MATERIALS AND METHODS Birds and Exp

MATERIALS AND METHODS Birds and Experimental Treatments Five hundred twenty-five 1-d-old male Cobb broilers were obtained from a local commercial hatchery. Broilers were vaccinated on d 1 for Marek, infectious bronchitis, and Newcastle disease and were randomly allocated in 5 experimental treatments for 6 wk. Each
treatment had 105 broilers arranged in 3 replicates of 35 broilers each. Each replicate was assigned to a clean floor pen (2 m2) and birds were raised on a wheat straw shavings litter. Heat was provided with a heating lamp per pen. The temperature was regulated at 27 ± 1°C during the starter phase and at 25 ± 1°C for the rest of the experiment (15 to 42 d). Except from d 1, a 23L:1D lighting program was applied during the experiment. Overall, housing and care of the birds conformed to Faculty of Animal Science and Aquaculture guidelines. The experimental treatments received a corn-SBM basal diet (BD) and depending on the addition were labeled as follows: BD-no other addition (C), BD containing a probiotic concentration of 108 cfu/kg of diet (P1), BD containing a probiotic concentration of 109 cfu/kg of diet (P2), BD containing a probiotic concentration of 1010 cfu/kg of diet (P3), and BD containing avilamycin (MAXUS 100, Elanco Hellas, Agia Paraskevi, Greece) at 2.5 mg/kg of diet (A). The BD was in mash form and was formulated for starter (1 to 14 d), grower (15 to 28 d), and finisher (29 to 42 d) broiler growth periods and its composition is shown in Table 1. There was no coccidiostat added in the BD. The BD was prepared every 2 wk and stored in sacks in a cool place. Experimental diets and water were available ad libitum. The probiotic used (PoultryStar ME, Biomin GmbH, Herzogenburg Austria) was a 5-bacterial species product that comprised probiotic bacteria isolated from the crop (Lactobacillus reuteri DSM 16350), jejunum (Enterococcus faecium DSM 16211), ileum (Bifidobacterium animalis DSM 16284), and ceca (Pediococcus acidilactici DSM 16210 and Lactobacillus salivarius DSM 16351) of healthy adult chickens. For each one of the probioticcontaining experimental treatments P1, P2, and P3, the probiotic product was especially formulated so that upon its addition at 1 g/kg of diet, it would give the desirable probiotic concentration in the diet expressed as colony-forming units per kilogram of diet. The probiotic product was added in the BD on a weekly basis. Two feed samples, one upon mixing and the second at the end of each week, were subjected to microbiological analysis to check mixing and product viability in feed.
Broiler Performance Responses Growth performance parameters such as BW, BW gain, feed intake (FI), and feed conversion ratio (FCR), defined as FI:weight gain (g:g), were determined every 2 wk. Overall BW gain, FI, and FCR were calculated for the whole duration of the experiment.
Bacterial Enumeration in Probiotic Product and Feed Probiotic product and feed samples were cultured according to Mountzouris et al. (2007) for the enumeration of total anaerobes, lactic acid bacteria, Lactobacillus spp., Bifidobacterium spp., and gram-positive cocci