No concomitant medications (prescription, over-the-counter, or herbal) were permitted to be administered during the study, unless they were prescribed by the investigator for treatment of specific clinical events or were approved by the medical monitor prior to dosing. The study was approved by the Institutional Review Boards of all study centers and conducted in accordance with Good Clinical Practice, as defined by the International Conference on Harmonization, in accordance Autophagy activator with the ethical principles underlying European Union Directive 2001/20/EC and the United States Code of Federal Regulations, Title 21, Part 50 (21CFR50), and in
accordance with the ethical principles that have their origin in the Declaration of Helsinki. Informed written consent was obtained from all patients. Patients were randomly assigned to receive BMS-790052 or placebo according to a computer-generated randomization scheme prepared by Bristol-Myers Squibb. An Interactive Voice Response System was used to assign a unique subject number and a blinded container number, which was provided to the blinded study staff who supervised and recorded the drug administration. The sample size was based on the primary endpoint of the study, defined as the change in log10 HCV RNA from baseline to Cell Cycle inhibitor day 7.
A mean decrease of at least 1.5 log10 HCV RNA within one dose panel would suggest that BMS-790052 was sufficiently active to proceed to late phase development. If BMS-790052 had no effect, administration of drug to four patients within a dose panel would yield a probability of 0.01 to observe a mean decrease in log10 HCV RNA of more than 1.5. If the true mean decrease was 2.0, the probability of observing a mean decrease in log10 HCV RNA of more than 1.5 would be 0.78. These calculations are based on the assumption
that log10 HCV RNA is normally distributed, with a standard deviation for the change of 1.3. Eligible patients for this study were men and women, ages 18-60 years inclusive, with a body mass index of 18-35 kg/m2, who were chronically infected (longer than 6 months) with HCV genotype 1, and who were treatment-naive selleckchem to interferon and RBV. Additional inclusion criteria were: plasma HCV RNA ≥100,000 IU/mL; documented FibroTest score of ≤0.72 and APRI ≤2, or the absence of cirrhosis based on liver biopsy within 12 months; women of childbearing potential were not to be nursing or pregnant and had to be willing to agree to use double barrier contraception for at least 1 month before dosing, during dosing, and at least 12 weeks after the last dose of study medication. The main exclusion criteria were: patients with prior documented cirrhosis on liver biopsy; previous exposure to a NS5A replication cofactor inhibitor; coinfection with human immunodeficiency virus; coinfection with hepatitis B virus.