CXCL9, a promising biomarker in the diagnosis of chronic Q fever

Four groups were included: healthy controls, patients with acute Q fever, patients with a history of cured acute Q fever (past Q fever), and patients with chronic Q fever (Fig. 1). Healthy controls (n = 28) were hospital personnel and students without a history of Q fever. Healthy controls with available serum samples (n = 9) were Q fever seronegative. Specimens of anonymous acute Q fever patients (n = 9), all PCR-positive for C. burnetii at the time of blood-drawing, were collected from left-over samples of patients identified between 2008 and 2009 in the Canisius Wilhelmina (CWZ) Hospital. Left-over serum specimens of past Q fever patients (n = 20), were also derived from the CWZ-hospital. Another 10 individuals with past Q fever, who provided heparin-anticoagulated blood, were recruited in the Q fever prevaccination screening program, described in detail by Schoffelen et al. [9]. All samples were Coxiella burnetii phase II IgG positive and had low phase I IgG titers, indicative for the absence of chronic Q fever. Chronic Q fever patients (n = 65) visited the outpatient clinic of the Radboud university medical center (n = 29) or the other participating hospitals: Catharina Hospital Eindhoven (n = 12), Elisabeth Hospital Tilburg (n = 9), CWZ-Hospital (n = 6), Elkerliek Hospital Helmond (n = 5) and Bernhoven Hospital Uden (n = 4). The chronic Q fever group comprised 47 proven and 18 probable chronic Q fever patients diagnosed according to the Dutch consensus guideline on chronic Q fever [4]. Thirty-seven patients presented with a vascular focus in an aneurysm or aortic prosthesis, 19 had valvular defects, 6 had both a vascular and valvular localization, and 3 patients were immunocomprised. All patients were on antibiotic treatment.

EDTA-anticoagulated blood for isolation of peripheral blood mononuclear cells (PBMCs) was collected from chronic Q fever patients and healthy controls. Heparin-anticoagulated blood for stimulation experiments was drawn from healthy controls, past Q fever and chronic Q fever patients.

PBMCs were isolated from blood centrifuged with Ficoll-Paque (GE Healthcare, Uppsala, Sweden) according to standardized procedures [10]. Cells were taken from the interphase layer, washed twice in Phosphate Buffered Saline, and counted in a Coulter Counter Z (Beckman Coulter, Fullerton, CA, USA). PBMCs were then incubated in flat-bottom 24-wells plates in 1 mL (10⁷cells/mL) and stimulated with heat-killed C. burnetii Nine Mile (NM) RSA493 phase I (kindly provided by dr HJ Roest, CVI, Lelystad) in 10⁷/mL at 37 °C for 8 h. RNA was extracted with the RNeasy Mini kit (Qiagen, Hilden, Germany). With the 2100 Bioanalyzer (Agilent Technologies, Massy, France) and the RNA 6000 Nano LabChip kit, the quality of the RNA was ensured. RNA quantity was determined with the Nanodrop (Thermo Scientific). Gene expression was analysed using Whole Human Genome 4x44K microarrays (Agilent Technologies, Massy, France) and One-color Microarray based Gene Expression Analysis kit, as previously described [11]. Gene expression data was analysed with R and Bioconductor software suite. Data was normalized with quantile normalization after being preprocessed and quality checked (Agi4x44PreProcess library). With the Limma library, differential gene expression was assessed. Data was compliant with the Minimun Information About a Microarray Experiment (MIAME) guidelines, accessible with number GSE66476 at the National Center for Biotechnology Information’s Gene Expression Omnibus, (www.​ncbi.​nlm.​nih.​gov/​geo/​).

Blood was drawn into 5 mL heparinized tubes. Subsequently 500 μL blood was incubated with either heat-killed C. burnetii NM in an end concentration of 10⁷/mL or with culture medium (negative control) [12]. After 24 h of incubation at 37 °C and 5% CO₂, the supernatants were harvested and stored at -80 °C.

Interferon-γ (IFN-γ) production in stimulated whole blood supernatants was measured with commercially available enzyme-linked immunosorbent assay (ELISA) (Sanquin, Amsterdam, Netherlands) according to the manufacturer’s instructions. The CXCR3-chemokines and CCL8 were determined in stimulated whole blood supernatants and serum using Luminex technology (Bio-Rad, CA, USA). CRP from serum was measured with immunoturbidimetry (Architect, Siemens; and Cobas 6000, Roche) and anti-C. burnetii antibodies were determined in serum by indirect immunofluorescence measuring IgM and IgG against C. burnetii NM phase I and II a commercially available immunofluorescence assay (IFA, Focus Diagnostics Inc., Cypress, CA, USA).

Transcriptional profiles of PBMCs of 4 healthy controls were compared to the PBMCs of 6 chronic Q fever patients that were in-vitro stimulated with heat-killed C. burnetii. To look for candidate biomarkers, genes were selected that were most differentially expressed in both groups. Four genes encoding for chemokines ended at the top of the list: CXCL9 also named Monokine Induced by IFN-γ (MIG), CXCL10 (IFN-γ Inducible Protein-10 (IP-10)), CXCL11 (IFN-γ T-cell Attractant Chemokine (I-TAC)), and CCL8 (Monocyte Chemotactic Protein (MCP-2)) (Table 1). CXCL9, CXCL10 and CXCL11 are ligands for CXCR3 and are therefore named CXCR3-chemokines.

To validate the results from the gene expression analysis and to assess the suitability of measurement of the gene-products, the production of these proteins in C. burnetii stimulated whole blood was determined (Fig. 2). These experiments were performed with blood from 15 healthy volunteers, 20 past Q fever and 36 chronic Q fever patients, who were diagnosed (median) 20 months before blood sampling.

Healthy controls showed significant C. burnetii-induced production of CXCL9, CXCL10 and CCL8, but no production of CXCL11. The same pattern was seen in past Q fever individuals. Chronic Q fever patients showed increased production of all four chemokines (CXCL9, CXCL10, CXCL11 and CCL8). CXCL9 production was significantly higher in chronic Q fever patients (median 15.1 ng/mL, IQR 8.5–26.5) than in healthy controls (median 3.6 ng/mL, IQR 1.7–8.2, p < 0.05) and past Q fever patients (median 3.8 ng/mL, IQR 2.8–5.3, p < 0.05). CXCL11 production in chronic Q fever patients (median 146 pg/mL, IQR 83–230) was higher than in past Q fever patients (median 66 pg/mL, IQR 43–183, p < 0.05).

A Receiver-operator-curve (ROC) analysis was performed for CXCL9 and CXCL11 to distinguish between chronic Q fever patients and past Q fever patients. The test accuracy, denoted by the area under the curve (AUC), was 85% (CI: 75–95%) for CXCL9 and 78% (CI: 66–90%) for CXCL11.

Further analysis of the CXCL11 production in chronic Q fever patients showed that production in samples taken within 3 months after diagnosis (n = 5) was significantly higher than in samples taken later in the course of the disease (n = 20, p < 0.05), but not for the other chemokines.

Because the identified chemokines are all induced by IFN-γ, their correlation with C. burnetii-specific IFN-γ production in the whole blood culture supernatants was assessed. Generally, correlation was moderate (Additional file 1: Fig. S1). The correlation coefficient (Spearman) was 0.54 for CXCL9 (p < 0.001), 0.70 for CXCL10 (p < 0.001), 0.50 for CXCL11 (p < 0.001) and 0.53 for CCL8 (p < 0.001).

We measured circulating chemokines in serum of 9 healthy controls, 10 past Q fever individuals, 9 acute Q fever and 51 chronic Q fever patients. Chronic Q fever patients were treated for a median of 13 months (range 0–46).

Chronic Q fever patients exhibited significantly higher serum concentrations of CXCL9 (median 899 pg/mL, range 92–12,734), CXCL10 (median 311 pg/mL, range 16–1497) and CXCL11 (median 21 pg/mL, 4–106) compared to healthy controls (CXCL9 230 pg/mL, 164–557, p < 0.001, CXCL10 151 pg/mL, 73–264, p < 0.05, CXCL11 10 pg/mL, 5–15, p < 0.01, Fig. 3). Chronic Q fever patients showed higher CXCL9 serum concentrations than past Q fever individuals (median 537 pg/mL, 82–927). Chronic Q fever patients did not have higher levels of CXCL10 or CXCL11 than past Q fever individuals (median 204 pg/mL,10–464 and median 18 pg/mL, 6–72). Concentrations of CCL8 were low in all groups and did not differ between groups. As compared to chronic Q fever patients, acute Q fever patients had higher CXCL10 serum concentrations (median 1204 pg/mL, 180–1439, p < 0.01). The other chemokines did not differ between chronic Q fever and acute Q fever patients.

ROC analysis of the CXCL9 serum concentrations of chronic Q fever compared to past Q fever individuals resulted in a test accuracy of 79% (denoted by the AUC, CI 67–92%, Fig. 3e). The sensitivity was 73% and specificity 80%, when a cut-off (580 pg/mL) was chosen that yielded both a high sensitivity and specificity.

Clinical parameters of the patients at diagnosis, such as PCR positivity in blood or tissue, and anti C. burnetii phase I IgG titers were compared to the performance of CXCL9 serum concentration at the 580 pg/mL cut-off value (Table 2 and a detailed description in Additional file 2: Table S1).

Further analysis of the CXCR3-chemokine serum concentrations revealed that samples taken within one month after diagnosis of chronic Q fever (n = 9) were significantly higher for CXCL9 (p < 0.05) and CXCL10 (p < 0.05) than samples taken more than 1 month after diagnosis (n = 41).

As circulating CXCR3-ligands were high in chronic Q fever patients, we investigated whether they would decrease during the course of treatment and could be used as marker for monitoring the effect of treatment. To this end, we analysed serum samples taken at regular intervals of 28 chronic Q fever patients during their visits to the outpatient clinic. In total, 137 serum samples were available (median 5 samples per patient (range 2–7), between 0 to 62 months after start of treatment). In a nonlinear best fit regression model, the slopes of the regression lines per patient were calculated and the median slope was generated for CXCL9 (−5.0, range − 1959 to 23), CXCL10 (−0.8, range − 125,550 to 22), CXCL11 (−0.2, −14 to 1.6) and CCL8 (−0, −19 to 35) indicating that there was no relation between chemokine levels and treatment duration per patient (Fig. 4). Similar results were obtained when time after last positive PCR in blood was taken into account.

In 135 serum samples from 40 chronic Q fever patients the corresponding anti-C. burnetii IgG phase I titers were known. There was a weak correlation between IgG phase I titers and CXCL9 (Spearman r = 0.24, p < 0.01) but no correlation with the other chemokines.

The acute phase protein C-reactive protein is elevated in various inflammatory conditions including Q fever and is determined during treatment to monitor disease activity. Seventy-six CRP values were available from 27 patients. Fifty-eight samples were below the detection limit of the test (5 mg/L), whereas only 5 CRP values were above 50 mg/L. We assessed the correlation of the CRP values to the concurrent chemokine serum concentrations and found a weak correlation with CXCL9 (r = 0.25, p < 0.05) and CXCL11 (r = 0.47, p < 0.001), but not with the other chemokines.