Among the various mechanisms used by bacteria to combat ROS-mediated damage, peroxiredoxins are unique in catalyzing the conversion of H2O2 and organic hydroperoxides using cysteine residues in their catalytic cycle rather than metal cofactors like superoxide dismutases, Stem Cells inhibitor catalases, and cytochrome c peroxidases (Baker & Poole, 2003; Dubbs & Mongkolsuk, 2007). So far, three bacterial members of peroxiredoxins
have been reported, and their contribution to aerotolerance and oxidative stress resistance has been well characterized in a number of organisms (Jacobson et al., 1989; Jeong et al., 2000; Seaver & Imlay, 2001; Cha et al., 2004; Wang et al., 2005; Atack et al., 2008). In this
study, genomic sequence analysis revealed that M. magneticum AMB-1 contains three peroxiredoxin homologues (amb0664, amb3876, and amb2684), which, based on sequence alignment, correspond to AhpC, Tpx, and BCP, respectively. In further support of the existence of functional peroxiredoxin-mediated catalytic cycles in AMB-1 was the revelation in the genome of other important catalytic partners, including thioredoxin reductases (amb3892 and amb0663), thioredoxins (amb4286 and amb0007), and glutaredoxins (amb1606 and amb2117). The catalytic properties displayed by these three peroxiredoxins in vitro appear to be similar to those described in other microorganisms (Jeong et al., 2000; Baker et al., 2001; Cha et al., 2004). Magnetospirillum this website magneticum AMB-1 may therefore be well equipped with a peroxiredoxin-mediated antioxidative system to counteract the potentially adverse effects incurred by reactive oxygen molecules in vivo. Our observation that the absence of all three Prxs caused a significant defect in growth and Selleckchem Ponatinib magnetosome formation under microaerobic or highly aerobic conditions indicates the individual importance of these Prxs in defending against oxidative stress. Note that, we cannot at present distinguish between whether Prxs were directly involved in magnetosome formation by scavenging
the generated hydrogen peroxide and whether the effect of Prxs on magnetosome synthesis was due to its role in cell growth. Nevertheless, hardly any effect was observed either for growth or magnetosome formation in the absence of these Prxs under anaerobic conditions. This is in contrast to Prx2 in E. coli, which has been shown to be essential for the anaerobic respiration-dependent growth (Cha et al., 2004). The reason for such a difference remains unknown, and it is probably because different internal electron acceptors were used during the electron transfer, where the accumulation of oxidative products was not as severe as those in E. coli during anaerobic respiration. A unique characteristic in magnetotactic bacteria including M.