In vivo reconstitution of an active siderophore transport system by a binding protein derivative lacking a signal sequence

Rohrbach, Martin; Paul, Sabine; Köster, Wolfgang

doi:10.1007/bf02456611

Cited by 20 publications

(26 citation statements)

References 74 publications

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“…Nevertheless, that such a muted conformational change can result in a protein form that is more resistant to proteolytic digestion is interesting and suggests that the ligand may protect a protease accessible site or loop structure within the binding pocket. This protection has now been demonstrated for three FhuD family members, E. coli FhuD (35) and S. aureus FhuD2 (14) and FhuD1 (this study).…”

Section: Fhud1 In S Aureussupporting

confidence: 67%

FhuD1, a Ferric Hydroxamate-binding Lipoprotein in Staphylococcus aureus

Sebulsky

Speziali

Shilton

et al. 2004

Journal of Biological Chemistry

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Staphylococcus aureus can utilize ferric hydroxamates as a source of iron under iron-restricted growth conditions. Proteins involved in this transport process are: FhuCBG, which encodes a traffic ATPase; FhuD2, a post-translationally modified lipoprotein that acts as a high affinity receptor at the cytoplasmic membrane for the efficient capture of ferric hydroxamates; and FhuD1, a protein with similarity to FhuD2. Gene duplication likely gave rise to fhuD1 and fhuD2. While the genomic locations of fhuCBG and fhuD2 in S. aureus strains are conserved, both the presence and the location of fhuD1 are variable. The apparent redundancy of FhuD1 led us to examine the role of this protein. We demonstrate that FhuD1 is expressed only under conditions of iron limitation through the regulatory activity of Fur. FhuD1 fractions with the cell membrane and binds hydroxamate siderophores but with lower affinity than FhuD2. Using small angle x-ray scattering, the solution structure of FhuD1 resembles that of FhuD2, and only a small conformational change is associated with ferrichrome binding. FhuD1, therefore, appears to be a receptor for ferric hydroxamates, like FhuD2. Our data to date suggest, however, that FhuD1 is redundant to FhuD2 and plays a minor role in hydroxamate transport. However, given the very real possibility that we have not yet identified the proper conditions where FhuD1 does provide an advantage over FhuD2, we anticipate that FhuD1 serves an enhanced role in the transport of untested hydroxamate siderophores and that it may play a prominent role during the growth of S. aureus in its natural environments.

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Section: Fhud1 In S Aureussupporting

confidence: 67%

FhuD1, a Ferric Hydroxamate-binding Lipoprotein in Staphylococcus aureus

Sebulsky

Speziali

Shilton

et al. 2004

Journal of Biological Chemistry

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“…As previously performed with other ABC importers (36,37), BtuF and the radiotracer are added to the spheroplast suspension and samples are removed at intervals. Bulk solution is removed by rapid filtration followed by several washes.…”

Section: Resultsmentioning

confidence: 99%

A single intact ATPase site of the ABC transporter BtuCD drives 5% transport activity yet supports full in vivo vitamin B ₁₂ utilization

Nir

Ovcharenko

Lewinson

2013

Proc. Natl. Acad. Sci. U.S.A.

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In all kingdoms of life, ATP binding cassette (ABC) transporters are essential to many cellular functions. In this large superfamily of proteins, two catalytic sites hydrolyze ATP to power uphill substrate translocation. A central question in the field concerns the relationship between the two ATPase catalytic sites: Are the sites independent of one another? Are both needed for function? Do they function cooperatively? These issues have been resolved for type I ABC transporters but never for a type II ABC transporter. The many mechanistic differences between type I and type II ABC transporters raise the question whether in respect to ATP hydrolysis the two subtypes are similar or different. We have addressed this question by studying the Escherichia coli vitamin B 12 type II ABC transporter BtuCD. We have constructed and purified a series of BtuCD variants where both, one, or none of the ATPase sites were rendered inactive by mutation. We find that, in a membrane environment, the ATPase sites of BtuCD are highly cooperative with a Hill coefficient of 2. We also find that, when one of the ATPase sites is inactive, ATP hydrolysis and vitamin B 12 transport by BtuCD is reduced by 95%. These exact features are also shared by the archetypical type I maltose ABC transporter. Remarkably, mutants that have lost 95% of their ATPase and transport capabilities still retain the ability to fully use vitamin B 12 in vivo. The results demonstrate that, despite the many differences between type I and type II ABC transporters, the fundamental mechanism of ATP hydrolysis remains conserved.cooperativity | membrane permeation | membrane proteins A TP binding cassette (ABC) transporters comprise one of the largest membrane protein superfamilies of any proteome (1-3). From bacteria to humans, they participate in processes such as cancer and bacterial multidrug resistance, antigen presentation, signal transduction, DNA repair, translation, cell division, homeostasis maintenance, detoxification, nutrient import, and antiviral defense (4-13). Hydrolyzing ATP to drive transport, ABC transporters shuttle cargo molecules to and fro the various cellular compartments, through the impermeable barriers of cell membranes. Notable mammalian examples include the multidrug exporters (4) and the transporter associated with antigen presentation (14). In prokaryotes, ABC transporters often function as importers and depend on a high-affinity substrate binding protein (SBP) that delivers the substrate to the cognate transporter. Structural and functional information derived from studies of prokaryotic systems largely shaped our mechanistic view of this superfamily of proteins (15)(16)(17)(18)(19)(20)(21)(22). An "alternating access" mechanistic model has been formulated over the years, according to which ATP hydrolysis power a sequence of conformational changes that shift the transporter between intracellular and extracellular accessible conformations (23)(24)(25)(26). This model has been most extensively demonstrated for the maltose transporter that i...

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“…His-tag FhuD was purified by metal chelate chromatography (POROS 20MC) charged with nickel, similarly as previously described (21) except that the BioCad high performance liquid chromatography system (PerSeptive Biosystems) was used. After cell lysis in 50 mM HEPES, pH 7.6, 0.5 M NaCl, the protein was bound to the column and washed with 10 volumes of 50 mM HEPES, pH 7.6, 0.5 M NaCl to remove unbound proteins and eluted with a gradient of 0 -0.5 M imidazole.…”

Section: Methodsmentioning

confidence: 99%

“…The protein was then dialyzed extensively against 10 mM Tris, pH 7.5 at 4°C. The His-tag of the protein was not cleaved off by enterokinase, because previous studies showed that the modified protein was functional (21).…”

Section: Methodsmentioning

confidence: 99%

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X-ray Crystallographic Structures of the Escherichia coli Periplasmic Protein FhuD Bound to Hydroxamate-type Siderophores and the Antibiotic Albomycin

Clarke¹,

Braun²,

Winkelmann³

et al. 2002

Journal of Biological Chemistry

135

108

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consists of an antibiotic group attached to a hydroxamate siderophore, electron density for the antibiotic portion was not observed. Therefore, this study provides a basis for the rational design of novel bacteriostatic agents, in the form of siderophore-antibiotic conjugates that can act as "Trojan horses," using the hydroxamatetype siderophore uptake system to actively deliver antibiotics directly into targeted pathogens.

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In vivo reconstitution of an active siderophore transport system by a binding protein derivative lacking a signal sequence

Cited by 20 publications

References 74 publications

FhuD1, a Ferric Hydroxamate-binding Lipoprotein in Staphylococcus aureus

FhuD1, a Ferric Hydroxamate-binding Lipoprotein in Staphylococcus aureus

A single intact ATPase site of the ABC transporter BtuCD drives 5% transport activity yet supports full in vivo vitamin B ₁₂ utilization

X-ray Crystallographic Structures of the Escherichia coli Periplasmic Protein FhuD Bound to Hydroxamate-type Siderophores and the Antibiotic Albomycin

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In vivo reconstitution of an active siderophore transport system by a binding protein derivative lacking a signal sequence

Cited by 20 publications

References 74 publications

FhuD1, a Ferric Hydroxamate-binding Lipoprotein in Staphylococcus aureus

FhuD1, a Ferric Hydroxamate-binding Lipoprotein in Staphylococcus aureus

A single intact ATPase site of the ABC transporter BtuCD drives 5% transport activity yet supports full in vivo vitamin B 12 utilization

X-ray Crystallographic Structures of the Escherichia coli Periplasmic Protein FhuD Bound to Hydroxamate-type Siderophores and the Antibiotic Albomycin

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A single intact ATPase site of the ABC transporter BtuCD drives 5% transport activity yet supports full in vivo vitamin B ₁₂ utilization