Measurement of C-reactive protein, procalcitonin and neutrophil elastase in saliva of COPD patients and healthy controls: correlation to self-reported wellbeing parameters

From January 2010 to March 2012, individuals were recruited consecutively from our research and outpatient clinic databases to one of 3 cohorts: life-long never-smokers (NS group); current smokers (S group; with > 20 pack years); or COPD, confirmed by spirometry according to GOLD criteria [45]. Patients with other respiratory disorders were excluded. All NS and S subjects had normal lung function. Participants were monitored over 14 days (3 visits, one week apart). At visit 1, demographic details were recorded (Table 1) (Additional file 1: Table S1); participants with any infection or unstable illness in the preceding 6 weeks were excluded. On each visit, the Medical Research Council (MRC) dyspnoea score was recorded [46], spirometry (Koko Legend, nSpire, USA) performed and unstimulated whole saliva collected (2 ml). Participants completed a daily self-assessment diary (Additional file 2) [47], incorporating scores on breathing, activities of daily living (ADL), sputum features and cough presence. In-between scheduled visits, patients were asked to contact the researchers on developing any change in symptoms. An exacerbation was defined as an increase in respiratory symptoms for two consecutive days, with at least two major symptoms (dyspnoea, sputum purulence, sputum volume) or a major plus a minor symptom (wheeze, cold, sore throat, cough) [48]. Randomly-selected subjects provided simultaneous saliva and blood samples. The study was approved by the local research ethics committee [REC project reference: 09/H1203/77]; all participants gave informed written consent.

Participants were asked to abstain from alcohol for at least 12 h; fast for 2 h; refrain from brushing their teeth and smoking for 30 min, prior to providing saliva samples. Oral hygiene was checked and mucosal examination performed at each visit. All visit samples were collected at same time of day for each subject.

Immediately before collection participants rinsed their mouths with 10mls water; they then sat in an upright position, tilted their heads forward, and allowed saliva to pool in the mouth before passively drooling into an ice-cooled marked sterile tube (Nunc, Denmark) up-to a total of 2mls.

Collected saliva samples were transported on ice and stored at − 80 °C until analysis. Prior to analysis, thawed saliva was centrifuged at 3000 revolutions per minute (RPM) for 15 min. Sample measurements were undertaken within 3 months of storage; all biomarker assays were performed in duplicate. All saliva samples were tested for blood contamination using an 8-parameter urine dip test strip (Bayer AG, USA). Briefly, 10ul of saliva was aliquoted onto the reagent square for blood, with the colour change after 5 s being read on the key and documented.

CRP was measured in 15ul of saliva using a salivary ELISA kit (Salimetrics Europe, UK) with a detection limit of 0.90 ng/ml; lower concentrations were assigned as 0.89 ng/ml.

Levels of PCT and NE in saliva were measured following in-house modification of commercially-available ELISAs [49].

Briefly, for adapting the VIDAS® BRAHMS PCT (bioMérieux, France) for use in saliva, pre-study experiments involved spiking saliva from non-smoker healthy subjects with PCT Control (provided by the manufacturer for assay calibration) in varying concentrations: 0.09–20 ng/ml. These spiked samples were analysed neat and in varying defined dilutions: 1:1, 1:2, 1:4, 1:8 using Phosphate Buffered Saline - Tween 20–0.05 % (PBS-T). Optimal recovery of PCT (85 %) at all concentrations occurred when saliva was diluted 1:2 in PBS-T. The manufacture’s test procedure for performing the assay was not altered. Thereafter, PCT was determined in 100ul of saliva diluted 1:2 in Phosphate Buffered Saline-Tween 20 − 0.05 % (PBS-T) using VIDAS® BRAHMS PCT (bioMérieux, France) with a detection limit of 0.10 ng/ml; lower concentrations were assigned as 0.09 ng/ml.

For adapting the PMN-Elastase ELISA Kit (Immundiagnostik AG, Germany) for use in saliva, we first spiked non-smoker healthy saliva with NE (provided by the manufacturer to calibrate the assay) in varying concentrations: 115–1000 ng/ml. These spiked samples were analysed in varying dilutions: 1:100, 1:200, 1:400, 1:800 using manufacturer-supplied ELISA wash buffer. Recovery of NE (90 %) was consistent across all 4 dilutions; for the study we elected to use a 1:200 dilution. The manufacture's test procedure for performing the assay was not altered. Thus, NE was measured in 7.0 ul of saliva diluted 1:200 in ELISA wash buffer using PMN-Elastase ELISA Kit (Immundiagnostik AG, Germany), with a detection limit of 70 ng/ml; lower concentrations were assigned as 69 ng/ml.

Peripheral blood was collected in supplement-free tubes and ethylene diaminetetra-acid vacutainer tubes (BD Bioscience, New Jersey, USA). Samples were then centrifuged at 2000 RPM for 15 min; retrieved serum was stored at 80 °C until analysis. Serum CRP was measured using ADVIA 2400 Chemistry System (Siemens AG, Germany) with detection limit of 0.3 mg/L. Serum PCT and NE were quantified using same assay kits as for saliva, but following manufacturers’ protocols. Serum levels were expressed as ng/ml except for CRP (mg/L). All assays were performed in duplicate.