients and controls. Juvenile Arthritis Disease Activity Score (JADAS-27) was calculated for patients with JIA.

Results. Circulating anticore LPS antibody concentrations in patients with polyarticular JIA (p = 0.001), oligoarticular JIA (p = 0.024), and SpA (p = 0.001) were significantly greater than in controls, but there were no significant intergroup differences. Circulating LBP concentrations were also significantly greater in patients with polyarticular JIA (p = 0.001), oligoarticular JIA (p = 0.002), and SpA (p = 0.006) than controls, as were α-1AGP concentrations (p = 0.001, 0.001, and 0.003, respectively). No differences were observed between controls and patients with IBD-RA in any of the assays. Circulating concentrations of LBP and α-1AGP correlated strongly with CRP concentrations (r = 0.78 and r = 0.66, respectively). Anticore LPS antibody levels and CRP (r = 0.26), LBP (r = 0.24), and α-AGP (r = 0.22) concentrations had weaker correlations. JADAS-27 scores correlated with LBP (r = 0.66) and α-1AGP concentrations (r = 0.58).

Conclusion. Children with polyarticular JIA, oligoarticular JIA, and SpA have evidence of increased exposure to gut bacterial products. These data reinforce the concept that the intestine is a source of immune stimulation in JIA.

Key Indexing Terms:

Emerging data suggest that the clinical course of juvenile idiopathic arthritis (JIA) might be influenced by nonhost factors, including gut microbes (reviewed1). These lines of evidence associate microbial dysbiosis with altered gut permeability and a proinflammatory extraintestinal cascade driven by gut processes that contribute to the development of arthritis2. Intestinal immune activation in patients with JIA is manifest as lymphonodular hyperplasia and increased tissue γ/δ+ and cytotoxic lymphocyte populations3,4. Additionally, patients with JIA have defective intestinal barrier function5,6, and many children with JIA and abdominal pain have evidence of microscopic colitis7. Also, exclusive enteral nutrition, which induces remission in Crohn disease, has been beneficial in patients with JIA8, and associations between gut microbiome alterations and JIA have been reported9,10,11. However, these studies have generally been performed on subjects with longstanding disease.

Lipopolysaccharide (LPS), an outer-membrane component of Gram-negative bacteria, consists of a highly conserved lipid A and a core oligosaccharide, and diverse sero-group-specific sugar (O) side chains12. The colon harbors an abundance of LPS-producing bacteria, and absorption of LPS from the gut may cause systemic inflammation13. LPS activates macrophages and neutrophils, which then synthesize proinflammatory cytokines that might initiate and/or perpetuate joint inflammation and degeneration14. LPS-binding protein (LBP) is upregulated by LPS and augments innate immunity to bacterial infections. LBP-bound LPS is transferred by CD14 on monocytes to the Toll-like receptor 4 (TLR-4)/myeloid differentiation factor 2 (MD-2) signaling complex, the activation of which triggers inflammation15,16. Indeed, LBP has been implicated in joint inflammation based on elevated intraarticular concentrations in rheumatoid arthritis17. There is also α-1-acid glycoprotein (α-1AGP), another acute-phase protein with immunomodulatory properties18 that neutralizes the toxicity of LPS and enhances its clearance from the body19. The circulating concentration of α-1AGP is associated with disease activity in adult rheumatoid arthritis and inflammatory bowel disease (IBD)20,21.

These findings prompted us to seek evidence of increased intestinal permeability and/or reactivity to gut bacterial contents in treatment-naive patients with JIA. Such increased permeability and exposure to gut contents might be reflected in antibodies directed against LPS and in elevated concentrations of circulating LBP. We also postulated variability in host response between children with different JIA subtypes.

MATERIALS AND METHODS

The study was approved by the institutional review board (IRB) at Washington University School of Medicine, St. Louis (IRB ID# 201408105). Patients with JIA were eligible for enrollment if they were systemic treatment-naive and had not received antibiotics for the prior month. Patients previously treated with intraarticular corticosteroids were included. JIA was defined according to the International League Against Rheumatism criteria for classifying idiopathic arthritis of childhood22. Sera and plasma from our pediatric rheumatology specimen bank were used as well. Patients with polyarticular JIA, oligoarticular JIA, enthesitis-related arthritis (ERA), and psoriatic arthritis (PsA) were included, but those with systemic JIA were excluded, because this entity is now widely thought to be an autoinflammatory condition23. Patients with ERA and PsA were considered together as spondyloarthropathies (SpA) for the purpose of this analysis. We also included patients who had IBD-related arthritis (IBD-RA) of variable duration. All patients with IBD-RA were receiving systemic treatment for IBD at the time they were studied, and their joint symptoms were assessed by a pediatric rheumatologist. Sera and plasma from healthy control subjects were obtained from our pediatric rheumatology plasma bank, as well as from normal controls obtained during studies of the pathophysiology of childhood hemolytic uremic syndrome24, and of children undergoing colonoscopy for suspected IBD, but whose colonoscopy did not demonstrate disease. The Juvenile Arthritis Disease Activity Score (JADAS-27)25 was calculated for patients with JIA who were prospectively recruited. All plasmas were collected in EDTA tubes, centrifuged (4°C, 15 min, 2500 g), and frozen (−80°C) in aliquots until tested.

Escherichia coli core LPS preparation and characterization

E. coli strain F12 (pSK+) is a TnphoA mutant of E. coli O157:H7 that cannot express the O157 LPS side chain26 and therefore can serve as a source of antigen with which to measure reactivity to generic Enterobacteriaceae LPS. This mutant was inoculated from frozen stock into 2 l of Luria-Bertani broth containing 100 μg/ml of ampicillin and placed in a shaking incubator (37°C, overnight). Bacteria were pelleted, washed once gently with purified sterile water, and suspended in 20 ml of sterile water per 3–4 g of pellet. The suspension was heated (68°C, 10 min) in a water bath with stirring. Then an equal volume of preheated (68°C) phenol was slowly added, and the resulting suspension was stirred vigorously (68°C, 60 min), placed in an ice water bath with continuous stirring (10 min), and centrifuged (4°C, 45 min). The upper layer was aspirated and saved on ice. The organic interface and phenol layer with bacterial pellet were reextracted with an equal volume of purified water, repeating the mixing, heating, cooling, and centrifugation steps as before. The upper layers from both extractions were pooled and dialyzed against 4 l of purified water using Spectra/Por 7 dialysis membrane 1000 kD MWCO (Spectrum Laboratories) for 2 days, with 2 water changes daily, after which the dialysate was ultracentrifuged (105,000 g, 4 h). The supernatant was removed and the LPS pellet was suspended in molecular biology grade de-ionized water (Corning). Following DNase (EZ Bioresearch) and proteinase K digestion, we mixed an equal volume of 1:1 phenol/chloroform solution and then chloroform to remove residual phenol27.

LPS was separated electrophoretically in a 10% sodium dodecyl sulfate-polyacrylamide gel28, and visualized by silver staining (GelCode SilverSNAP Stain kit), and quantified in endotoxin units (EU/ml) by the chromogenic limulus amebocyte lysate assay (Pierce Biotechnology).

E. coli anticore LPS antibodies enzyme immunoassay

The concentration of circulating anticore LPS antibodies was determined by a laboratory-developed enzyme immunoassay (EIA). Nunc Maxisorp microplates (Thermo Scientific) were coated (4°C, overnight) with 1000 EU of LPS per well diluted in 100 μl of 0.1 M carbonate-bicarbonate buffer (pH 9.6; Sigma). The plates were washed 4 times with phosphate-buffered saline (PBS; pH 7.4) containing 0.05% Tween-20 (PBS/T) followed by incubation (room temperature, 2 h) with 100 μl of blocking solution [1% bovine serum albumin (BSA) in PBS/T], and washed again 4 times with PBS/T. The wells were then incubated with 100 μl of subject serum or plasma (1:100 diluted in 0.5% BSA in PBS/T; room temperature, 2 h). After washing 4 times with PBS/T, anti-human IgG/Fcγ-horseradish peroxidase (Jackson Laboratory), 1:10,000 in 0.5% BSA in PBS/T, was added (100 µl) to each well and incubated (room temperature, 1 h). The plates were then washed as before and incubated with 100 μl of o-phenylenediamine dihydrochloride (Sigma) substrate solution (25 min) before reaction termination with 100 μl of 2N H2SO4. Absorbance was measured at 490 nm with Molecular Devices VERSAmax tunable microplate reader (Conquer Scientific).

Each sample was measured in 3 independent experiments performed in duplicate on different days. For each experiment, we included as a standard the serum of a patient with polyarticular JIA with strong reactivity against core LPS. This reactivity was arbitrarily defined as 1000 EIA units.

LBP, α-1AGP, and CRP concentrations

Commercial EIA were used to determine concentrations of circulating LBP (HyCult) and α-1AGP and CRP (R&D Systems), according to the manufacturers’ instructions.

Statistics

The Shapiro-Wilk test was used to determine whether the data were normally distributed. The nonparametric Levene’s test was used to verify the equality of variances in the samples. The Kruskal-Wallis test was used for multiple between-group comparisons. Spearman rank-order correlations were used to determine whether age of control subjects was related to resulting values. In the 10 pairwise comparisons between groups for the variables in Table 1, we considered p values < 0.005 to be significant (i.e., 0.05 ÷ 10) after correcting for multiple comparisons. After demonstrating statistically significant differences using uncorrected p values for single comparisons between individual JIA subgroups (but not the IBD-RA group) and the controls for all values, we compared the assay results for the polyarticular JIA to oligoarticular JIA, polyarticular JIA to SpA, and oligoarticular JIA to SpA groups. For the 3 pairwise comparisons among the juvenile arthritis subgroups, we provide uncorrected p values, but consider p values < 0.017 (i.e., 0.05 ÷ 3) as significant after correcting for multiple comparisons. Linear relationships between the variables were measured with the Spearman’s ϱ test. The family error was set to p < 0.05. SPSS 22.0 was used for these analyses. All p values were 2-tailed.

View this table:
Table 1.

Patient demographics.

RESULTS

Samples from 114 subjects were analyzed. After correcting for multiple comparisons, the only statistically significant differences in the demographic data were between the ages of the oligoarticular JIA group and all other groups (Table 1). The clinical features of the patients with IBD-RA are provided in more detail in Supplementary Table 1 (available with the online version of this article).

We detected significant differences between the median EIA values for anticore LPS antibody concentrations (Table 2 and Figure 1) of healthy controls and polyarticular JIA (p < 0.001), oligoarticular JIA (p = 0.02), and SpA (p = 0.001) groups. There was not a significant difference in circulating anticore LPS antibody concentrations between the healthy controls and IBD-RA subjects. Circulating LBP concentrations (Table 2 and Figure 2) were significantly greater in the polyarticular (p = 0.001), oligoarticular (p = 0.002), and SpA (p = 0.006) groups than in healthy controls. The IBD-RA subjects’ circulating LPB concentrations were not significantly higher than those in the controls. Circulating α-1AGP concentrations (Table 2 and Figure 3) were also significantly greater in all 3 JIA arthritis subgroups than in the healthy controls (p = 0.001 for the polyarticular and oligoarticular JIA groups; p = 0.003 for the SpA groups), but were not greater in the patients with IBD-RA than in the healthy controls. CRP concentrations were significantly lower in the healthy controls than in all 3 JIA disease subgroups (p = 0.001, p < 0.001, and p = 0.001 for oligoarticular JIA, polyarticular JIA, and SpA groups, respectively; Table 2). As with the values for anticore LPS antibodies, LBP, and α-1AGP, the CRP values did not differ between healthy controls and the IBD-RA group.

Figure 1.
Figure 1.

Circulating anticore LPS antibody concentrations across groups. * Outliers above Q3 + 1.5 IQR. Open circles are outliers between Q3 and Q3 + 1.5 IQR. IQR: interquartile range; LPS: lipopolysaccharide; EIA: enzyme immunoassay; IBD-RA: inflammatory bowel disease–related arthritis.

Figure 2.
Figure 2.

Circulating LBP concentrations across groups. Open circles are outliers between Q3 and Q3 + 1.5 IQR. IQR: interquartile range; IBD-RA: inflammatory bowel disease–related arthritis.

Figure 3.
Figure 3.

Circulating α-1AGP concentrations across groups. Open circles are outliers between Q3 and Q3 + 1.5 IQR. α-1AGP: α-1-acid glycoprotein; IQR: interquartile range; IBD-RA: inflammatory bowel disease–related arthritis.

View this table:
Table 2.

Concentrations (median, interquartile range) of circulating anti-LPS, LBP, α-1AGP, and CRP in different groups. All comparisons are between individual patient groups and healthy controls for each assay. P values < 0.05 are considered significant.

Supplementary Table 2 (available with the online version of this article) presents pairwise comparisons among the 3 JIA disease subgroups. Circulating LBP concentrations were lower in the oligoarticular group than in the polyarticular JIA group (p = 0.02), and circulating α-1AGP concentrations were lower in the oligoarticular JIA and the SpA groups (p = 0.033 and p = 0.026, respectively) than in the polyarticular JIA group. However, none of these differences retained statistical significance after correcting for multiple comparisons.

The concentrations of circulating CRP and α-1AGP (r = 0.77; p < 0.001), CRP and LBP (r = 0.78; p < 0.001), and LBP and α-1AGP (r = 0.66; p < 0.001) were strongly correlated. The concentrations of anticore LPS antibodies and α-1AGP (r = 0.22; p = 0.02), LBP (r = 0.24; p = 0.012), and CRP (r = 0.26; p = 0.007) had weaker correlations. The JADAS-27 score calculated for the 29 patients with JIA prospectively enrolled correlated strongly with the LBP (r = 0.66; p < 0.001) and α-1AGP (r = 0.58; p = 0.001) concentrations, but not with concentrations of circulating anticore LPS antibodies.

We were concerned that the age of the controls was at variance with the ages of the members of the oligoarticular JIA group. However, for all values determined, only the concentration of circulating antibodies to LPS changed significantly over age (rs = 0.5288, t = 3.52, df = 32; p = 0.001). Therefore, for this variable, we compared concentrations of antibodies to LPS between 11 controls in the youngest control group tertile [median age 6.0 yrs, interquartile range (IQR) 4.0–7.0] and the 31 subjects in the oligoarticular JIA group (median age 4.0 yrs, 3.0–9.0). The median circulating antibody concentration was 124 (IQR 57.1–236.5) EIA units in the controls, compared to 333 (IQR 227–472) EIA units in the oligoarticular group (p < 0.001), confirming the significance of the higher value in the oligoarticular group after controlling for age effects.

DISCUSSION

The gut is a major habitat of microbes and their by-products. The seroreactivity of patients with JIA to anticore LPS, a component of Gram-negative bacterial cell walls, suggests that such organisms and their systemic absorption may explain at least part of the inappropriate immune activation in JIA. Because the E. coli mutant used to produce the core LPS antigen for the EIA lacks the LPS O-side chain, we conclude that the reactivity reflects a response to generic Gram-negative LPS in which the core and lipid A moieties are conserved29, and does not reflect exposure to E. coli O157:H7.

We found comparatively greater concentrations of circulating LBP and α-1AGP in treatment-naive patients with polyarticular JIA, oligoarticular JIA, and SpA than in healthy controls, suggesting systemic inflammation. Although the elevation of LBP (and of α-1AGP) could reflect acute-phase reaction, the simultaneous presence of elevated anticore LPS antibodies and LBP and α-1AGP concentrations indicates that Gram-negative bacteria or their products have influenced this upregulation for an extended interval before sampling, because antibody responses are slower to develop than acute-phase reactants. Because the gut is the largest habitat of Gram-negative bacteria in the body, this finding implicates the intestine in the induction of systemic inflammation. Our findings of elevated concentrations of circulating LBP and anticore LPS antibodies in patients with SpA are also consistent with the observation that many such patients have subclinical intestinal inflammation30. Also, there are recent reports of histologically determined intestinal inflammation in patients with JIA7. The same finding has been confirmed in patients with SpA31, a group in which elevated levels of acute-phase reactants and anti-LPS were also observed.

Circulating LPS plausibly initiates or perpetuates systemic inflammation. LPS is the primary ligand of TLR-4, and LPS upregulates TLR-4, which in turn activates nuclear factor-κB and PI-3K pathways that exert proinflammatory activity14. LPS in human joint cartilage induces matrix breakdown and chondrocyte apoptosis, thereby degrading cartilage11. TLR-4–deficient mice are relatively resistant to LPS-induced arthritis and joint destruction32,33. In addition, patients with rheumatoid arthritis are sensitized to Prevotella copri34 or antigens common to Enterobacteriaceae, including LPS35. Further, Yersinia enterocolitica O:3 LPS is detectable in the synovial fluid for extended periods in patients with post-infectious reactive arthritis36. However, the elevated concentrations of anticore LPS and LBP in polyarticular JIA and oligoarticular JIA are novel findings, because little published evidence exists for increased intestinal permeability or dysfunction in these disorders5,6. Moreover, our data are derived from treatment-naive patients, thereby lending credence to a potential role for gut bacterial content in precipitating juvenile arthritis.

Our data suggest the potential utility of α-1AGP to follow disease activity in patients with JIA. Levels of α-1AGP were elevated in all 3 groups, and interestingly, were correlated with the concentrations of LBP, CRP, and JADAS-27. Although not well studied in inflammatory arthritis, α-1AGP might play a role in the mechanisms of joint erosions and also be of value as a biomarker in predicting the potential risk of erosions37,38,39.

CRP correlated strongly with the other 2 acute-phase proteins, namely LBP and α-1AGP, but only weakly with the anticore LPS antibodies. The fact that LBP is directly linked to LPS stimulation suggests that this acute-phase reaction is initiated by products from the intestine. Alternatively, systemic inflammation might increase intestinal permeability and secondarily increase concentrations of circulating anticore LPS antibodies and/or LBP40. Although we found a strong correlation between LBP and CRP concentrations in the circulation (not surprising because both proteins are acute-phase reactants), we found only a weak correlation between α-1AGP and CRP concentrations and circulating anticore LPS antibodies. This suggests that anticore LPS antibody production is independent of a systemic inflammatory state, but present chiefly in the polyarticular JIA, oligoarticular JIA, and SpA groups. JADAS-27 correlated significantly both with the LBP and α-1AGP, but not with anticore LPS antibodies, which is not surprising because both acute-phase markers are related to CRP.

Even though differences between some of the medians in pairwise comparisons between JIA subgroups were statistically significant using uncorrected p values, none of the assay values differ significantly after correcting for multiple comparisons. Hence, our data do not suggest that these markers can differentiate between oligoarticular JIA, polyarticular JIA, and SpA patients with confidence.

We acknowledge several limitations to our study. First, our databases did not permit us to identify reliably nonsteroidal antiinflammatory drug (NSAID) use prior to enrollment, and it is possible that these agents altered intestinal permeability. It will be important to account for this variable in future prospective studies that seek to corroborate our findings. Second, we used both sera and plasmas in the assays. However, plasma and serum CRP41 and antimicrobial antibody concentrations42,43 correlate well, and LBP concentrations from sera and plasmas are used in multiple case series (review44).

The patients with IBD-RA warrant several comments. First, the inability to find a significant elevation of any of the tested circulating markers in the IBD-RA group compared to healthy controls was unexpected, because LBP concentrations in Crohn disease exceed those in ulcerative colitis and in normal controls45, and CRP is often used to indicate IBD activity. However, the central tendencies for each of these values exceeded those in the controls, suggesting some degree of immune activation in the IBD-RA group. Second, patients with IBD are admonished to avoid NSAID, and several patients had high circulating concentrations of antibodies to E. coli LPS, suggesting that systemic reaction to gut LPS can occur without this inciting agent, and even without active gut disease. Third, the comparative nonreactivity of this cohort might be attributed to the universal use of immunosuppressant agents. It is not clear why arthritis developed under these circumstances, but we must consider the alternative hypothesis that the pathogenesis of IBD-RA, unlike JIA, is not related to systemic inflammation. Indeed, there is little overlap in serologic profiles between adults with IBD-RA and rheumatoid arthritis46. However, the small size of the IBD-RA group and the heterogeneity of immunosuppressants used limit the interpretations that can be drawn from this group.

Overall, our findings and emerging knowledge of altered intestinal microbiota in patients with JIA suggest a potential role for the gut in JIA. Although the concept of intestinal dysfunction cannot yet be generalized to all patients with JIA, those that have evidence of intestinal dysfunction as indicated by elevated anti-LPS or LBP levels could be candidates for further evaluation of their gut bacterial population. It would also be interesting to study the response of patients to bacterial antigens in the context of JIA disease monitoring. Notably, in our present study, patients with IBD-RA, all of whom were treated with immune suppressants and most of whom had quiescent gut disease, have in aggregate low anti-LPS and LBP levels. However, it is premature to use any of these markers as a treatment target in JIA. Additionally, in future studies, it will be worthwhile to obtain stool from patients to study fecal markers of gut reactivity at instructive points in the JIA disease process, and to perform sequence analysis to determine the presence and extent of potential dysbiotic gut communities, and correlate these values with markers of systemic inflammation as used in our study.

The concurrent increase in the concentrations of anticore LPS antibody and LBP in the circulation of treatment-naive patients with polyarticular JIA, oligoarticular JIA, and SpA suggest systemic exposure to gut contents. Circulating LPS increases tight junction permeability in mice47, and a similar process is postulated in patients with IBD, where circulating LPS concentrations correlate with tissue (gut) inflammation and disease activity45,48,49. This exposure potentially induced a systemic inflammatory reaction in our cohorts, as evidenced by increased circulating LBP and α-1AGP concentrations in all subgroups except IBD-RA (the only group in which patients were under treatment), with the majority being in disease remission. The concentrations of the gut-related circulating acute-phase proteins (LBP and α-1AGP) correlate well with disease activity scores of patients with JIA, and therefore these molecules are worthy of further consideration in monitoring disease activity.

ONLINE SUPPLEMENT

Supplementary material accompanies the online version of this article.

Footnotes

  • Supported by US National Institutes of Health Grants P30DK052574 (DDRCC Biobank Core), UL1TR000448, and P30CA091842 (for REDCap), and funding from the Melvin E. Carnahan Professorship (Dr. Tarr).

  • Accepted for publication June 21, 2017.

REFERENCES

  1. 1.
    1. Arvonen M,
    2. Berntson L,
    3. Pokka T,
    4. Karttunen TJ,
    5. Vähäsalo P,
    6. Stoll ML
    . Gut microbiota-host interactions and juvenile idiopathic arthritis. Pediatr Rheumatol Online J 2016;14:44.
    OpenUrl
  2. 2.
    1. Lerner A,
    2. Matthias T
    . Rheumatoid arthritis-celiac disease relationship: joints get that gut feeling. Autoimmun Rev 2015;14:103847.
    OpenUrl
  3. 3.
    1. Kokkonen J,
    2. Arvonen M,
    3. Vähäsalo P,
    4. Karttunen TJ
    . Intestinal immune activation in juvenile idiopathic arthritis and connective tissue disease. Scand J Rheumatol 2007;36:3869.
    OpenUrlCrossRefPubMed
  4. 4.
    1. Arvonen M,
    2. Ikni L,
    3. Augustin M,
    4. Karttunen TJ,
    5. Vähäsalo P
    . Increase of duodenal and ileal mucosal cytotoxic lymphocytes in juvenile idiopathic arthritis. Clin Exp Rheumatol 2010;28:12834.
    OpenUrlPubMed
  5. 5.
    1. Weber P,
    2. Brune T,
    3. Ganser G,
    4. Zimmer KP
    . Gastrointestinal symptoms and permeability in patients with juvenile idiopathic arthritis. Clin Exp Rheumatol 2003;21:65762.
    OpenUrlPubMed
  6. 6.
    1. Picco P,
    2. Gattorno M,
    3. Marchese N,
    4. Vignola S,
    5. Sormani MP,
    6. Barabino A,
    7. et al.
    Increased gut permeability in juvenile chronic arthritides. A multivariate analysis of the diagnostic parameters. Clin Exp Rheumatol 2000;18:7738.
    OpenUrlPubMed
  7. 7.
    1. Pichler J,
    2. Ong C,
    3. Shah N,
    4. Sebire N,
    5. Kiparrissi F,
    6. Borrelli O,
    7. et al.
    Histopathological features of gastrointestinal mucosal biopsies in children with juvenile idiopathic arthritis. Pediatr Res 2016;79:895901.
    OpenUrl
  8. 8.
    1. Berntson L,
    2. Hedlund-Treutiger I,
    3. Alving K
    . Anti-inflammatory effect of exclusive enteral nutrition in patients with juvenile idiopathic arthritis. Clin Exp Rheumatol 2016;34:9415.
    OpenUrl
  9. 9.
    1. Tejesvi MV,
    2. Arvonen M,
    3. Kangas SM,
    4. Keskitalo PL,
    5. Pirttilä AM,
    6. Karttunen TJ,
    7. et al.
    Faecal microbiome in new-onset juvenile idiopathic arthritis. Eur J Clin Microbiol Infect Dis 2016;35:36370.
    OpenUrlPubMed
  10. 10.
    1. Aggarwal A,
    2. Sarangi AN,
    3. Gaur P,
    4. Shukla A,
    5. Aggarwal R
    . Gut microbiome in children with enthesitis-related arthritis in a developing country and the effect of probiotic administration. Clin Exp Immunol 2017;187:4809.
    OpenUrl
  11. 11.
    1. Stoll ML,
    2. Kumar R,
    3. Morrow CD,
    4. Lefkowitz EJ,
    5. Cui X,
    6. Genin A,
    7. et al.
    Altered microbiota associated with abnormal humoral immune responses to commensal organisms in enthesitis-related arthritis. Arthritis Res Ther 2014;16:486.
    OpenUrlCrossRefPubMed
  12. 12.
    1. Trent MS,
    2. Stead CM,
    3. Tran AX,
    4. Hankins JV
    . Diversity of endotoxin and its impact on pathogenesis. J Endotoxin Res 2006;12:20523.
    OpenUrlCrossRefPubMed
  13. 13.
    1. de Punder K,
    2. Pruimboom L
    . Stress induces endotoxemia and low-grade inflammation by increasing barrier permeability. Front Immunol 2015;6:223.
    OpenUrlPubMed
  14. 14.
    1. Lorenz W,
    2. Buhrmann C,
    3. Mobasheri A,
    4. Lueders C,
    5. Shakibaei M
    . Bacterial lipopolysaccharides form procollagen-endotoxin complexes that trigger cartilage inflammation and degeneration: implications for the development of rheumatoid arthritis. Arthritis Res Ther 2013;15:R111.
    OpenUrlCrossRefPubMed
  15. 15.
    1. Gutsmann T,
    2. Müller M,
    3. Carroll SF,
    4. MacKenzie RC,
    5. Wiese A,
    6. Seydel U
    . Dual role of lipopolysaccharide (LPS)-binding protein in neutralization of LPS and enhancement of LPS-induced activation of mononuclear cells. Infect Immun 2001;69:694250.
    OpenUrlAbstract/FREE Full Text
  16. 16.
    1. Berner R,
    2. Fürll B,
    3. Stelter F,
    4. Dröse J,
    5. Müller H-P,
    6. Schütt C
    . Elevated levels of lipopolysaccharide-binding protein and soluble CD14 in plasma in neonatal early-onset sepsis. Clin Diagn Lab Immunol 2002;9:4405.
    OpenUrlCrossRefPubMed
  17. 17.
    1. Heumann D,
    2. Bas S,
    3. Gallay P,
    4. Le Roy D,
    5. Barras C,
    6. Mensi N,
    7. et al.
    Lipopolysaccharide binding protein as a marker of inflammation in synovial fluid of patients with arthritis: correlation with interleukin 6 and C-reactive protein. J Rheumatol 1995;22:12249.
    OpenUrlPubMed
  18. 18.
    1. Hochepied T,
    2. Berger FG,
    3. Baumann H,
    4. Libert C
    . α1-Acid glycoprotein: an acute phase protein with inflammatory and immunomodulating properties. Cytokine Growth Factor Rev 2003;14:2534.
    OpenUrlCrossRefPubMed
  19. 19.
    1. Moore DF,
    2. Rosenfeld MR,
    3. Gribbon PM,
    4. Winlove CP,
    5. Tsai CM
    . Alpha-1-acid (AAG, orosomucoid) glycoprotein: interaction with bacterial lipopolysaccharide and protection from sepsis. Inflammation 1997;21:6982.
    OpenUrlCrossRefPubMed
  20. 20.
    1. Cylwik B,
    2. Chrostek L,
    3. Gindzienska-Sieskiewicz E,
    4. Sierakowski S,
    5. Szmitkowski M
    . Relationship between serum acute-phase proteins and high disease activity in patients with rheumatoid arthritis. Adv Med Sci 2010;55:805.
    OpenUrlPubMed
  21. 21.
    1. Nielsen OH,
    2. Vainer B,
    3. Madsen SM,
    4. Seidelin JB,
    5. Heegaard NH
    . Established and emerging biological activity markers of inflammatory bowel disease. Am J Gastroenterol 2000;95:35967.
    OpenUrlPubMed
  22. 22.
    1. Petty RE,
    2. Southwood TR,
    3. Baum J,
    4. Bhettay E,
    5. Glass DN,
    6. Manners P,
    7. et al.
    Revision of the proposed classification criteria for juvenile idiopathic arthritis: Durban, 1997. J Rheumatol 1998;25:19914.
    OpenUrlPubMed
  23. 23.
    1. Prakken B,
    2. Albani S,
    3. Martini A
    . Juvenile idiopathic arthritis. Lancet 2011;377:213849.
    OpenUrlCrossRefPubMed
  24. 24.
    1. Chandler WL,
    2. Jelacic S,
    3. Boster DR,
    4. Ciol MA,
    5. Williams GD,
    6. Watkins SL,
    7. et al.
    Prothrombotic coagulation abnormalities preceding the hemolytic-uremic syndrome. N Engl J Med 2002;346:2332.
    OpenUrlCrossRefPubMed
  25. 25.
    1. Nordal EB,
    2. Zak M,
    3. Aalto K,
    4. Berntson L,
    5. Fasth A,
    6. Herlin T,
    7. et al.
    Validity and predictive ability of the juvenile arthritis disease activity score based on CRP versus ESR in a Nordic population-based setting. Ann Rheum Dis 2012;71:11227.
    OpenUrlAbstract/FREE Full Text
  26. 26.
    1. Bilge SS,
    2. Vary JC,
    3. Dowell SF,
    4. Tarr PI
    . Role of the Escherichia coli O157:H7 O side chain in adherence and analysis of an rfb locus. Infect Immun 1996;64:4795801.
    OpenUrlAbstract/FREE Full Text
  27. 27.
    1. Inzana TJ
    . Electrophoretic heterogeneity and interstrain variation of the lipopolysaccharide of Haemophilus influenzae. J Infect Dis 1983;148:4929.
    OpenUrlCrossRefPubMed
  28. 28.
    1. Tsai CM,
    2. Frasch CE
    . A sensitive silver stain for detecting lipopolysaccharides in polyacrylamide gels. Anal Biochem 1982;119:1159.
    OpenUrlCrossRefPubMed
  29. 29.
    1. Tyler JW,
    2. Cullor JS,
    3. Spier SJ,
    4. Smith BP
    . Immunity targeting common core antigens of gram-negative bacteria. J Vet Intern Med 1990;4:1725.
    OpenUrlPubMed
  30. 30.
    1. Mielants H,
    2. Veys EM,
    3. Cuvelier C,
    4. De Vos M,
    5. Goemaere S,
    6. De Clercq L,
    7. et al.
    The evolution of spondyloarthropathies in relation to gut histology. II. Histological aspects. J Rheumatol 1995;22:22738.
    OpenUrlPubMed
  31. 31.
    1. Conti F,
    2. Borrelli O,
    3. Anania C,
    4. Marocchi E,
    5. Romeo EF,
    6. Paganelli M,
    7. et al.
    Chronic intestinal inflammation and seronegative spondyloarthropathy in children. Dig Liver Dis 2005;37:7617.
    OpenUrlCrossRefPubMed
  32. 32.
    1. Lee EK,
    2. Kang SM,
    3. Paik DJ,
    4. Kim JM,
    5. Youn J
    . Essential roles of Toll-like receptor-4 signaling in arthritis induced by type II collagen antibody and LPS. Int Immunol 2005;17:32533.
    OpenUrlCrossRefPubMed
  33. 33.
    1. Pierer M,
    2. Wagner U,
    3. Rossol M,
    4. Ibrahim S
    . Toll-like receptor 4 is involved in inflammatory and joint destructive pathways in collagen-induced arthritis in DBA1J mice. PLoS One 2011;6:e23539.
    OpenUrlCrossRefPubMed
  34. 34.
    1. Pianta A,
    2. Arvikar S,
    3. Strle K,
    4. Drouin EE,
    5. Wang Q,
    6. Costello CE,
    7. et al.
    Evidence for immune relevance of Prevotella copri, a gut microbe, in patients with rheumatoid arthritis. Arthritis Rheumatol 2017;69:96475.
    OpenUrl
  35. 35.
    1. Aoki S,
    2. Yoshikawa K,
    3. Yokoyama T,
    4. Nonogaki T,
    5. Iwasaki S,
    6. Mitsui T,
    7. et al.
    Role of enteric bacteria in the pathogenesis of rheumatoid arthritis: evidence for antibodies to enterobacterial common antigens in rheumatoid sera and synovial fluids. Ann Rheum Dis 1996;55:3639.
    OpenUrlAbstract/FREE Full Text
  36. 36.
    1. Granfors K,
    2. Merilahti-Palo R,
    3. Luukkainen R,
    4. Möttönen T,
    5. Lahesmaa R,
    6. Probst P,
    7. et al.
    Persistence of Yersinia antigens in peripheral blood cells from patients with Yersinia enterocolitica O:3 infection with or without reactive arthritis. Arthritis Rheum 1998;41:85562.
    OpenUrlCrossRefPubMed
  37. 37.
    1. Olewicz-Gawlik A,
    2. Korczowska-Łacka I,
    3. Łacki JK,
    4. Klama K,
    5. Hrycaj P
    . Fucosylation of serum alpha1-acid glycoprotein in rheumatoid arthritis patients treated with infliximab. Clin Rheumatol 2007;26:167984.
    OpenUrlCrossRefPubMed
  38. 38.
    1. Haston JL,
    2. FitzGerald O,
    3. Kane D,
    4. Smith KD
    . The influence of alpha1-acid glycoprotein on collagenase-3 activity in early rheumatoid arthritis. Biomed Chromatogr 2003;17:3614.
    OpenUrlCrossRefPubMed
  39. 39.
    1. De Graaf TW,
    2. Van Ommen EC,
    3. Van der Stelt ME,
    4. Kerstens PJ,
    5. Boerbooms AM,
    6. Van Dijk W
    . Effects of low dose methotrexate therapy on the concentration and the glycosylation of alpha 1-acid glycoprotein in the serum of patients with rheumatoid arthritis: a longitudinal study. J Rheumatol 1994;21:220916.
    OpenUrlPubMed
  40. 40.
    1. Hietbrink F,
    2. Besselink MG,
    3. Renooij W,
    4. de Smet MB,
    5. Draisma A,
    6. van der Hoeven H,
    7. et al.
    Systemic inflammation increases intestinal permeability during experimental human endotoxemia. Shock 2009;32:3748.
    OpenUrlCrossRefPubMed
  41. 41.
    1. Dossus L,
    2. Becker S,
    3. Achaintre D,
    4. Kaaks R,
    5. Rinaldi S
    . Validity of multiplex-based assays for cytokine measurements in serum and plasma from “non-diseased” subjects: Comparison with ELISA. J Immunol Methods 2009;350:12532.
    OpenUrlCrossRefPubMed
  42. 42.
    1. Siev M,
    2. Yu X,
    3. Prados-Rosales R,
    4. Martiniuk FT,
    5. Casadevall A,
    6. Achkar JM
    . Correlation between serum and plasma antibody titers to mycobacterial antigens. Clin Vaccine Immunol 2011;18:1735.
    OpenUrlAbstract/FREE Full Text
  43. 43.
    1. Cherpes TL,
    2. Meyn LA,
    3. Hillier SL
    . Plasma versus serum for detection of herpes simplex virus type 2-specific immunoglobulin G antibodies with a glycoprotein G2-based enzyme immunoassay. J Clin Microbiol 2003;41:27589.
    OpenUrlAbstract/FREE Full Text
  44. 44.
    1. Gonzalez-Quintela A,
    2. Alonso M,
    3. Campos J,
    4. Vizcaino L,
    5. Loidi L,
    6. Gude F
    . Determinants of serum concentrations of lipopolysaccharide-binding protein (LBP) in the adult population: the role of obesity. PLoS One 2013;8:e54600.
    OpenUrlCrossRefPubMed
  45. 45.
    1. Pasternak BA,
    2. D’Mello S,
    3. Jurickova II,
    4. Han X,
    5. Willson T,
    6. Flick L,
    7. et al.
    Lipopolysaccharide exposure is linked to activation of the acute phase response and growth failure in pediatric Crohn’s disease and murine colitis. Inflamm Bowel Dis 2010;16:85669.
    OpenUrlCrossRefPubMed
  46. 46.
    1. Van Erp SJ,
    2. Verheul MK,
    3. Levarht EW,
    4. van der Reijden JJ,
    5. van der Heijde D,
    6. van Gaalen FA,
    7. et al.
    Short article: Absence of serological rheumatoid arthritis biomarkers in inflammatory bowel disease patients with arthropathies. Eur J Gastroenterol Hepatol 2017;29:3458.
    OpenUrl
  47. 47.
    1. Guo S,
    2. Nighot M,
    3. Al-Sadi R,
    4. Alhmoud T,
    5. Nighot P,
    6. Ma TY
    . Lipopolysaccharide regulation of intestinal tight junction permeability is mediated by TLR4 signal transduction pathway activation of FAK and MyD88. J Immunol 2015;195:49995010.
    OpenUrlAbstract/FREE Full Text
  48. 48.
    1. Lakatos PL,
    2. Kiss LS,
    3. Palatka K,
    4. Altorjay I,
    5. Antal-Szalmas P,
    6. Palyu E,
    7. et al.
    Serum lipopolysaccharide-binding protein and soluble CD14 are markers of disease activity in patients with Crohn’s disease. Inflamm Bowel Dis 2011;17:76777.
    OpenUrlCrossRefPubMed
  49. 49.
    1. Pastor Rojo O,
    2. López San Román A,
    3. Albéniz Arbizu E,
    4. de la Hera Martínez A,
    5. Ripoll Sevillano E,
    6. Albillos Martínez A
    . Serum lipopolysaccharide-binding protein in endotoxemic patients with inflammatory bowel disease. Inflamm Bowel Dis 2007;13:26977.
    OpenUrlCrossRefPubMed
Back to top

In this issue

Print
Download PDF
Article Alerts
Email Article
Citation Tools

 Request Permissions

Bookmark this article

Jump to section

Keywords

JUVENILE IDIOPATHIC ARTHRITIS
ACUTE-PHASE PROTEINS
α1-ACID GLYCOPROTEIN
INTESTINAL PERMEABILITY
LIPOPOLYSACCHARIDE
LIPOPOLYSACCHARIDE-BINDING PROTEIN

Keywords