Routine use of Staphylococcus aureus rapid diagnostic test in patients with suspected ventilator-associated pneumonia

The bronchial secretions were collected using a BAL or a mini-BAL. Qualitative and quantitative cultures were performed. A quantitative BAL or mini-BAL was defined as negative if there was less than 10⁴ colony-forming units (cfu)/mL and 10³ cfu/mL of growth from the culture [11, 12].

All respiratory tract samples were divided into two aliquots. A first aliquot was inoculated on Columbia 5% sheep-blood, chocolate PolyViteX and MacConkey agar media (bioMérieux, Marcy l'Etoile, France). Incubation was performed at 36°C under 5% CO₂ atmosphere for Columbia 5% sheep-blood and chocolate PolyViteX. Growing microorganisms were identified by using matrix-assisted laser desorption ionization time-of-flight [13]. Methicillin resistance was determined for Staphylococcus aureus by using a disk-diffusion method (Mast Diagnostics, Amiens, France) after 18 to 24 hours of incubation on Mueller-Hinton agar media (bioMerieux) according with the European Committee on Antimicrobial Susceptibility Testing (EUCAST) breakpoints.

Staphylococcus aureus was identified using a rapid diagnostic test on a platform Cepheid Xpert real time PCR assay (Cepheid, Sunnyvale, CA, USA). In the Marseille study center, an Xpert SA Nasal Complete Kit was used. In the Lyon study center, an Xpert MRSA/SA SSTI was used. The extraction, amplification and detection steps take place in different chambers of a self-contained, single-use cartridge containing all reagents required for the bacterial target detection. Samples were adsorbed onto a swab, which was inserted in the extraction buffer vial of the Xpert assay, transferred into the cartridge, and treated according to the manufacturer's instructions. Both the Xpert SA Nasal Complete and the Xpert MRSA/SA SSTI target the staphylococcal protein A (spa) gene, the gene for methicillin resistance (mecA) and the staphylococcal cassette chromosome (SCCmec) inserted into the S. aureus chromosomal attB insertion site, and an internal-control sample processing control (SPC) three genetic markers (Bacillus globigii).

The rPCR test was available 24 h a day and 7 days a week. In Marseille, a microbiologist was responsible for the procedure in a point-of-care laboratory. In Lyon, a clinical research assistant performed the rPCR test directly in the intensive care unit. The detection of a microorganism is accompanied by a positive signal. This detection is possible in 58 minutes.

We collected the simplified acute physiology score (SAPS 2) at admission, reason for admission and the duration of the ICU stay, day of occurrence of the episode of VAP, result of rPCR test, result of Gram stain and result of microbiological culture. The analysis was conducted in the entire cohort and then in the patients with risk factors for MRSA infection, as defined elsewhere [2].

The economic assessment conducted examined rPCR test kit testing as an adjunct for antibiotic management of VAP empirical treatment in 2013 Euros. Estimates of the cost of running a rapid detection test are approximately €45 per test. We considered two approaches to model antibiotic costs in the empirical treatment of VAP: 1) a less expensive option, such as what might be used for patients without renal failure (€50/day), and 2) a more expensive option, such as what might be used for patients with renal impairment (€150/day). The estimate of the duration of empirical antibiotics (three-days) is derived from our prior publications [14].