OD625 was chosen for evaluating the cell growth because absorbance of photosynthetic pigments is minimal around 625 nm (as shown in Figure 6). Phototrophic cultures were grown in low-intensity light (10 ± this website 1 W/m2), and chemotrophic cultures were grown in darkness. The list of growth
media used in this report and organic carbon sources included in each medium are described in Table 1. The pyruvate mineral salts (PMS, with 20 mM (2.2 g/L) pyruvate included) medium were prepared as reported previously [2]. The chemicals in yeast extract (YE) medium (per liter) are: K2HPO4 (1.0 g), MgSO4•7H2O (0.2 g), CaCl2•2H2O (20 mg), selleckchem Na2S2O3•5H2O (0.2 g), yeast extract (4.0 g), (NH4)2SO4 (1.0 g), chelated iron solution [21] (2 ml), d-biotin (15 μg), vitamin B12 find more (20 μg) and trace element solution (1 ml) with the final pH adjusted to pH 6.9-7.0. Components of the trace element solution were reported previously [2]. Pyruvate (20 mM for phototrophic growth and 40 mM for chemotrophic growth) is added to YE medium to prepare pyruvate-yeast extract (PYE) medium. Sodium acetate (40 mM) and HCO3 – (20 mM) are included in acetate-mineral salts (AMS) medium, and sugar (hexose or ribose)
(40 mM) and “”vitamin level”" yeast extract (0.02%) are included in sugar-grown medium. Cultures of H. modesticaldum were grown either photoheterotrophically in PMS, YE, PYE, AMS and different sugar-grown medium (listed in Table 1) or chemotrophically (dark, anoxic) in PYE medium. NH4Cl (in mineral salts medium), (NH4)2SO4 (in YE and PYE medium), and N2/H2 = 98/2 (under nitrogen fixation conditions) was used as the nitrogen source. Typically, 1-2% cultures (50-100 fold dilution) in the late exponential growth phase were used to inoculate fresh Ponatinib cell line media. Measurement of the uptake of pyruvate, acetate, lactate, fructose and glucose
The amount of pyruvate and lactate in the cultures of H. modesticaldum under different growth conditions was determined by the methods reported previously [9, 29]. The amount of D-glucose and pyruvate in the cultures of H. modesticaldum under different growth conditions was determined by the methods reported previously [9]. Uptake of D-fructose was estimated by a coupled hexokinase/phosphoglucose isomerase/glucose-6-phosphate dehydrogenase assay, and the amount of NADPH formed in the reaction, measured by the increase of the absorbance at 340 nm, is stoichiometric to the amount of D-fructose in solution. The amount of acetate production was determined by a coupled acetyl-CoA synthase/citrate synthase/malate dehydrogenase assay following the formation of NADH [30]. RNA extraction and quantitative real-time PCR (QRT-PCR) The methods used to extract RNA and perform QRT-PCR were described previously [9, 31]. QRT-PCR was performed to profile the gene expression under different growth conditions of H. modesticaldum. The primers for QRT-PCR in this report are listed in Additional file 6: Table S2.