The physiological properties that d

The physiological properties that differentiated strain S16–07T from S. smyrnaeus SM3501T, S. abikoensis NBRC 13860T, S. thermocarboxydovorans NBRC 16324T and S. lilacinus ISP 5254T are shown in Table 2. Strain S16–07T utilized adonitol, D(−)rhamnose, raffinose and sucrose, whereas S. abikoensis NBRC 13860T, S. thermocarboxydovorans NBRC 16324T and S. lilacinus ISP 5254T did not. In addition, S16–07T could use L(+)arabinose, D(+)cellobiose, D(+)galactose, beta-lactose and D(−)mannitol, a property which was negative in S. abikoensis NBRC 13860T and S. lilacinus ISP 5254T. S. smyrnaeus SM3501T utilized D(−)sorbitol and xylitol as the sole carbon source but strain S16–07T could not. Strain S16–07T could utilize urea and degrade casein, whereas S. smyrnaeus SM3501T and S. abikoensis NBRC 13860T could not. Strain S16–07T could tolerate NaCl at concentration up to 10%, whereas S. smyrnaeus SM3501T could tolerate up to 20%. On the other hand, S. abikoensis NBRC 13860T, S. thermocarboxydovorans NBRC 16324T and S. lilacinus ISP 5254T could tolerate only 5% NaCl. Strain S16–07T utilized fructose, glycerol, myo-inositol, maltose, trehalose and xylose as the sole carbon source but not melibiose, D(−)sorbitol and sorbose. Alkaline phosphatase, leucine aminopeptidase, acid phosphatase, phosphoamidase, α-glucosidase and glucosaminidase were detected with the API ZYM enzyme assay, but not chymotrypsin, cystine aminopeptidase, esterase (C4), esterase lipase (C8), α-fucosidase, α-galactosidase, β-galactosidase, β-glucosidase, β-glucuronidase, lipase (C14), α-mannosidase, trypsin and valine aminopeptidase. The temperature range for growth of strain S16–07T was 14–43 °C, with the optimum temperature 23–32 °C. The pH range for growth was 6.0–9.0.