A systematic search was conducted for potential literature in two databases: PubMed and EMBASE (up to September 2019) . The key words used for the searches were as follows: “Interleukin-6 OR IL-6 OR Interleukin 6 OR IL6” and “systemic lupus erythematosus OR SLE.” No language or region limitations were used in the literature search.

Articles were included based on the following criteria: 1) case-control, cohort, or cross-sectional study designs in humans; 2) reports regarding details of serum IL-6 levels in SLE patients compared to those in normal controls and/or in SLE patients with active disease compared to inactive disease; 3) no limitations with regard to the definition of SLE activity; 4) reports regarding the mean and standard deviation/error of serum IL-6 levels.

The exclusion criteria included: 1) abstracts, case reports, animal studies, and reviews; 2) no full-text studies; 3) overlapping data; 4) insufficient data for meta-analysis, defined as reporting serum IL-6 levels without the mean and SD/SE.

The following data were extracted independently by two investigators: first author, publication year, country, sample size of active/inactive SLE patients and the matched normal controls, mean age, percent of females in the sample population, mean and the standard deviation of IL-6 levels of two groups (pg/mL), detection method, definition of active SLE, and Pearson/Spearman correlation coefficient between the IL-6 level and SLE disease activity.

The quality of included studies was assessed using the Newcastle-Ottawa scale (NOS), and the high-quality articles were defined as those with a score higher than 5.

The relationship between serum IL-6 levels and SLE was evaluated in the meta-analysis. For the continuous outcomes, we used standardized mean differences (SMDs) with 95% confidence intervals (95% CIs). For correlation coefficients, the published Spearman correlation coefficient (r) values were converted to Pearson correlation coefficient (r) values, which were used for the meta-analysis (14). After a Fisher r-to-z transformation for Pearson correlation coefficients (15,16), the pooled correlation coefficient results were presented as Fisher's z values with the 95% CIs (17). p<0.05 was considered statistically significant. The Q-statistic and I2 statistic test were used to evaluate heterogeneity. Significant heterogeneity was defined based on the criteria: PQ<0.1 or I2>50%, and a random-effects model was used to calculate the pooled results. Otherwise, a fixed-effects model was applied. To detect the increased heterogeneity, subgroup analysis was performed according to the region, age, and the IL-6 assay method. Sensitivity analysis was conducted to evaluate the influence of each study on the pooled results. Publication bias was assessed using funnel plots and the Begg's and Egger's tests (18–21). The symmetric of funnel plots or the p<0.05 of the Begg's or Egger's tests indicated statistically significant publication bias, and the ''trim-and-fill“ method was used to adjust the summary estimates (22). All heterogeneity, meta-analysis, and sensitivity tests of the extracted data were performed using Review Manager 5.3 (Review Manager, 2014). Publication bias assessment and ''trim-and-fill” analysis was conducted using STATA version 12.0 (Stata Corporation, College Station, TX, United States).

A total of 2619 articles were initially collected from PubMed and EMBASE. First, we excluded 1227 duplicate publications using EndNote X7 software. In next step, we reviewed titles and abstracts to further exclude 1351 articles featuring animal studies, cell experiments, unrelated topics, letters, and conference abstracts, and review articles. Then, we carefully reviewed the full text of the remaining 41 studies, removing 17 studies due to overlapping patient data and insufficient data. Finally, a total of 24 eligible studies were included in this meta-analysis (23–46). The flow chart of literature selection is presented in Figure 1.

Figure 1..

Flow chart of the selection process for eligible studies.

(0.09MB).

A total of 24 eligible studies with 1817 SLE patients and 874 healthy controls were included in this meta-analysis (23–46). These studies were published from 1996 to 2019. There were 12 studies enrolling patients from Asian countries (China (28,29,43,46), Japan (42), South Korea (26), Iran (36), Singapore (34), Malaysia (45), Thailand (44), and Turkey (32,33)). The serum IL-6 levels in most eligible studies were measured using enzyme-linked immunosorbent assay (ELISA) kits (23,24,26–29,31–33,37–39,41,43–45). The serum IL-6 levels ranged from 4.272±0.4222 to 123.71±81.783 (pg/mL) in SLE patients and 0.93±0.95 to 10.46±4.33 (pg/mL) in healthy controls. A total of 13 studies compared the serum IL-6 levels between SLE patients and healthy controls (23–25,27–29,32–34,39,40,43,46). Serum IL-6 levels between active and inactive SLE patients were compared in 9 studies (24–26,29,31,39,41–43). Additionally, the correlation coefficient between serum IL-6 level and SLE disease activity was reported in 13 studies (24–26,29–31,35–39,44,45). Among all included studies, 3 studies focused on children with SLE (25,28,46), and 21 studies focused on adults with SLE (23,24,26,27,29–45). The NOS scores for the included studies ranged from six to seven, indicating that they were of moderate to high quality and suitable for pooled analysis. The characteristics of the eligible studies are summarized in Table 1.

A total of 13 studies compared serum IL-6 levels between SLE patients (n=612) and healthy controls (n=376) (23–25,27–29,32–34,39,40,43,46). Among the 612 patients, 465 were female and 148 were male. Additionally, seven studies were from Asia, and six studies were conducted outside Asia. Moreover, ten studies only included adult patients with SLE, while three studies enrolled 161 children with SLE. Considering the significant heterogeneity (I2=97%, p<0.01), we used a random-effects model to perform the pooled analysis. We found that the serum IL-6 level was markedly higher in SLE patients than in healthy controls (pooled SMD: 2.12, 95% CI: 1.21-3.03, p<0.01) (Figure 2).

Figure 2..

Meta-analysis comparing the serum IL-6 levels in SLE patients and healthy controls.

(0.1MB).

A total of nine studies compared the serum IL-6 levels between patients with active SLE and inactive SLE (24–26,29,31,39,41–43). The random-effects model was used to perform the pooled analysis due to the significant heterogeneity (I2=96%, p<0.01). We found that the serum IL-6 level was significantly higher in active SLE patients than in the inactive SLE patients (pooled SMD: 2.12, 95% CI: 1.21-3.03) (Figure 3). Additionally, 13 studies assessed the correlation between the serum IL-6 level and SLE activity using correlation coefficients (24–26,29–31,35–39,44,45). Considering the significant heterogeneity (I2=60%, p<0.01), we also pooled these data using a random-effects model. As shown in Figure 4, there was a positive correlation between the serum IL-6 level and SLE activity (Fisher's z=0.36, 95% CI: 0.26-0.46, p<0.01).

Figure 3..

Meta-analysis comparing the serum IL-6 levels in active SLE patients and inactive SLE patients.

(0.12MB).

Figure 4..

Meta-analysis of the correlation between the serum IL-6 level and SLE activity.

(0.16MB).

To explore the source of heterogeneity for the overall pooled results, we conducted subgroup analyses based on age, region, assay method, and definition of disease activity. The results showed that SLE patients had a higher serum IL-6 level than healthy controls (Table 2), and the serum IL-6 level was positively correlated with SLE activity (Table 3) in the subgroup analyses with regard to the age, region, and assay method. Meanwhile, we observed that significant heterogeneity still existed in these subgroup analyses (Table 2 and 3). Thus, age, region, or assay method might not be a source of heterogeneity. Notably, subgroup analysis based on the definition of disease activity yielded inconsistent results. When Systemic Lupus Erythematosus Disease Activity Index 2000 (SLEDAI-2K)>4 was defined as active disease, no correlation between serum IL-6 level and SLE activity was identified (Table 3). In contrast, the correlation of serum IL-6 level with SLE activity was significant when active disease was defined as Systemic Lupus Erythematosus Disease Activity Index (SLEDAI)>4 (Table 3). Moreover, we found that there was no statistically significant heterogeneity in the subgroup with SLEDAI>4 (Table 3). These results indicated that the definition of disease activity might be a source of heterogeneity for the correlation between serum IL-6 level and SLE activity.

Sensitivity analysis was performed by sequentially deleting a single study to explore the source of heterogeneity. As shown in Figure 5, the overall pooled SMDs were not significantly altered. Egger's tests and Begg's tests were conducted to evaluate publication bias. As illustrated in Figure 6A, the funnel plot from Begg's tests was asymmetric. Moreover, the p values of Egger's tests (p=0.001) and Begg's tests (p=0.005) were less than 0.05. These results suggested that there was significant publication bias. Subsequently, we utilized the trim-and-fill method to examine whether publication bias substantially affected the robustness of the pooled SMD. The results showed that the adjusted funnel plot became symmetric (Figure 6B). Meanwhile, the pooled SMD (SMD: 2.15, 95% CI: 1.23-3.07) obtained after trim-and-fill adjustment still showed that the serum IL-6 level was higher in SLE patients than in healthy controls, suggesting that publication bias did not substantially affect the robustness of the pooled SMD. For the pooled Fisher's z value assessing the correlation between serum IL-6 level and SLE activity, Egger's tests (p=0.056) showed no significant publication bias, but Begg's tests (p=0.02) indicated that significant publication bias existed. Additionally, the funnel plot in Begg's test was also asymmetric (Figure 6C), further confirming that there was significant publication bias. Next, we applied the trim-and-fill method to determine whether the robustness of the pooled Fisher's z value was influenced by publication bias. As shown in Figure 6D, the adjusted funnel plot became symmetric, indicating that publication bias did not significantly affect the robustness of the pooled Fisher's z value. Consistently, the pooled Fisher's z value (0.360, 95% CI: 0.264-0.456, p<0.01) after trim-and-fill adjustment still suggested that there was a positive correlation between serum IL-6 level and SLE activity.

Figure 5..

Sensitivity analysis for the pooled results of differences between the serum IL-6 levels in SLE patients and healthy controls (A); Sensitivity analysis for the pooled results of the differences between the serum IL-6 level in active SLE patients and inactive SLE patients (B); Sensitivity analysis for the pooled results of the correlation between the serum IL-6 level and SLE activity (C).

(0.14MB).

Figure 6..

Funnel plot of the pooled results of differences between serum IL-6 levels in SLE patients and healthy controls (A); The adjusted funnel plot of the pooled results of differences between serum IL-6 levels in SLE patients and healthy controls (B); Funnel plot of the pooled results of the correlation between the serum IL-6 level and SLE activity (C); The adjusted funnel plot of the pooled results of the correlation between the serum IL-6 level and SLE activity (D).

(0.07MB).