Chemokine (C–C motif) receptor 2 is associated with the pathological grade and inflammatory response in IgAN children

Rabbit anti-CCR2 antibody was obtained from BioVision (Milpitas, CA). Rabbit anti-MCP-1, rabbit anti-IL-17, mouse anti-IL-6 and rabbit anti-TNF-α antibodies and were obtained from AbCam (Cambridge, MA). Pre-immune rabbit serum, secondary antibodies (PV-9000 kit) and DAB Detection Kit were purchased from Zsbio (Beijing, CHN). FITC-labeled anti-human IgA was purchased from Zsbio (Beijing, CHN). Other chemicals and reagents were purchased from Zsbio (Beijing, CHN).

Fifteen children with a diagnosis of IgAN presenting to the Department of Pediatrics, First Affiliated Hospital of Anhui Medical University, were enrolled between July 2014 to September 2017. All children were diagnosed with primary IgAN by kidney biopsy [20]. The procedure for the kidney biopsy was performed as previously described with some modifications [21], and the pathological staining was shown in the supplementary materials (sFigure 1 and sFigure 2). All patients did not receive the treatment with steroid or other immunosuppressant agents before kidney biopsy. All children were excluded from secondary IgAN caused by allergic purpura nephritis, lupus nephritis, or hepatitis B virus-related nephritis. Eight control kidney tissue specimens were taken from children with kidney surgery because of other kidney diseases, such as kidney duplication. Wax block specimens of kidney biopsy were used for subsequent immunohistochemical staining. Twelve control blood and urine specimens were taken from normal children with health checkup. Study protocol was approved by the hospital institutional review board of the First Affiliated Hospital of Anhui Medical University, and the number of the ethics approval was NO. 20140235. Kidney biopsy specimens from patients and control group had obtained the informed consent of the patient's family.

The wax block of kidney biopsy tissue and control kidney tissues were cut at 5 μm thickness sections. The procedure for immunohistochemistry has been previously described [22]. Briefly, the sections were treated with conventional dewaxing tissue sections to water, and sodium citrate buffer solution antigen repair, and 3% H₂O₂ to reduce the non-specific staining, and 5% BSA was added to block endogenous antigen. The slides were incubated with rabbit anti-CCR2 (dilution 1:200), or free-immune serum (1:50), rabbit anti-MCP1 (1:100), IL-17 (1:100), TNF-ɑ (1:100) and mouse anti-IL-6 (1:500) overnight at 4 °C. After rinsing in PBS, the sections were incubated with peroxidase-conjugated goat anti-rabbit or anti-mouse IgG at room temperature for 1 h. After PBS washing for three times, DAB color solution dropped onto the section, and incubated for 3–5 min. Then the section was stained with hematoxylin for 2 min. After drying and transparent, the section was observed under microscope. The analysis of specific staining was performed using Image J software (NIH, Bethesda, MD, USA). Negative controls were performed by replacing the primary antibody with free-immune serum, and the results was shown in the supplementary materials (sFigure 3). The relative optical density (OD) was counted at 200 × magnification, and the positive signaling were counted in twenty randomly selected sections using the software of Image J v1.8.0 (National Institutes of Health, Bethesda, MD).

The serum and urine samples were obtained by centrifugation, and 20ul was used to measure urine red blood cell count (URBC), 24-h urine protein (UPro), blood urea nitrogen (BUN), and serum creatinine (SCr) were measured on Abbot architect ci8200 analyser (Abbott, Abbot Park, IL, USA). Each sample was tested 3 times, and the average value was used for statistical analysis.

Fifteen IgAN children, including 10 males and 5 females (mean age 11.67 ± 1.76 years old, absolute range 7.4–13.2 years), were enrolled in the study. Eight control kidney tissue specimens were taken from children, including 5 males and 3 females (mean age 10.75 ± 2.24 years old, absolute range 6.3–14.5 years), with normal pathological examination after kidney disease. Twelve control blood and urine specimens were taken from normal children with health checkup.

All children with IgAN had gross hematuria or microscopic hematuria, and the urinary red blood cell count was 689 ± 427 cells per μl, which was significantly higher than control group (P < 0.05). Twelve control blood and urine specimens taken from normal children, including 8 males and 7 females (mean age 11.64 ± 3.17 years old, absolute range 6.8–15.6 years), were detected for UPro, URBC, SCr and BUN. Compared with the control group, UPro and URBC of the children were significantly increased in IgAN children (P < 0.01), and no significant difference were found in serum BUN and SCr (P > 0.05), as shown in sTable 1. Blood test and liver function tests were normal in IgAN children (P > 0.05), and the data were not shown.

As shown in the Figs. 1A and 2A, CCR2 was rarely observed in the kidney tissues of normal control group. However, CCR2 expression increased significantly in IgAN children (Figs. 1A and 2A). CCR2 positive signals were concentrated in the glomeruli, while in the renal tubular were rare (Figs. 1A, B and 2A). Most of the CCR2 positive signals were expressed in the glomerular mesangial cells of IgAN children, whereas in the vascular endothelial cells were rare (Figs. 1A and B). As shown in Fig. 1C, compared with normal control group, the relative optical density (OD) of CCR2 positive signals calculated by the software (Image J) had significantly increased in IgAN children (P < 0.001).

According to Lee's classification of IgAN [6, 20], the renal pathology of 15 children was classified, including 1 case of grade I, 6 cases of grade II, 7 cases of grade III, and 1 case of grade IV. We had divided 15 patients into 2 groups, low grade group (Lee’s grade I to II) (n = 7), and high grade group (Lee’s grade III to IV) (n = 8). In IgAN children of high grade group, CCR2 positive signals were significantly higher than that of low grade group (Fig. 2A). Quantitative analysis of optical density (OD) also confirmed the above results (P < 0.001) (Fig. 2B). Interestingly, we found that the relative OD value of CCR2 had a significant positive correlation with the pathological grade of Lee’s classification in IgAN children (r = 0.9152, P = 0.0001) (Fig. 2C). However, in 15 cases of children, we did not find any correlations between Lee’s grade and IgA deposition (r = 0.2322, P = 0.4050), as shown in sFigure 2B. Furthermore, there was no correlation between IgA deposition and the relative optical density (OD) of CCR2 expression analyzed by DAB staining in IgAN children (r = 0.2783, P = 0.3152) (sFigure 2C).

Moreover, the expression levels of inflammatory factors were detected by immunohistochemistry, including MCP-1, IL-17, IL-6 and TNF-α (Fig. 3). As shown in Fig. 3A, MCP-1 expression was mainly concentrated in the renal tubules, especially in the epithelial cells of collecting duct, while IL-17 (Fig. 3B), IL-6 (Fig. 3C) and TNF-α (Fig. 3D) were mainly concentrated in the glomerulus and collecting duct. Compared with the normal control group, MCP-1, IL-17, IL-6 and TNF-α increased significantly in the kidney tissue of IgAN children (P < 0.05) (Fig. 3A-D), and the similar results were found in the relative optical density (OD) of MCP-1, IL-17, IL-6 and TNF-α (Fig. 3A-D).

As shown in Fig. 4, the expression levels of inflammatory factors in high grade group (Lee’s grade III to IV) were significantly higher than that of low grade group (Lee’s grade I to II) (P < 0.05). Furtherly, the relationships between CCR2 expression and the expression levels of inflammatory factors were also studied. We found that CCR2 expression had a significant positive correlation with the expression levels of MCP-1 (r = 0.8929, P = 0.0001), IL-17 (r = 0.6607, P = 0.0073), IL-6 (r = 0.7167, P = 0.0026) and TNF-α (r = 0.8022, P = 0.0003) in IgAN children (Fig. 5).