2. Materials and methods2.1. Bacter

2. Materials and methods
2.1. Bacterial cultures
In this study, Bacillus licheniformis NBRC 12195 (from now abbreviated as B. licheniformis) and Lactobacillus paracasei subsp.paracasei NBRC 15889 (from now abbreviated as L. paracasei) were used to represent Bacillus species which are one of the most detected spoilage bacteria in raw milk (White, 2001) and lactic acid bacteria which are commonly present in dairy products (Mayra-Makinen & Bigret, 2004), respectively. These strains were obtained from the collection of National Institute of Technology and Evaluation, Biological Resource Center (NBRC), Japan. B. licheniformis was aerobically grown in nutrition agar (NA) medium (polypepton, 10.0 g; yeast extract, 2.0 g; MgSO4.7H2O,
1.0 g; agar, 15.0 g; distilled water, 1000 ml; pH 7.0). L. paracasei was anaerobically grown in de Man, Rogosa and Sharp medium (MRS agar or broth, Merck, Germany). These bacteria were incubated at 30
C for 48 h in correspondent growth agar plates. Anaerobic conditions were created in a parafilm-sealed plastic box using oxygen-absorbing and carbon dioxide-generating agents (Anaero-Pack-MicroAero, Mitsubishi Gas Chemical Co., Inc). Cells were harvested by spreaders and then suspended in correspondent growth media. After being reincubated at 30
C for 48 h, they were
removed from growth suspensions and washed twice with water.The cells were pelleted by centrifugation (3000 rpm, 10 min, and 4
C). Obtained bacteria were resuspended in sterile distilled water at an initial concentration of about 108e109 colony forming unit per milliliter (CFU/ml). Thiswas done by adjusting the optical density of the suspension to a previously calculated absorbance at 600 nm.