Method

We conducted a single-center prospective study from May 2017 to January 2018 at the GZA Hospitals, a secondary care hospital (1012 beds) in Antwerp, Belgium. IPTS from patients undergoing revision arthroplasty were consecutively processed. Each IPTS was aseptically divided in two equal parts: one was processed by direct inoculation on agar and in broths (non-homogenized method); the other was transferred in a sterile vial with saline solution and glass beads (EOLabs), homogenized using a mechanic cell disruptor for 30s (Disruptor genie, Scientific Industries), 2mL of the suspension was inoculated in (an)aerobic BCBs, agar plates and broths (homogenized method). Agar plates were incubated for 4d; broths and BCBs in BacT/Alert (bioMerieux) for 14d. Micro-organisms were identified using MALDI-TOF MS (Bruker). Sensitivity (Se) and specificity (Sp) were calculated against the IDSA definition of PJI for different culture sets: non-homogenized and agar/broth; homogenized processing and agar/broth, agar/broth/BCB, agar/BCB. Ethics committee approved the study.