Journal
JOURNAL OF MEMBRANE BIOLOGY
Volume 201, Issue 2, Pages 97-107Publisher
SPRINGER
DOI: 10.1007/s00232-004-0711-x
Keywords
symporter; Nramp; manganese transport
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A bioinformatic approach was used for the identification of residues that are conserved within the Nramp family of metal transporters. Site-directed mutagenesis was then carried out to change six conserved acidic residues (i.e., Asp-34, Glu-102, Asp-109, Glu-112, Glu-154, and Asp-238) in the E. coli Nramp homolog mntH. Of these six, five of them, Asp-34, Glu-102, Asp-109, Glu-112, and Asp-238 appear to be important for function since conservative substitutions at these sites result in a substantial loss of transport function. In addition, all of the residues within the signature sequence of the Nramp family, DPGN, were also mutated in this study. Each residue was changed to several different side chains, and of ten site-directed mutations made in this motif, only P35G showed any measurable level of Mn-54(2+) uptake with a V-max value of approximately 10% of wildtype and a slightly elevated Km value. Overall, the data are consistent with a model where helix breakers in the conserved DPGN motif in TMS-1 provide a binding pocket in which Asp-34, Asn-37, Asp-109, Glu-112 (and possibly other residues) are involved in the coordination of Mn2+. Other residues such as Glu-102 and Asp238 may play a role in the release of Mn2+ to the cytoplasm or may be involved in maintaining secondary structure.
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