Gluconacetobacter diazotrophicus PAL5 (ATCC 49037) was grown at

Gluconacetobacter diazotrophicus PAL5 (ATCC 49037) was grown at

30 °C in LGIP medium supplemented with 0.75% ethanol (Reis et al., 1994) in a 60-L-working-volume Bioflow 5000 fermentor (New Brunswick Scientific, NJ). Procedures used for the culture, cell recovery, disruption, Akt inhibitor and cell membranes preparation have been described previously (Gómez-Manzo et al., 2008). Membrane particles were suspended (10 mg protein mL−1) in 10 mM potassium phosphate buffer, pH 6.0 (KP buffer), and Triton X-100 was added to a final concentration of 0.75%. The suspension was incubated on ice under gentle agitation for 120 min and centrifuged at 86 000 g for 30 min. The supernatant was used as a source of the ADHa and ADHi and purified by QAE-toyopearl column (6 × 20 cm), followed by a HA-Ultrogel column (3 × 20 cm) and Sephacryl-S200 column (3 × 120 cm) according to methods previously published (Gómez-Manzo et al., 2008). Inactive and active forms of ADH were conveniently separated during Sephacryl-S200 purification step. Fractions beta-catenin mutation that contained the active and the inactive forms of ADH were separately pooled, concentrated by ultrafiltration, and stored at 4 °C for further analysis. The purified ADH complexes were analyzed by SDS-PAGE (16 × 14 cm slab gels, 10% polyacrylamide)

by the method of Goodhew et al. (1986). For native PAGE, SDS was replaced by 0.1% Triton X-100, and polyacrylamide was decreased to 7.5%. Native gels were stained with 0.05% Coomassie

brilliant blue R-250. For HPLC analysis, PQQ was extracted from the purified enzyme according to the procedure described by Castro-Guerrero et al. (2004). The extracted and the standards quinones were analyzed by reverse-phase HPLC as previously described (González et al., 2006). The [2Fe-2S] cluster group of ADH (10) was quantified in a Shimadzu UV-2401 PC spectrophotometer by determining the acid-labile sulfur in the purified ADHi by the semi-micro method of Beinert (1983). Redox titration was performed in a cell equipped with a combined Ag/AgCl-Pt electrode (Cole-Palmer) and a potentiometer (Orion 520 A+; Thermo Fisher Scientific) as described by Dutton (1976). Redox mediators (50 μM) and titration procedures of cytochrome c associated with ADHi (15 mg of protein) were Ixazomib order the same as previously used for ADHa (Gómez-Manzo et al., 2010). All potentials values are reported against the standard hydrogen electrode (SHE). Experimental data were fitted by Nerst curves for four single-electron components (n = 1) with unknown redox potentials with a program kindly provided by Dr R. Louro (Universidade Nova de Lisboa). Minimization of the sum of the squared residuals was used for the selection of the best fitting model and gave the values of the mid-point potentials. Purified ADHi (10 mg protein) in 500 μL of 10 mM potassium phosphate, pH 6.

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