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Itions, the strain was grown in chemically defined medium with or without acetate supplementation (12 mM), under aerobic or anaerobic conditions. Analogous to what was observed with respect to the CO2 dependency, anaerobic 52232-67-4 site growth of L. johnsonii NCC 533 depended more strictly on acetate supplementation as compared to aerobic growth, which could be sustained without an external acetate source, albeit with a slower growth rate and a lower final biomass yield (Figure 4). This implies that the endogenous production of acetate under these conditions may be expected to be in the same range as the 12 mM that allowed similar growth restoration under anaerobic conditions 12926553 (see above). Both aerobic and anaerobic growth of L. johnsonii in chemically defined medium with 12 mM or 120 mM of acetate were analyzed with respect to acetate metabolism: significant change inOxygen Effect on Lactobacillus Growth RequirementsFigure 1. Microcolony growth and viability in environments varying in oxygen and CO2 content. L. johnsonii NCC 533 is grown on AnoporeTM slides that are transferred from a 2 hour pre-incubation period in an N2+5 CO2 environment to environments that vary in CO2 and O2 content. Average size of microcolonies grown aerobically (A) and anaerobically (B) and average viability of microcolonies grown aerobically (C) and anaerobically (D). Growth after the pre-incubation was either in the presence (closed symbols) or absence (open symbols) of 5 CO2. Data shown are the mean of all colonies counted for that time point and condition 6 standard deviation. doi:10.1371/journal.pone.0057235.gextracellular acetate were not detected by HPLC analysis nor by a highly specific and sensitive acetate kinase/pyruvate kinase assay (ref) (results not shown). This result is likely caused by analytical limitations that did not allow detection of the minute amounts of acetate that are required to sustain growth under these conditions, (estimated detection limit in spent medium is 200 mM).In most organisms acetyl-CoA functions as the central C2intermediate in several biosynthetic pathways. This metabolite can be produced from pyruvate by reactions catalyzed by pyruvate dehydrogenase (PDH) or pyruvate formate lyase (PFL). However, apart from a homologue for one subunit of pyruvate dehydrogenase, the corresponding genes appeared to be absent in the L. johnsonii NCC 533 genome [4]. This genotype is shared with theFigure 2. Effect of CO2 TBHQ depletion on aerobic and anaerobic growth. Growth in stirred pH-controlled batch cultures sparged by N2+5 CO2 (closed symbols) or N2+20 O2+5 CO2 (open symbols) as measured at OD600. Data shown are the mean of at least two independent experiments 6 standard error of the mean. In panel B, the gas regime was switched after 15755315 3 hours of exponential growth from a CO2-rich gas to a CO2-free gas: N2 (closed symbols curve), N2+20 O2 (open symbols). Growth curves are the average 6 standard deviation of triplicate experiments. doi:10.1371/journal.pone.0057235.gOxygen Effect on Lactobacillus Growth RequirementsFigure 3. Acetate requirement for anaerobic growth. Growth of L. johnsonii NCC 533 in a chemically defined medium with varying concentrations of sodium acetate: 12 mM as in standard CDM (closed square symbols) 120 mM (round symbols), 12 mM (triangular symbols) and without any Na-acetate supplemented (open square symbols) in stirred pH controlled cultures sparged with N2+5 CO2 at a rate of 500 ml/min. The growth curves are the average of d.Itions, the strain was grown in chemically defined medium with or without acetate supplementation (12 mM), under aerobic or anaerobic conditions. Analogous to what was observed with respect to the CO2 dependency, anaerobic growth of L. johnsonii NCC 533 depended more strictly on acetate supplementation as compared to aerobic growth, which could be sustained without an external acetate source, albeit with a slower growth rate and a lower final biomass yield (Figure 4). This implies that the endogenous production of acetate under these conditions may be expected to be in the same range as the 12 mM that allowed similar growth restoration under anaerobic conditions 12926553 (see above). Both aerobic and anaerobic growth of L. johnsonii in chemically defined medium with 12 mM or 120 mM of acetate were analyzed with respect to acetate metabolism: significant change inOxygen Effect on Lactobacillus Growth RequirementsFigure 1. Microcolony growth and viability in environments varying in oxygen and CO2 content. L. johnsonii NCC 533 is grown on AnoporeTM slides that are transferred from a 2 hour pre-incubation period in an N2+5 CO2 environment to environments that vary in CO2 and O2 content. Average size of microcolonies grown aerobically (A) and anaerobically (B) and average viability of microcolonies grown aerobically (C) and anaerobically (D). Growth after the pre-incubation was either in the presence (closed symbols) or absence (open symbols) of 5 CO2. Data shown are the mean of all colonies counted for that time point and condition 6 standard deviation. doi:10.1371/journal.pone.0057235.gextracellular acetate were not detected by HPLC analysis nor by a highly specific and sensitive acetate kinase/pyruvate kinase assay (ref) (results not shown). This result is likely caused by analytical limitations that did not allow detection of the minute amounts of acetate that are required to sustain growth under these conditions, (estimated detection limit in spent medium is 200 mM).In most organisms acetyl-CoA functions as the central C2intermediate in several biosynthetic pathways. This metabolite can be produced from pyruvate by reactions catalyzed by pyruvate dehydrogenase (PDH) or pyruvate formate lyase (PFL). However, apart from a homologue for one subunit of pyruvate dehydrogenase, the corresponding genes appeared to be absent in the L. johnsonii NCC 533 genome [4]. This genotype is shared with theFigure 2. Effect of CO2 depletion on aerobic and anaerobic growth. Growth in stirred pH-controlled batch cultures sparged by N2+5 CO2 (closed symbols) or N2+20 O2+5 CO2 (open symbols) as measured at OD600. Data shown are the mean of at least two independent experiments 6 standard error of the mean. In panel B, the gas regime was switched after 15755315 3 hours of exponential growth from a CO2-rich gas to a CO2-free gas: N2 (closed symbols curve), N2+20 O2 (open symbols). Growth curves are the average 6 standard deviation of triplicate experiments. doi:10.1371/journal.pone.0057235.gOxygen Effect on Lactobacillus Growth RequirementsFigure 3. Acetate requirement for anaerobic growth. Growth of L. johnsonii NCC 533 in a chemically defined medium with varying concentrations of sodium acetate: 12 mM as in standard CDM (closed square symbols) 120 mM (round symbols), 12 mM (triangular symbols) and without any Na-acetate supplemented (open square symbols) in stirred pH controlled cultures sparged with N2+5 CO2 at a rate of 500 ml/min. The growth curves are the average of d.

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