Fig. 2

Turbidity, substrate utilisation and metabolite formation of C. perfringens FMT 1006. C. perfringens was incubated in YC-G50 (50 mM glucose) and YC-PD50 (50 mM 1,2PD) or in YC in 30 mL serum flasks for 24 h anaerobically at 37 °C, OD₆₀₀ was monitored, and substrate utilisation and metabolite formation were analysed by HPLC-RI. (A) OD₆₀₀, (B) glucose utilisation, (C) 1,2PD utilisation, and (D) lactate, (E) 1-propanol, (F) acetate, (G) propanal, (H) butyrate, and (I) propionate formation in. Each time point is an average of n = 2–7 biological replicates