, 2007) harboring a suicide plasmid pBSL180 (Alexeyev & Shokolenk

, 2007) harboring a suicide plasmid pBSL180 (Alexeyev & Shokolenko,

1995), containing mini-Tn10Kmr, according to Kouzuma et al. (2010). Tn-insertion mutants were transferred to LMM plates overlaid with a thin LMM-agar layer containing Km and 8 mM MnO2 (brown in color). After incubation for 48 h under aerobic condition, halo zones formed around colonies were compared. Current generation was evaluated using a single-chamber MFC equipped with a graphite-felt anode (50 cm2; GF-80-3F; Sohgoh Carbon) and an air cathode (approximately 20 cm2, 0.7 mg platinum per cm, and four polytetrafluoroethylene layers) according to the method described previously (Newton Selleck GSK2118436 et al., 2009). In-frame disruption of the SO3030 gene in strain MR-1 was performed using suicide plasmid pSMV-10 (Saltikov & Newman, 2003) as described previously (Kouzuma et al., 2010). Briefly, a 1.6-kb fusion product, consisting of an upstream sequence of the SO3030 gene (784 bp), insertion sequence (18 bp), and downstream sequence (748 bp), was constructed by PCR and in-vitro extension Trametinib using primers listed in Table S1 (Supporting Information). This

fusion product was ligated into pSMV10 at a SpeI site. Resultant plasmid pSMV-3030 was introduced into MR-1 by filter mating with E. coli WM6026 to construct double-crossover mutants (designated ΔSO3030). For the complementation of the SO3030 gene, SO3030 was amplified by PCR using primers SO3030-F-HindIII and SO3030-R-XbaI (Table S1) and a resultant PCR product was digested and ligated into HindIII–XbaI-digested pBBR1MCS-5 (Kovach et al., 1995). A resultant plasmid, pBBR1-3030, was introduced into ΔSO3030 cells by the PLEKHB2 filter mating. Bottles containing LMM and 10 mM MnO2 or Fe(III) oxide were prepared in triplicate. They were inoculated with Shewanella cells and incubated at 30 °C. At a fixed time interval, amounts of Mn (IV) or Fe(II) in cultures were quantified by a colorimetric assay with leucoberbelin blue (Krumbein & Altmann, 1973) or ferrozine (Stookey, 1970), respectively, according to a method

described previously (Newton et al., 2009). Siderophore in a culture supernatant was analyzed by a method described by Kadi et al. (2008) with modifications. Shewanella cells were grown overnight in 100 mL of LMM supplemented with a mineral solution (1 mM MgSO4·7H2O, 0.1 mM CaCl2·2H2O, and 0.5 μM FeSO4·7H2O). A culture was centrifuged at 5000 g for 15 min, and 80 mL of a supernatant was loaded to a column used for solid-phase extraction (Sep-Pak C18, 100 mg; Waters). The column was washed with 10 mL of pure water, and adsorbed substances were eluted with 5 mL of methanol. The methanol solution was subsequently evaporated, and residual substances were dissolved in 0.5 mL of water. LC-MS analysis of the extracted supernatant was performed according to Kadi et al. (2008) using a LCMS-2010 EV (Shimadzu) equipped with an Eclipse XDB-C18 column (2.1 × 150 mm, 5 μm; Agilent) and operated in a positive ion mode.

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