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J Rheum Dis 2025; 32(1): 48-56

Published online January 1, 2025

© Korean College of Rheumatology

Associations between circulating interleukin-18 levels and adult-onset Still’s disease: a meta-analysis

Young Ho Lee , M.D., Ph.D., Gwan Gyu Song , M.D., Ph.D.

Division of Rheumatology, Department of Internal Medicine, Korea University Medical Center, Korea University College of Medicine, Seoul, Korea

Correspondence to : Young Ho Lee, https://orcid.org/0000-0003-4213-1909
Division of Rheumatology, Department of Internal Medicine, Korea University Anam Hospital, Korea University College of Medicine, 73 Goryeodae-ro, Seongbuk-gu, Seoul 02841, Korea. E-mail: lyhcgh@korea.ac.kr

Received: August 1, 2024; Revised: September 18, 2024; Accepted: October 17, 2024

This is an Open Access article distributed under the terms of the Creative Commons Attribution Non-Commercial License (http://creativecommons.org/licenses/by-nc/4.0) which permits unrestricted non-commercial use, distribution, and reproduction in any medium, provided the original work is properly cited.

Objective: This study aimed to investigate the link between circulating interleukin-18 (IL-18) levels and adult-onset Still’s disease (AOSD).
Methods: A thorough search was performed on MEDLINE, Embase, and Web of Science to find relevant articles. A meta-analysis was conducted to compare serum/plasma IL-18 levels in AOSD patients to those in control subjects.
Results: The meta-analysis included 13 studies with a total of 562 AOSD patients and 790 controls. The results showed a significant increase in IL-18 levels in the AOSD group compared to the control group (standard mean difference [SMD]=1.899, 95% confidence interval [CI]=1.078~2.720, p<0.001). When stratified by ethnicity, higher IL-18 levels were found in both Asian and European populations with AOSD. Subgroup analysis, regardless of variable adjustments, consistently indicated significantly higher IL-18 levels in the AOSD group. Significant elevations in IL-18 levels were observed in both small (n<50) and large groups (n>50), as well as in original and imputed data groups after data type stratification. Free IL-18 levels were significantly higher in the active group compared to the inactive group (SMD=0.900, 95% CI=0.532~1.268, p<0.001). The meta-analysis showed a positive correlation between IL-18 levels and ferritin (correlation coefficient=0.542, 95% CI=0.431~0.637, p<0.001) and C-reactive protein.
Conclusion: This meta-analysis demonstrated a significant increase in circulating IL-18 levels and a positive correlation between IL-18 levels and ferritin and C-reactive protein levels in patients with AOSD.

Keywords Adult-onset Still’s disease, Interleukin-18, Ferritin, Polymorphism, Genetic, Meta-analysis

Adult-onset Still’s disease (AOSD) is a systemic inflammatory condition marked by a range of clinical symptoms such as spiking fever, transient skin rash, joint pain or arthritis, sore throat, and enlarged liver or spleen [1,2]. Diagnostic laboratory findings often include neutrophilic leukocytosis, abnormal liver function tests, high serum ferritin levels, and increased acute-phase reactants. Despite significant medical advancements, the precise cause of AOSD remains unknown. Active AOSD is characterized by immune-mediated inflammation, typically triggered by abnormal immune responses in genetically predisposed individuals exposed to environmental factors [3].

Interleukin-18 (IL-18), initially identified as interferon-γ-inducing factor, plays a critical role in AOSD pathogenesis. IL-18 has various functions, such as inducing interferon-γ synthesis in T cells and natural killer (NK) cells, promoting Th1-type immune responses, and enhancing proliferative responses and cytokine production in activated T cells [4]. IL-18 has been linked to several inflammatory conditions, including acute liver injury, inflammatory arthritis, allergic inflammation, and other autoimmune diseases. The biological effects of IL-18 align with the key features of AOSD, indicating a potential connection between IL-18 dysregulation and AOSD [5]. The IL-18 gene, located on chromosome 11q22.2q22.3, includes promoters upstream of exons 1 and 2. Two significant single nucleotide polymorphisms (SNPs) at positions 607 and 137 in the promoter region of IL-18 exon 1 are of particular interest [6]. Given IL-18’s crucial role in the cytokine network and its overexpression in AOSD, researchers have focused on studying the relationship between blood IL-18 levels, IL-18 gene polymorphisms, and AOSD susceptibility.

Although many studies have investigated these associations, debates continue about whether serum IL-18 levels are reliable markers of disease activity [7-19]. Additionally, the role of IL-18 polymorphisms in AOSD onset remains controversial, with earlier studies yielding inconsistent results. To resolve these issues, a comprehensive review and meta-analysis are needed to better understand the complex relationship between IL-18 and AOSD [20]. The objectives of this study were to systematically review evidence on serum/plasma IL-18 levels in AOSD patients versus controls, determine IL-18 serum levels in active versus inactive AOSD, correlate these levels with other disease activity markers, and investigate the link between IL-18 polymorphisms and AOSD susceptibility.

Selection of relevant studies and data compilation

We conducted a comprehensive search of scientific literature to identify studies that measured circulating IL-18 levels (plasma or serum), explored the association between AOSD and IL-18 gene polymorphisms, and analyzed the relationship between these IL-18 levels and AOSD. Searches were performed on PubMed, Embase, and Cochrane Databases for all relevant publications up to June 2024. The search terms included &quot;interleukin-18,&quot; &quot;serum OR plasma OR circulating OR blood,&quot; &quot;polymorphism,&quot; and &quot;adult-onset Still’s disease.&quot; Additionally, we manually reviewed the references of retrieved articles to identify any further relevant studies not indexed in these databases.

Eligible studies were required to be case-control, cohort, or cross-sectional in design and to provide data on IL-18 levels in both affected and control groups, as well as information on IL-18 gene polymorphisms in both AOSD and control groups. We excluded studies that provided duplicate data, case reports, reviews, or those lacking sufficient information. For each selected study, we collected data on the author, publication year, country, ethnicity, age, sex, number of participants, mean and standard deviation of IL-18 levels, and genotype and allele frequencies of IL-18 polymorphisms. When data were reported as ranges, medians, or interquartile ranges, we converted these to means and standard deviations using established formulas [21,22].

Two independent evaluators, who were part of the initial study, reviewed and disclosed the study methods and findings. Discrepancies between reviewers were resolved by consensus. Each study’s quality was assessed using the Newcastle-Ottawa Scale [23], and we adhered to Preferred Reporting Items for Systematic Reviews and Meta-Analyses guidelines throughout the process [24].

Statistical correlation analysis

We performed a meta-analysis to examine the allelic effects of various IL-18 gene variations and the association between AOSD and IL-18 levels. The results are presented as 95% confidence intervals (CIs) for continuous data and mean and standard deviation. For dichotomous data, we calculated 95% CIs and odds ratios (ORs). Variations and heterogeneities within and across studies were assessed using Cochran’s Q tests [25]. A heterogeneity test was used to test the null hypothesis that each study estimated the same effect. For meta-analysis, a fixed-effects model was used unless the Q-statistic indicated significant heterogeneity (p<0.10), in which case a random-effects model was applied [26]. The influence of heterogeneity was quantified using I2=100%×(Q-df)/Q [27], which determines whether total variation across trials is due to chance or heterogeneity and measures the inconsistency between studies. I2 values ranged from 0% to 100%, with thresholds of 25%, 50%, and 75% representing low, moderate, and high levels of I2, respectively [27]. Statistical analyses were conducted using the Comprehensive Meta-Analysis software (Biostat Inc., Englewood, NJ, USA).

Evaluation of risks and publication bias

To explore potential sources of heterogeneity in the meta-analysis, we used explanatory variables such as ethnicity, publication year, sample size, matched variables, data type, and study quality. Sensitivity analysis was performed by eliminating one study at a time to determine its effect on the overall effect size. Funnel plots and Egger’s linear regression test were used to assess the presence of publication bias [28], utilizing standard mean differences (SMDs) or ORs on a natural logarithmic scale to evaluate funnel plot asymmetry.

Studies included in the meta-analysis

We identified 573 publications using both manual and computerized search methods. From these, 19 were selected for full-text review based on their titles and abstracts, while six were excluded due to a lack of IL-18 data. Ultimately, 13 studies, comprising 562 AOSD patients and 790 controls, were included in the meta-analysis (Figure 1) [7-19]. Ten studies analyzed IL-18 levels in affected and control groups in a meta-analysis (Table 1) [7-16], and three studies on IL-18 polymorphisms were included in the systematic review (Table 2) [17-19]. Each study received a quality grade between six and seven. The demographics of the participants and quality assessments are summarized in Tables 1 and 2.

Table 1 . Characteristics of individual studies included in the meta-analysis (IL-18 level)

AuthorCountryEthnicityCohort size (n)IL-18 level (pg/mL or ng/L)Statistical findingStudy quality
CaseControlCaseControlSMDMagnitude*p-value
Chen et al. [9]ChinaAsian23313496.007.561.173Large<0.0016
Ichikawa et al. [10]JapanAsian25122267.6072.105.855Large<0.0016
Hung et al. [11]TaiwanAsian66128977.70142.103.676Large<0.0017
Kim et al. [12]KoreaAsian13193016.2030.001.976Small<0.0016
Jung et al. [13]KoreaAsian803027219.60211.500.603Moderate<0.0017
Colafrancesco et al. [7]ItalyEuropean16212424.70227.000.689Moderate0.0436
Kim et al. [14]KoreaAsian36337560.30139.201.355Large<0.0016
Priori et al. [8]UKEuropean21212366.70212.000.639Moderate0.0436
Chen et al. [15]TaiwanAsian5020506.1860.231.070Large<0.0016
Choi et al. [16]KoreaAsian141565.9010.002.950Large<0.0016

IL-18: interleukin-18, SMD: standard mean difference, n: number. *Magnitude of Cohen’s d effect size where 0.2 to 0.5 is a small effect, 0.5 to 0.8 is a medium effect, and ≥0.8 is a large effect. †Newcastle-Ottawa Scale.



Table 2 . Characteristics of individual studies included in systematic review (IL-18 polymorphisms)

AuthorCountryEthnicityCohort size (n)IL-18 gene and polymorphism testedStatistical finding (p-value)NOS score
CaseControl
Chen et al. [17]ChinaAsian96164–607 C/A–607 AA (p<0.05)7
Her et al. [18]KoreaAsian70204–607 C/A, –137 G/C–607 C/A (p=0.044), –137 G/C (NS)7
Sugiura et al. [19]JapanAsian1692C to T substitution at position –5890 (SNP1), A to G at position –5316 (SNP2), T to C at position –5207 (SNP3), T to C at position –4762 (SNP4), C to G at position –4675 (SNP5), T to C at position –3268 (SNP6), C to T at position –2835 (SNP7), T to C at position –2565 (SNP8), G to T at position –689 (SNP9), C to A at position –640 (SNP10), and a 9 bp (AACAGGACA) insertion between positions –6311 and –6310SNP1, 2, 4, 5, 6, 9, and 10 and the 9 bp insertion (p<0.05)7

IL-18: interleukin-18, n: number, NS: not significant, NOS: Newcastle-Ottawa Scale.



Fig. 1. Flowchart depicting the study selection process for the meta-analysis.

Comparison of circulating IL-18 levels between AOSD patients and healthy controls

The meta-analysis revealed that IL-18 levels were significantly higher in the AOSD group compared to the control group (SMD=1.899, 95% CI=1.078~2.720, p<0.001) (Table 3, Figure 2) [7-16]. Subgroup analyses were conducted based on ethnicity, age, sex, sample size, and data type. Both Asian and European populations exhibited higher IL-18 levels in the AOSD group according to ethnicity-based stratification (Table 3). Subgroup analysis consistently showed significantly higher IL-18 levels in the AOSD group across all variables. Higher IL-18 levels were also observed in both small (n<50) and large groups (n>50), as well as in original and imputed data groups (Table 3). No significant difference in IL-18 levels was found between active and inactive disease groups. There were two studies on free IL-18 in AOSD [13,29]. Free IL-18 levels were significantly higher in the active group compared to the inactive group (SMD=0.900, 95% CI=0.532~1.268, p<0.001) (Table 3).

Table 3 . Meta-analysis of the association between circulating IL-18 levels and AOSD

GroupPopulationNo. of studyTest of associationTest of heterogeneity
SMD*95% CIp-valueModelp-valueI2
AllOverall101.8991.078~2.720<0.001R<0.00194.2
EthnicityAsian82.2281.254~3.201<0.001R<0.00194.9
European20.6620.208~1.1170.004F0.9150
Matched for age and sexYes62.4061.259~3.553<0.001R<0.00194.9
No41.6010.326~1.8760.005R0.00182.5
Sample sizen>5051.5770.437~2.7170.001R<0.00196.0
n<5052.2980.896~3.7000.001R<0.00192.5
Data typeOriginal41.1740.660~1.688<0.001R0.01870.0
Calculated62.4131.034~3.7910.001R<0.00195.7
Disease activityActive vs. Inactive group32.099–0.390~4.5890.098R<0.00194.1
Disease activity (free IL-18)Active vs. Inactive group30.9000.532~1.268<0.001F0.9360

IL-18: interleukin-18, AOSD: adult-onset Still’s disease, SMD: standardized mean difference, CI: confidence interval, n: number, F: fixed effects model, R: random effects model, NA: not available. *Magnitude of Cohen’s d effect size (SMD): 0.2~0.5, small effect; 0.5~0.8, medium effect; ≥0.8, large effect.



Fig. 2. Meta-analysis illustrating the relationship between circulating IL-18 levels and AOSD. IL-18: interleukin-18, AOSD: adult-onset Still’s disease, CI: confidence interval.

Correlation between IL-18 levels and activity markers

The meta-analysis demonstrated a positive correlation between IL-18 and ferritin levels (correlation coefficient=0.542, 95% CI=0.431~0.637, p<0.001) (Table 4, Figure 3A) [7,13-16]. Additionally, IL-18 showed positive correlations with C-reactive protein (CRP) (correlation coefficient=0.306, 95% CI=0.168~0.431, p<0.001) (Table 4, Figure 3B) [7,13-16].

Table 4 . Meta-analysis of the correlation coefficient between IL-18 level and ferritin, CRP in AOSD

ParameterNo. of studyTest of associationTest of heterogeneity
Correlation coefficient95% CIp-valueModelp-valueI2
Ferritin50.5420.431~0.637<0.001F0.26723.1
CRP50.3060.168~0.431<0.001F0.7350

IL-18: interleukin-18, CRP: C-reactive protein, AOSD: adult-onset Still’s disease, CI: confidence interval, F: fixed effects model.



Fig. 3. Meta-analysis showing the correlation coefficient between circulating IL-18 levels and ferritin (A), as well as CRP (B). IL-18: interleukin-18, CRP: C-reactive protein, CI: confidence interval.

IL-18 polymorphisms and AOSD: a systematic review

Three studies were included in this review. One study suggested that the A allele and AA genotype at position –607 of IL-18 gene polymorphisms could be genetic risk factors for AOSD in the Korean population. Patients with AOSD had a significantly higher frequency of AA genotypes at –607 compared to controls (AA vs. CA and CC, OR=1.90, 95% CI=1.01~3.58, p=0.044) [18]. Another study indicated that the SNP 607/AA genotype, associated with lower IL-18 levels, might be a genetic protective factor against AOSD in the Chinese population. Significantly lower frequencies of the –607/AA genotype were observed in AOSD patients compared to controls (18.8% vs. 31.1%, respectively; p<0.05). Median serum IL-18 levels were significantly lower in AOSD patients with the AA genotype compared to those with the CA or CC genotypes [17]. The last Japanese study investigated a 6.7 kb region upstream of exon 2 of the IL-18 gene, which included promoter activity, and identified seven SNPs and a single 9 bp insertion frequently present in AOSD patients [19]. This study found a significantly higher frequency of individuals carrying the S01/S01 genotype in AOSD patients compared to healthy controls (OR=7.81, 95% CI=2.48~24.65, p<0.001) [19].

Heterogeneity, sensitivity test, and publication bias

Heterogeneity was observed in the meta-analysis of IL-18 levels in AOSD patients (Table 3). A significant portion of the variability was attributed to different effect sizes, although the effect sizes were consistently oriented across studies. Significant heterogeneity was noted in the meta-analysis of IL-18 levels in relation to sample size and ethnicity (p<0.05); however, study quality, data format, and publication year had no significant impact on heterogeneity based on meta-regression tests. Sensitivity analysis indicated that the inclusion or exclusion of any single study did not affect the meta-analysis results, demonstrating reliability. We found no evidence of publication bias, as indicated by the absence of asymmetry in the funnel plot and non-significant Egger’s regression test results (p>0.05).

This study shows that the significant increase in circulating IL-18 levels among patients with AOSD compared to controls underscores the potential role of this cytokine in the disease’s pathogenesis. Higher IL-18 levels observed in both Asian and European populations with AOSD suggest the broad applicability of these results across different ethnic groups. This meta-analysis revealed a positive correlation between IL-18 levels and established inflammation markers, ferritin, and CRP, strengthening the argument that IL-18 is involved in the inflammatory processes associated with AOSD. The lack of significant differences in IL-18 levels between active and inactive disease groups is noted. This discrepancy may be due to the comparison of total IL-18 levels rather than free IL-18 levels. It is possible that free IL-18 levels differ between active and inactive patients with AOSD [29]. Therefore, free IL-18 levels or the IL-18/IL-18 binding protein ratio imbalance may serve as more useful biomarkers for AOSD [30]. We included a comparison based on free IL-18 levels as a subgroup analysis. Free IL-18 levels were significantly higher in the active group compared to the inactive group (SMD=0.900, 95% CI=0.532~1.268, p<0.001).

The IL-18 gene polymorphisms, particularly the –607 C/A polymorphism, may be a susceptibility factor for AOSD, implying a potential genetic predisposition related to the regulatory regions of IL-18. The A allele at position 607 in the IL-18 promoter region may be linked to susceptibility to AOSD in the Korean population [18]. This allele, part of haplotype of the IL-18 gene reported by Sugiura et al. [19], was associated with AOSD development in a Japanese population. However, lower frequencies of single-nucleotide polymorphisms (607/AA) were observed in Chinese patients with AOSD compared to healthy controls [17], suggesting variation in genetic susceptibility among ethnic groups. Genetic studies suggest that the regulatory regions of IL-18 are associated with AOSD development. The A allele at position –607 in the IL-18 promoter region was associated with the susceptibility to AOSD in Korean and Japanese populations, but the SNP –607/AA genotype was a protective factor against occurrence of AOSD in the Chinese population. Population-specific genetic backgrounds and environmental influences likely contribute to the observed differences in the role of the –607/AA genotype in AOSD susceptibility between Korean, Japanese, and Chinese populations.

Elevated IL-18 levels enhance the activation of various immune cells, leading to an exaggerated inflammatory response [1]. IL-18 contributes directly to disease activity through multiple mechanisms, including the promotion of pro-inflammatory Th1 responses, the induction of cytokine and chemokine production, the activation of NK cells, and the promotion of apoptosis and tissue damage [31]. IL-18’s ability to promote Th1-type immune responses may be a key mechanism underlying AOSD [3]. The upregulation of Th1 cytokines, such as interferon-γ, may perpetuate the inflammatory cascade, contributing to the clinical manifestations of AOSD. The positive correlation between IL-18 levels, ferritin, and CRP levels suggests that IL-18 amplifies inflammatory responses, stimulating the production of these acute-phase reactants and contributing to the systemic inflammation and clinical manifestations of AOSD. The correlation with ferritin, a marker of macrophage activation, implies that IL-18 may be involved in macrophage dysregulation, contributing to the hyperinflammatory state observed in AOSD [32]. Polymorphisms in the IL-18 gene, such as the –607 C/A variant, may modulate IL-18 expression. Genetic predisposition through variations in the regulatory regions of IL-18 could influence IL-18 production and release, contributing to AOSD susceptibility. Genetic variations may lead to an altered immune response, affecting the balance between pro- and anti-inflammatory signals, potentially triggering or exacerbating AOSD. Higher IL-18 concentrations have been measured in AOSD patients with macrophage activation syndrome (MAS) than patients with an active disease without MAS [33]. IL-18 plays a central role in the pathogenesis of MAS in AOSD by driving the hyperinflammatory response, promoting cytokine storms, and contributing to the dysfunction of immune cells like NK cells [5]. IL-18 has a role comparable to IL-1β, but unlike IL-1β, which is not reliably detected in peripheral blood, IL-18 or free IL-18 can be measured in peripheral blood using ELISA (enzyme-linked immunosorbent assay) [34]. This makes IL-18, along with ferritin and CRP, an important biomarker for diagnosing AOSD, evaluating disease activity, and predicting outcomes, such as the risk of progression to MAS. On the other hand, IL-6 is more strongly linked to articular symptoms rather than systemic manifestations in AOSD.

It is important to acknowledge the limitations of this meta-analysis. First, the limited number of included studies may have reduced the statistical power. Second, considerable variability among the included studies may have compromised the reliability of the conclusions. We performed the subgroup analysis and meta-regression test to explore potential sources of heterogeneity. Subgroup analysis showed no heterogeneity in Europeans and meta-regression test revealed ethnicity and sample size had significant impact on heterogeneity. Third, the predominant use of a cross-sectional design in the included studies poses challenges in establishing a causal relationship between IL-18 and AOSD. Therefore, longitudinal studies or larger cohort studies are necessary to establish causality between IL-18 and AOSD. Nevertheless, this meta-analysis has strengths. To our knowledge, this is the first study to concurrently examine two key aspects: IL-18 levels and polymorphisms in IL-18-encoding loci in patients with AOSD. Despite individual trial cohort sizes ranging from 13 to 204 patients, our combined analysis included 562 patients. Moreover, our approach, which combined findings from multiple independent analyses, enhanced the statistical power and resolution of the study [35].

This meta-analysis revealed a significant elevation in circulating IL-18 levels in patients with AOSD compared to controls, showed a positive correlation between IL-18 levels and ferritin and CRP levels, and suggested an association between IL-18 polymorphisms and AOSD susceptibility. These findings suggest a crucial role for IL-18 in the pathogenesis of AOSD. However, further investigations are necessary to determine the direct contribution of IL-18 to AOSD pathogenesis.

Y.H.L. has been an editorial board member since March 2013, but has no role in the decision to publish this article.

Y.H.L. was involved in conception and design of study, acquisition of data, analysis and/or interpretation of data, drafting the manuscript, revising the manuscript critically for important intellectual content. G.G.S. was involved in conception and design of study, analysis and interpretation of data, and drafting the manuscript.

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Article

Original Article

J Rheum Dis 2025; 32(1): 48-56

Published online January 1, 2025 https://doi.org/10.4078/jrd.2024.0095

Copyright © Korean College of Rheumatology.

Associations between circulating interleukin-18 levels and adult-onset Still’s disease: a meta-analysis

Young Ho Lee , M.D., Ph.D., Gwan Gyu Song , M.D., Ph.D.

Division of Rheumatology, Department of Internal Medicine, Korea University Medical Center, Korea University College of Medicine, Seoul, Korea

Correspondence to:Young Ho Lee, https://orcid.org/0000-0003-4213-1909
Division of Rheumatology, Department of Internal Medicine, Korea University Anam Hospital, Korea University College of Medicine, 73 Goryeodae-ro, Seongbuk-gu, Seoul 02841, Korea. E-mail: lyhcgh@korea.ac.kr

Received: August 1, 2024; Revised: September 18, 2024; Accepted: October 17, 2024

This is an Open Access article distributed under the terms of the Creative Commons Attribution Non-Commercial License (http://creativecommons.org/licenses/by-nc/4.0) which permits unrestricted non-commercial use, distribution, and reproduction in any medium, provided the original work is properly cited.

Abstract

Objective: This study aimed to investigate the link between circulating interleukin-18 (IL-18) levels and adult-onset Still’s disease (AOSD).
Methods: A thorough search was performed on MEDLINE, Embase, and Web of Science to find relevant articles. A meta-analysis was conducted to compare serum/plasma IL-18 levels in AOSD patients to those in control subjects.
Results: The meta-analysis included 13 studies with a total of 562 AOSD patients and 790 controls. The results showed a significant increase in IL-18 levels in the AOSD group compared to the control group (standard mean difference [SMD]=1.899, 95% confidence interval [CI]=1.078~2.720, p<0.001). When stratified by ethnicity, higher IL-18 levels were found in both Asian and European populations with AOSD. Subgroup analysis, regardless of variable adjustments, consistently indicated significantly higher IL-18 levels in the AOSD group. Significant elevations in IL-18 levels were observed in both small (n<50) and large groups (n>50), as well as in original and imputed data groups after data type stratification. Free IL-18 levels were significantly higher in the active group compared to the inactive group (SMD=0.900, 95% CI=0.532~1.268, p<0.001). The meta-analysis showed a positive correlation between IL-18 levels and ferritin (correlation coefficient=0.542, 95% CI=0.431~0.637, p<0.001) and C-reactive protein.
Conclusion: This meta-analysis demonstrated a significant increase in circulating IL-18 levels and a positive correlation between IL-18 levels and ferritin and C-reactive protein levels in patients with AOSD.

Keywords: Adult-onset Still’s disease, Interleukin-18, Ferritin, Polymorphism, Genetic, Meta-analysis

INTRODUCTION

Adult-onset Still’s disease (AOSD) is a systemic inflammatory condition marked by a range of clinical symptoms such as spiking fever, transient skin rash, joint pain or arthritis, sore throat, and enlarged liver or spleen [1,2]. Diagnostic laboratory findings often include neutrophilic leukocytosis, abnormal liver function tests, high serum ferritin levels, and increased acute-phase reactants. Despite significant medical advancements, the precise cause of AOSD remains unknown. Active AOSD is characterized by immune-mediated inflammation, typically triggered by abnormal immune responses in genetically predisposed individuals exposed to environmental factors [3].

Interleukin-18 (IL-18), initially identified as interferon-γ-inducing factor, plays a critical role in AOSD pathogenesis. IL-18 has various functions, such as inducing interferon-γ synthesis in T cells and natural killer (NK) cells, promoting Th1-type immune responses, and enhancing proliferative responses and cytokine production in activated T cells [4]. IL-18 has been linked to several inflammatory conditions, including acute liver injury, inflammatory arthritis, allergic inflammation, and other autoimmune diseases. The biological effects of IL-18 align with the key features of AOSD, indicating a potential connection between IL-18 dysregulation and AOSD [5]. The IL-18 gene, located on chromosome 11q22.2q22.3, includes promoters upstream of exons 1 and 2. Two significant single nucleotide polymorphisms (SNPs) at positions 607 and 137 in the promoter region of IL-18 exon 1 are of particular interest [6]. Given IL-18’s crucial role in the cytokine network and its overexpression in AOSD, researchers have focused on studying the relationship between blood IL-18 levels, IL-18 gene polymorphisms, and AOSD susceptibility.

Although many studies have investigated these associations, debates continue about whether serum IL-18 levels are reliable markers of disease activity [7-19]. Additionally, the role of IL-18 polymorphisms in AOSD onset remains controversial, with earlier studies yielding inconsistent results. To resolve these issues, a comprehensive review and meta-analysis are needed to better understand the complex relationship between IL-18 and AOSD [20]. The objectives of this study were to systematically review evidence on serum/plasma IL-18 levels in AOSD patients versus controls, determine IL-18 serum levels in active versus inactive AOSD, correlate these levels with other disease activity markers, and investigate the link between IL-18 polymorphisms and AOSD susceptibility.

MATERIALS AND METHODS

Selection of relevant studies and data compilation

We conducted a comprehensive search of scientific literature to identify studies that measured circulating IL-18 levels (plasma or serum), explored the association between AOSD and IL-18 gene polymorphisms, and analyzed the relationship between these IL-18 levels and AOSD. Searches were performed on PubMed, Embase, and Cochrane Databases for all relevant publications up to June 2024. The search terms included &quot;interleukin-18,&quot; &quot;serum OR plasma OR circulating OR blood,&quot; &quot;polymorphism,&quot; and &quot;adult-onset Still’s disease.&quot; Additionally, we manually reviewed the references of retrieved articles to identify any further relevant studies not indexed in these databases.

Eligible studies were required to be case-control, cohort, or cross-sectional in design and to provide data on IL-18 levels in both affected and control groups, as well as information on IL-18 gene polymorphisms in both AOSD and control groups. We excluded studies that provided duplicate data, case reports, reviews, or those lacking sufficient information. For each selected study, we collected data on the author, publication year, country, ethnicity, age, sex, number of participants, mean and standard deviation of IL-18 levels, and genotype and allele frequencies of IL-18 polymorphisms. When data were reported as ranges, medians, or interquartile ranges, we converted these to means and standard deviations using established formulas [21,22].

Two independent evaluators, who were part of the initial study, reviewed and disclosed the study methods and findings. Discrepancies between reviewers were resolved by consensus. Each study’s quality was assessed using the Newcastle-Ottawa Scale [23], and we adhered to Preferred Reporting Items for Systematic Reviews and Meta-Analyses guidelines throughout the process [24].

Statistical correlation analysis

We performed a meta-analysis to examine the allelic effects of various IL-18 gene variations and the association between AOSD and IL-18 levels. The results are presented as 95% confidence intervals (CIs) for continuous data and mean and standard deviation. For dichotomous data, we calculated 95% CIs and odds ratios (ORs). Variations and heterogeneities within and across studies were assessed using Cochran’s Q tests [25]. A heterogeneity test was used to test the null hypothesis that each study estimated the same effect. For meta-analysis, a fixed-effects model was used unless the Q-statistic indicated significant heterogeneity (p<0.10), in which case a random-effects model was applied [26]. The influence of heterogeneity was quantified using I2=100%×(Q-df)/Q [27], which determines whether total variation across trials is due to chance or heterogeneity and measures the inconsistency between studies. I2 values ranged from 0% to 100%, with thresholds of 25%, 50%, and 75% representing low, moderate, and high levels of I2, respectively [27]. Statistical analyses were conducted using the Comprehensive Meta-Analysis software (Biostat Inc., Englewood, NJ, USA).

Evaluation of risks and publication bias

To explore potential sources of heterogeneity in the meta-analysis, we used explanatory variables such as ethnicity, publication year, sample size, matched variables, data type, and study quality. Sensitivity analysis was performed by eliminating one study at a time to determine its effect on the overall effect size. Funnel plots and Egger’s linear regression test were used to assess the presence of publication bias [28], utilizing standard mean differences (SMDs) or ORs on a natural logarithmic scale to evaluate funnel plot asymmetry.

RESULTS

Studies included in the meta-analysis

We identified 573 publications using both manual and computerized search methods. From these, 19 were selected for full-text review based on their titles and abstracts, while six were excluded due to a lack of IL-18 data. Ultimately, 13 studies, comprising 562 AOSD patients and 790 controls, were included in the meta-analysis (Figure 1) [7-19]. Ten studies analyzed IL-18 levels in affected and control groups in a meta-analysis (Table 1) [7-16], and three studies on IL-18 polymorphisms were included in the systematic review (Table 2) [17-19]. Each study received a quality grade between six and seven. The demographics of the participants and quality assessments are summarized in Tables 1 and 2.

Table 1 . Characteristics of individual studies included in the meta-analysis (IL-18 level).

AuthorCountryEthnicityCohort size (n)IL-18 level (pg/mL or ng/L)Statistical findingStudy quality
CaseControlCaseControlSMDMagnitude*p-value
Chen et al. [9]ChinaAsian23313496.007.561.173Large<0.0016
Ichikawa et al. [10]JapanAsian25122267.6072.105.855Large<0.0016
Hung et al. [11]TaiwanAsian66128977.70142.103.676Large<0.0017
Kim et al. [12]KoreaAsian13193016.2030.001.976Small<0.0016
Jung et al. [13]KoreaAsian803027219.60211.500.603Moderate<0.0017
Colafrancesco et al. [7]ItalyEuropean16212424.70227.000.689Moderate0.0436
Kim et al. [14]KoreaAsian36337560.30139.201.355Large<0.0016
Priori et al. [8]UKEuropean21212366.70212.000.639Moderate0.0436
Chen et al. [15]TaiwanAsian5020506.1860.231.070Large<0.0016
Choi et al. [16]KoreaAsian141565.9010.002.950Large<0.0016

IL-18: interleukin-18, SMD: standard mean difference, n: number. *Magnitude of Cohen’s d effect size where 0.2 to 0.5 is a small effect, 0.5 to 0.8 is a medium effect, and ≥0.8 is a large effect. †Newcastle-Ottawa Scale..



Table 2 . Characteristics of individual studies included in systematic review (IL-18 polymorphisms).

AuthorCountryEthnicityCohort size (n)IL-18 gene and polymorphism testedStatistical finding (p-value)NOS score
CaseControl
Chen et al. [17]ChinaAsian96164–607 C/A–607 AA (p<0.05)7
Her et al. [18]KoreaAsian70204–607 C/A, –137 G/C–607 C/A (p=0.044), –137 G/C (NS)7
Sugiura et al. [19]JapanAsian1692C to T substitution at position –5890 (SNP1), A to G at position –5316 (SNP2), T to C at position –5207 (SNP3), T to C at position –4762 (SNP4), C to G at position –4675 (SNP5), T to C at position –3268 (SNP6), C to T at position –2835 (SNP7), T to C at position –2565 (SNP8), G to T at position –689 (SNP9), C to A at position –640 (SNP10), and a 9 bp (AACAGGACA) insertion between positions –6311 and –6310SNP1, 2, 4, 5, 6, 9, and 10 and the 9 bp insertion (p<0.05)7

IL-18: interleukin-18, n: number, NS: not significant, NOS: Newcastle-Ottawa Scale..



Figure 1. Flowchart depicting the study selection process for the meta-analysis.

Comparison of circulating IL-18 levels between AOSD patients and healthy controls

The meta-analysis revealed that IL-18 levels were significantly higher in the AOSD group compared to the control group (SMD=1.899, 95% CI=1.078~2.720, p<0.001) (Table 3, Figure 2) [7-16]. Subgroup analyses were conducted based on ethnicity, age, sex, sample size, and data type. Both Asian and European populations exhibited higher IL-18 levels in the AOSD group according to ethnicity-based stratification (Table 3). Subgroup analysis consistently showed significantly higher IL-18 levels in the AOSD group across all variables. Higher IL-18 levels were also observed in both small (n<50) and large groups (n>50), as well as in original and imputed data groups (Table 3). No significant difference in IL-18 levels was found between active and inactive disease groups. There were two studies on free IL-18 in AOSD [13,29]. Free IL-18 levels were significantly higher in the active group compared to the inactive group (SMD=0.900, 95% CI=0.532~1.268, p<0.001) (Table 3).

Table 3 . Meta-analysis of the association between circulating IL-18 levels and AOSD.

GroupPopulationNo. of studyTest of associationTest of heterogeneity
SMD*95% CIp-valueModelp-valueI2
AllOverall101.8991.078~2.720<0.001R<0.00194.2
EthnicityAsian82.2281.254~3.201<0.001R<0.00194.9
European20.6620.208~1.1170.004F0.9150
Matched for age and sexYes62.4061.259~3.553<0.001R<0.00194.9
No41.6010.326~1.8760.005R0.00182.5
Sample sizen>5051.5770.437~2.7170.001R<0.00196.0
n<5052.2980.896~3.7000.001R<0.00192.5
Data typeOriginal41.1740.660~1.688<0.001R0.01870.0
Calculated62.4131.034~3.7910.001R<0.00195.7
Disease activityActive vs. Inactive group32.099–0.390~4.5890.098R<0.00194.1
Disease activity (free IL-18)Active vs. Inactive group30.9000.532~1.268<0.001F0.9360

IL-18: interleukin-18, AOSD: adult-onset Still’s disease, SMD: standardized mean difference, CI: confidence interval, n: number, F: fixed effects model, R: random effects model, NA: not available. *Magnitude of Cohen’s d effect size (SMD): 0.2~0.5, small effect; 0.5~0.8, medium effect; ≥0.8, large effect..



Figure 2. Meta-analysis illustrating the relationship between circulating IL-18 levels and AOSD. IL-18: interleukin-18, AOSD: adult-onset Still’s disease, CI: confidence interval.

Correlation between IL-18 levels and activity markers

The meta-analysis demonstrated a positive correlation between IL-18 and ferritin levels (correlation coefficient=0.542, 95% CI=0.431~0.637, p<0.001) (Table 4, Figure 3A) [7,13-16]. Additionally, IL-18 showed positive correlations with C-reactive protein (CRP) (correlation coefficient=0.306, 95% CI=0.168~0.431, p<0.001) (Table 4, Figure 3B) [7,13-16].

Table 4 . Meta-analysis of the correlation coefficient between IL-18 level and ferritin, CRP in AOSD.

ParameterNo. of studyTest of associationTest of heterogeneity
Correlation coefficient95% CIp-valueModelp-valueI2
Ferritin50.5420.431~0.637<0.001F0.26723.1
CRP50.3060.168~0.431<0.001F0.7350

IL-18: interleukin-18, CRP: C-reactive protein, AOSD: adult-onset Still’s disease, CI: confidence interval, F: fixed effects model..



Figure 3. Meta-analysis showing the correlation coefficient between circulating IL-18 levels and ferritin (A), as well as CRP (B). IL-18: interleukin-18, CRP: C-reactive protein, CI: confidence interval.

IL-18 polymorphisms and AOSD: a systematic review

Three studies were included in this review. One study suggested that the A allele and AA genotype at position –607 of IL-18 gene polymorphisms could be genetic risk factors for AOSD in the Korean population. Patients with AOSD had a significantly higher frequency of AA genotypes at –607 compared to controls (AA vs. CA and CC, OR=1.90, 95% CI=1.01~3.58, p=0.044) [18]. Another study indicated that the SNP 607/AA genotype, associated with lower IL-18 levels, might be a genetic protective factor against AOSD in the Chinese population. Significantly lower frequencies of the –607/AA genotype were observed in AOSD patients compared to controls (18.8% vs. 31.1%, respectively; p<0.05). Median serum IL-18 levels were significantly lower in AOSD patients with the AA genotype compared to those with the CA or CC genotypes [17]. The last Japanese study investigated a 6.7 kb region upstream of exon 2 of the IL-18 gene, which included promoter activity, and identified seven SNPs and a single 9 bp insertion frequently present in AOSD patients [19]. This study found a significantly higher frequency of individuals carrying the S01/S01 genotype in AOSD patients compared to healthy controls (OR=7.81, 95% CI=2.48~24.65, p<0.001) [19].

Heterogeneity, sensitivity test, and publication bias

Heterogeneity was observed in the meta-analysis of IL-18 levels in AOSD patients (Table 3). A significant portion of the variability was attributed to different effect sizes, although the effect sizes were consistently oriented across studies. Significant heterogeneity was noted in the meta-analysis of IL-18 levels in relation to sample size and ethnicity (p<0.05); however, study quality, data format, and publication year had no significant impact on heterogeneity based on meta-regression tests. Sensitivity analysis indicated that the inclusion or exclusion of any single study did not affect the meta-analysis results, demonstrating reliability. We found no evidence of publication bias, as indicated by the absence of asymmetry in the funnel plot and non-significant Egger’s regression test results (p>0.05).

DISCUSSION

This study shows that the significant increase in circulating IL-18 levels among patients with AOSD compared to controls underscores the potential role of this cytokine in the disease’s pathogenesis. Higher IL-18 levels observed in both Asian and European populations with AOSD suggest the broad applicability of these results across different ethnic groups. This meta-analysis revealed a positive correlation between IL-18 levels and established inflammation markers, ferritin, and CRP, strengthening the argument that IL-18 is involved in the inflammatory processes associated with AOSD. The lack of significant differences in IL-18 levels between active and inactive disease groups is noted. This discrepancy may be due to the comparison of total IL-18 levels rather than free IL-18 levels. It is possible that free IL-18 levels differ between active and inactive patients with AOSD [29]. Therefore, free IL-18 levels or the IL-18/IL-18 binding protein ratio imbalance may serve as more useful biomarkers for AOSD [30]. We included a comparison based on free IL-18 levels as a subgroup analysis. Free IL-18 levels were significantly higher in the active group compared to the inactive group (SMD=0.900, 95% CI=0.532~1.268, p<0.001).

The IL-18 gene polymorphisms, particularly the –607 C/A polymorphism, may be a susceptibility factor for AOSD, implying a potential genetic predisposition related to the regulatory regions of IL-18. The A allele at position 607 in the IL-18 promoter region may be linked to susceptibility to AOSD in the Korean population [18]. This allele, part of haplotype of the IL-18 gene reported by Sugiura et al. [19], was associated with AOSD development in a Japanese population. However, lower frequencies of single-nucleotide polymorphisms (607/AA) were observed in Chinese patients with AOSD compared to healthy controls [17], suggesting variation in genetic susceptibility among ethnic groups. Genetic studies suggest that the regulatory regions of IL-18 are associated with AOSD development. The A allele at position –607 in the IL-18 promoter region was associated with the susceptibility to AOSD in Korean and Japanese populations, but the SNP –607/AA genotype was a protective factor against occurrence of AOSD in the Chinese population. Population-specific genetic backgrounds and environmental influences likely contribute to the observed differences in the role of the –607/AA genotype in AOSD susceptibility between Korean, Japanese, and Chinese populations.

Elevated IL-18 levels enhance the activation of various immune cells, leading to an exaggerated inflammatory response [1]. IL-18 contributes directly to disease activity through multiple mechanisms, including the promotion of pro-inflammatory Th1 responses, the induction of cytokine and chemokine production, the activation of NK cells, and the promotion of apoptosis and tissue damage [31]. IL-18’s ability to promote Th1-type immune responses may be a key mechanism underlying AOSD [3]. The upregulation of Th1 cytokines, such as interferon-γ, may perpetuate the inflammatory cascade, contributing to the clinical manifestations of AOSD. The positive correlation between IL-18 levels, ferritin, and CRP levels suggests that IL-18 amplifies inflammatory responses, stimulating the production of these acute-phase reactants and contributing to the systemic inflammation and clinical manifestations of AOSD. The correlation with ferritin, a marker of macrophage activation, implies that IL-18 may be involved in macrophage dysregulation, contributing to the hyperinflammatory state observed in AOSD [32]. Polymorphisms in the IL-18 gene, such as the –607 C/A variant, may modulate IL-18 expression. Genetic predisposition through variations in the regulatory regions of IL-18 could influence IL-18 production and release, contributing to AOSD susceptibility. Genetic variations may lead to an altered immune response, affecting the balance between pro- and anti-inflammatory signals, potentially triggering or exacerbating AOSD. Higher IL-18 concentrations have been measured in AOSD patients with macrophage activation syndrome (MAS) than patients with an active disease without MAS [33]. IL-18 plays a central role in the pathogenesis of MAS in AOSD by driving the hyperinflammatory response, promoting cytokine storms, and contributing to the dysfunction of immune cells like NK cells [5]. IL-18 has a role comparable to IL-1β, but unlike IL-1β, which is not reliably detected in peripheral blood, IL-18 or free IL-18 can be measured in peripheral blood using ELISA (enzyme-linked immunosorbent assay) [34]. This makes IL-18, along with ferritin and CRP, an important biomarker for diagnosing AOSD, evaluating disease activity, and predicting outcomes, such as the risk of progression to MAS. On the other hand, IL-6 is more strongly linked to articular symptoms rather than systemic manifestations in AOSD.

It is important to acknowledge the limitations of this meta-analysis. First, the limited number of included studies may have reduced the statistical power. Second, considerable variability among the included studies may have compromised the reliability of the conclusions. We performed the subgroup analysis and meta-regression test to explore potential sources of heterogeneity. Subgroup analysis showed no heterogeneity in Europeans and meta-regression test revealed ethnicity and sample size had significant impact on heterogeneity. Third, the predominant use of a cross-sectional design in the included studies poses challenges in establishing a causal relationship between IL-18 and AOSD. Therefore, longitudinal studies or larger cohort studies are necessary to establish causality between IL-18 and AOSD. Nevertheless, this meta-analysis has strengths. To our knowledge, this is the first study to concurrently examine two key aspects: IL-18 levels and polymorphisms in IL-18-encoding loci in patients with AOSD. Despite individual trial cohort sizes ranging from 13 to 204 patients, our combined analysis included 562 patients. Moreover, our approach, which combined findings from multiple independent analyses, enhanced the statistical power and resolution of the study [35].

CONCLUSION

This meta-analysis revealed a significant elevation in circulating IL-18 levels in patients with AOSD compared to controls, showed a positive correlation between IL-18 levels and ferritin and CRP levels, and suggested an association between IL-18 polymorphisms and AOSD susceptibility. These findings suggest a crucial role for IL-18 in the pathogenesis of AOSD. However, further investigations are necessary to determine the direct contribution of IL-18 to AOSD pathogenesis.

ACKNOWLEDGMENTS

None.

CONFLICT OF INTEREST

Y.H.L. has been an editorial board member since March 2013, but has no role in the decision to publish this article.

AUTHOR CONTRIBUTIONS

Y.H.L. was involved in conception and design of study, acquisition of data, analysis and/or interpretation of data, drafting the manuscript, revising the manuscript critically for important intellectual content. G.G.S. was involved in conception and design of study, analysis and interpretation of data, and drafting the manuscript.

Fig 1.

Figure 1.Flowchart depicting the study selection process for the meta-analysis.
Journal of Rheumatic Diseases 2025; 32: 48-56https://doi.org/10.4078/jrd.2024.0095

Fig 2.

Figure 2.Meta-analysis illustrating the relationship between circulating IL-18 levels and AOSD. IL-18: interleukin-18, AOSD: adult-onset Still’s disease, CI: confidence interval.
Journal of Rheumatic Diseases 2025; 32: 48-56https://doi.org/10.4078/jrd.2024.0095

Fig 3.

Figure 3.Meta-analysis showing the correlation coefficient between circulating IL-18 levels and ferritin (A), as well as CRP (B). IL-18: interleukin-18, CRP: C-reactive protein, CI: confidence interval.
Journal of Rheumatic Diseases 2025; 32: 48-56https://doi.org/10.4078/jrd.2024.0095

Table 1 . Characteristics of individual studies included in the meta-analysis (IL-18 level).

AuthorCountryEthnicityCohort size (n)IL-18 level (pg/mL or ng/L)Statistical findingStudy quality
CaseControlCaseControlSMDMagnitude*p-value
Chen et al. [9]ChinaAsian23313496.007.561.173Large<0.0016
Ichikawa et al. [10]JapanAsian25122267.6072.105.855Large<0.0016
Hung et al. [11]TaiwanAsian66128977.70142.103.676Large<0.0017
Kim et al. [12]KoreaAsian13193016.2030.001.976Small<0.0016
Jung et al. [13]KoreaAsian803027219.60211.500.603Moderate<0.0017
Colafrancesco et al. [7]ItalyEuropean16212424.70227.000.689Moderate0.0436
Kim et al. [14]KoreaAsian36337560.30139.201.355Large<0.0016
Priori et al. [8]UKEuropean21212366.70212.000.639Moderate0.0436
Chen et al. [15]TaiwanAsian5020506.1860.231.070Large<0.0016
Choi et al. [16]KoreaAsian141565.9010.002.950Large<0.0016

IL-18: interleukin-18, SMD: standard mean difference, n: number. *Magnitude of Cohen’s d effect size where 0.2 to 0.5 is a small effect, 0.5 to 0.8 is a medium effect, and ≥0.8 is a large effect. †Newcastle-Ottawa Scale..


Table 2 . Characteristics of individual studies included in systematic review (IL-18 polymorphisms).

AuthorCountryEthnicityCohort size (n)IL-18 gene and polymorphism testedStatistical finding (p-value)NOS score
CaseControl
Chen et al. [17]ChinaAsian96164–607 C/A–607 AA (p<0.05)7
Her et al. [18]KoreaAsian70204–607 C/A, –137 G/C–607 C/A (p=0.044), –137 G/C (NS)7
Sugiura et al. [19]JapanAsian1692C to T substitution at position –5890 (SNP1), A to G at position –5316 (SNP2), T to C at position –5207 (SNP3), T to C at position –4762 (SNP4), C to G at position –4675 (SNP5), T to C at position –3268 (SNP6), C to T at position –2835 (SNP7), T to C at position –2565 (SNP8), G to T at position –689 (SNP9), C to A at position –640 (SNP10), and a 9 bp (AACAGGACA) insertion between positions –6311 and –6310SNP1, 2, 4, 5, 6, 9, and 10 and the 9 bp insertion (p<0.05)7

IL-18: interleukin-18, n: number, NS: not significant, NOS: Newcastle-Ottawa Scale..


Table 3 . Meta-analysis of the association between circulating IL-18 levels and AOSD.

GroupPopulationNo. of studyTest of associationTest of heterogeneity
SMD*95% CIp-valueModelp-valueI2
AllOverall101.8991.078~2.720<0.001R<0.00194.2
EthnicityAsian82.2281.254~3.201<0.001R<0.00194.9
European20.6620.208~1.1170.004F0.9150
Matched for age and sexYes62.4061.259~3.553<0.001R<0.00194.9
No41.6010.326~1.8760.005R0.00182.5
Sample sizen>5051.5770.437~2.7170.001R<0.00196.0
n<5052.2980.896~3.7000.001R<0.00192.5
Data typeOriginal41.1740.660~1.688<0.001R0.01870.0
Calculated62.4131.034~3.7910.001R<0.00195.7
Disease activityActive vs. Inactive group32.099–0.390~4.5890.098R<0.00194.1
Disease activity (free IL-18)Active vs. Inactive group30.9000.532~1.268<0.001F0.9360

IL-18: interleukin-18, AOSD: adult-onset Still’s disease, SMD: standardized mean difference, CI: confidence interval, n: number, F: fixed effects model, R: random effects model, NA: not available. *Magnitude of Cohen’s d effect size (SMD): 0.2~0.5, small effect; 0.5~0.8, medium effect; ≥0.8, large effect..


Table 4 . Meta-analysis of the correlation coefficient between IL-18 level and ferritin, CRP in AOSD.

ParameterNo. of studyTest of associationTest of heterogeneity
Correlation coefficient95% CIp-valueModelp-valueI2
Ferritin50.5420.431~0.637<0.001F0.26723.1
CRP50.3060.168~0.431<0.001F0.7350

IL-18: interleukin-18, CRP: C-reactive protein, AOSD: adult-onset Still’s disease, CI: confidence interval, F: fixed effects model..


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JRD
Jan 01, 2025 Vol.32 No.1, pp. 1~7
COVER PICTURE
Cumulative growth of rheumatology members and specialists (1980~2024). Cumulative distribution of the number of the (A) Korean College of Rheumatology members and (B) rheumatology specialists. (J Rheum Dis 2025;32:63-65)

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