For additional information, see Supplementary material. This was a four-armed, randomized, double-blind, placebo-controlled, single-center Phase I trial. The study was approved by the Ethical Review Board in the Gothenburg Region, the Western Institutional Review Board, USA and the Swedish Medical Product Agency. Healthy adult subjects, 18 to 43 years, were randomized into one of four groups (A–D); each group was given two oral doses two weeks apart of one of the following treatments: (A) vaccine buffer alone (n = 34), (B)

MEV alone (n = 35), (C) MEV plus 10 μg dmLT (n = 30) or (D) MEV plus 25 μg dmLT (n = 30). A computer-generated randomization list was prepared by a statistician otherwise not involved in the study. MEV (also called Etvax) consists of four inactivated recombinant E. coli

strains (ETEX 21–24) which overexpress CFA/I, CS3, CS5 and CS6, respectively, Enzalutamide mixed with LCTBA [9]. The CFA/I, CS3 and CS5 expressing strains, all based on a toxin-negative O78 ETEC strain, were inactivated with formalin and the CS6 expressing E. coli K12 strain with phenol to retain CF expression on the bacterial surface [10] and [13]. click here LCTBA is a recombinantly produced LTB/CTB hybrid protein in which seven amino acids in CTB have been replaced by corresponding amino acids of LTB [12]. dmLT (R192G/L211A) is an LT-derived protein which contains two genetic substitutions in the A subunit which eliminates the enterotoxic activity without removing the

adjuvant activity [14]. Volunteers received two oral doses of vaccine ± dmLT in bicarbonate buffer or placebo (buffer alone) two weeks apart (day 0 and day 14 ± 2). Fecal samples were collected on days 0, 7 ± 1, 14 ± 2, 19 ± 1, 21 ± 1 and 28 ± 2, blood too samples for isolation of inhibitors peripheral blood mononuclear cells (PBMCs) on days 0, 7 ± 1, 19 and 21 ± 1 and serum samples on days 0, 7 ± 1, 14 ± 2, 19 ± 1, 21 ± 1, 28 ± 2 and 40–56. Safety was determined by evaluation of adverse event (AE) reports (diary cards and interviews) from day 0 until day 40–56, by clinical chemistry and hematology tests performed at screening and on days 7 ± 1 and 21 ± 1 and by physical examination at screening and on day 40–56. Solicited AEs listed in the study diaries were gastrointestinal symptoms (i.e. abdominal pain, nausea, vomiting, diarrhea, loose stools) plus fever. Mucosal immune responses were evaluated by measuring intestine-derived antibody secreting cells (ASCs) and intestinal secretory IgA (SIgA) responses in fecal extracts. Systemic immune responses were analyzed by measuring serum antibody levels. PBMCs were isolated and used for ASC analyses by the antibodies in lymphocyte supernatants (ALS) and ELISPOT assays as described [11]. ASCs were detected by the ELISPOT technique using plates coated with in-house purified CFA/I, CS3, CS5 or GM1 ganglioside plus LTB or CS6 (Gift from F.