5; Roche Molecular Systems, Branchburg, New Jersey, USA). Patients needed to have HIV RNA < 50 copies/mL at screening, but could then have HIV RNA > 50 copies/mL at the baseline visit. HCV coinfection was classified based on antibody testing at a central laboratory. Data on HCV viral load were not collected systematically. For samples with HIV RNA < 50 copies/mL, the Roche Amplicor assay produces two different results. Either traces of HIV RNA can be detected, which are below the 50 copies/mL limit, or no HIV
RNA is detected (the optical density for the sample is the same as for the negative control). Any patient with an HIV RNA result > 50 copies/mL attended a confirmation visit, for repeated selleck screening library testing of HIV RNA, drug resistance and
plasma drug levels. If a patient had two consecutive HIV RNA levels > 50 copies/mL, investigators could intensify or change antiretrovirals. Viral Selleck Roxadustat genotypic tests were performed using Virco TYPE HIV-1 assays (Virco BVBA, Beerse, Belgium). The number of patients with treatment-emergent primary International AIDS Society (IAS)-USA PI mutations [16] was analysed by treatment arm. Mean adherence to randomized medication was assessed using the Modified Medication Adherence Self-Report Inventory (M-MASRI) questionnaire, which was completed by patients at each study visit. Adverse events were recorded by the trial investigators at each study visit, and classified using the Division of AIDS 2004 system [17]. Written informed consent was obtained from all participating patients Baricitinib before the study started. Study protocols were reviewed and approved by the appropriate institutional ethics committees and health authorities, and were undertaken in accordance with good clinical practice, and the Declaration of Helsinki. The funding for the trial was from Janssen (Beerse, Belgium). TheClinicaltrials.gov identifier is NCT00458302. The MONET trial was designed to show noninferior efficacy of the monotherapy arm vs. the triple therapy arm at week 48, with a noninferiority margin of −12% [18]. The sample size calculations assumed 80% power, a one-sided significance level of 0.025, a 90% overall response rate
and 10% of patients excluded from the per protocol population. The primary analysis used the TLOVR algorithm [19]: virological failure was defined as two consecutive HIV RNA levels > 50 copies/mL at any time in the trial, even if the HIV RNA level was then resuppressed < 50 copies/mL at subsequent visits; discontinuation of randomized treatment was also classified as treatment failure in this analysis (the ‘switch equals failure’ approach) [20]. In addition we used a strict ITT (switches not considered failures) analysis, for which all patients who had HIV RNA levels < 50 copies/mL at week 144 were counted as successes, even if they had temporary HIV RNA elevations during the trial and/or had changed their randomized treatment. This was a pre-planned analysis.