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1

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Diffusion through channel derivatives of the Escherichia coli FhuA transport protein : FhuA transport protein of E. coli

Braun, Michael ; Killmann, Helmut ; Maier, Elke ; [weitere]

Wiley ; 2002

In: European Journal of Biochemistry Vol. 269, No. 20 ( 2002-10), p. 4948-4959

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In: European Journal of Biochemistry, Wiley, Vol. 269, No. 20 ( 2002-10), p. 4948-4959

Materialart: Online-Ressource

ISSN: 0014-2956

URL: Article

DOI: 10.1046/j.1432-1033.2002.03195.x

RVK:

WA 15000

Sprache: Englisch

Verlag: Wiley

Publikationsdatum: 2002

ZDB Id: 2172518-4

SSG: 12

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2

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Mutant Analysis of the Escherichia coli FhuA Protein Reveals Sites of FhuA Activity

Endriß, Franziska ; Braun, Michael ; Killmann, Helmut ; [weitere]

American Society for Microbiology ; 2003

In: Journal of Bacteriology Vol. 185, No. 16 ( 2003-08-15), p. 4683-4692

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In: Journal of Bacteriology, American Society for Microbiology, Vol. 185, No. 16 ( 2003-08-15), p. 4683-4692

Kurzfassung: The FhuA outer membrane protein of Escherichia coli actively transports ferrichrome, albomycin, and rifamycin CGP 4832, and confers sensitivity to microcin J25, colicin M, and the phages T1, T5, and φ80. Guided by the FhuA crystal structure and derived predictions on how FhuA might function, mutants were isolated in the cork domain (residues 1 to 160) and in the β-barrel domain (residues 161 to 714). Deletion of the TonB box (residues 7 to 11) completely inactivated all TonB-dependent functions of FhuA. Fixation of the cork to turn 7 of the barrel through a disulfide bridge between introduced C27 and C533 residues abolished ferrichrome transport, which was restored by reduction of the disulfide bond. Deletion of residues 24 to 31, including the switch helix (residues 24 to 29), which upon binding of ferrichrome to FhuA undergoes a large structural transition (17 Å) and exposes the N terminus of FhuA (TonB box) to the periplasm, reduced FhuA transport activity (79% of the wild-type activity) but conferred full sensitivity to colicin M and the phages. Duplication of residues 23 to 30 or deletion of residues 13 to 20 resulted in FhuA derivatives with properties similar to those of FhuA with a deletion of residues 24 to 31. However, a frameshift mutation that changed QSEA at positions 18 to 21 to KKAP abolished almost completely most of FhuA's activities. The conserved residues R93 and R133 among energy-coupled outer membrane transporters are thought to fix the cork to the β-barrel by forming salt bridges to the conserved residues E522 and E571 of the β-barrel. Proteins with the E522R and E571R mutations were inactive, but inactivity was not caused by repulsion of R93 by R522 and R571 and of R133 by R571. Point mutations in the cork at sites that move or do not move upon the binding of ferrichrome had no effect or conferred only slightly reduced activities. It is concluded that the TonB box is essential for FhuA activity. The TonB box region has to be flexible, but its distance from the cork domain can greatly vary. The removal of salt bridges between the cork and the barrel affects the structure but not the function of FhuA.

Materialart: Online-Ressource

ISSN: 0021-9193 , 1098-5530

URL: Article

DOI: 10.1128/JB.185.16.4683-4692.2003

Sprache: Englisch

Verlag: American Society for Microbiology

Publikationsdatum: 2003

ZDB Id: 1481988-0

SSG: 12

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3

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Iron transport and signaling in Escherichia coli

Braun, Volkmar ; Braun, Michael

Wiley ; 2002

In: FEBS Letters Vol. 529, No. 1 ( 2002-10-02), p. 78-85

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In: FEBS Letters, Wiley, Vol. 529, No. 1 ( 2002-10-02), p. 78-85

Kurzfassung: Bacteria solve the iron supply problem caused by the insolubility of Fe 3+ by synthesizing iron‐complexing compounds, called siderophores, and by using iron sources of their hosts, such as heme and iron bound to transferrin and lactoferrin. Escherichia coli , as an example of Gram‐negative bacteria, forms sophisticated Fe 3+ –siderophore and heme transport systems across the outer membrane. The crystal structures of three outer membrane transport proteins now allow insights into energy‐coupled transport mechanisms. These involve large long‐range structural transitions in the transport proteins in response to substrate binding, including substrate gating. Energy is provided by the proton motive force of the cytoplasmic membrane through the activity of a protein complex that is inserted in the cytoplasmic membrane and that contacts the outer membrane transporters. Certain transport proteins also function in siderophore‐mediated signaling cascades that start at the cell surface and flow to the cytoplasm to initiate transcription of genes encoding proteins for transport and siderophore biosynthesis.

Materialart: Online-Ressource

ISSN: 0014-5793 , 1873-3468

URL: Article

DOI: 10.1016/S0014-5793(02)03185-X

RVK:

WA 15000

Sprache: Englisch

Verlag: Wiley

Publikationsdatum: 2002

ZDB Id: 1460391-3

SSG: 12

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4

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Outer Membrane Channels and Active Transporters for the Uptake of Antibiotics

Braun, Volkmar ; Bös, Christoph ; Braun, Michael ; [weitere]

Oxford University Press (OUP) ; 2001

In: The Journal of Infectious Diseases Vol. 183, No. s1 ( 2001-03), p. S12-S16

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In: The Journal of Infectious Diseases, Oxford University Press (OUP), Vol. 183, No. s1 ( 2001-03), p. S12-S16

Materialart: Online-Ressource

ISSN: 0022-1899 , 1537-6613

URL: Issue

URL: Article

DOI: 10.1086/jid.2001.183.issue-s1

DOI: 10.1086/318840

RVK:

XA 10000

Sprache: Englisch

Verlag: Oxford University Press (OUP)

Publikationsdatum: 2001

ZDB Id: 1473843-0

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5

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The beta-barrel domain of FhuADelta5-160 is sufficient for TonB-dependent FhuA activities of Escherichia coli

Braun, Michael ; Killmann, Helmut ; Braun, Volkmar

Wiley ; 1999

In: Molecular Microbiology Vol. 33, No. 5 ( 1999-09), p. 1037-1049

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In: Molecular Microbiology, Wiley, Vol. 33, No. 5 ( 1999-09), p. 1037-1049

Materialart: Online-Ressource

ISSN: 0950-382X , 1365-2958

URL: Article

DOI: 10.1046/j.1365-2958.1999.01546.x

Sprache: Englisch

Verlag: Wiley

Publikationsdatum: 1999

ZDB Id: 1501537-3

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6

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FhuA Barrel-Cork Hybrids Are Active Transporters and Receptors

Killmann, Helmut ; Braun, Michael ; Herrmann, Christina ; [weitere]

American Society for Microbiology ; 2001

In: Journal of Bacteriology Vol. 183, No. 11 ( 2001-06), p. 3476-3487

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In: Journal of Bacteriology, American Society for Microbiology, Vol. 183, No. 11 ( 2001-06), p. 3476-3487

Kurzfassung: The crystal structure of Escherichia coli FhuA reveals a β-barrel domain that is closed by a globular cork domain. It has been assumed that the proton motive force of the cytoplasmic membrane through the interaction of the TonB protein with the TonB box of the cork opens the FhuA channel. Yet, deletion of the cork results in an FhuA derivative, FhuAΔ5–160, that still displays TonB-dependent substrate transport and phage receptor activity. To investigate this unexpected finding further, we constructed FhuAΔ5–160 derivatives of FhuA proteins from Salmonella paratyphi B, Salmonella enterica serovar Typhimurium, and Pantoea agglomerans . The FhuAΔ5–160 proteins inserted correctly into the outer membrane, and with the exception of the P. agglomerans protein, transported ferrichrome and albomycin. FhuA hybrids consisting of the β-barrel of one strain and the cork of another strain were active and showed higher TonB-dependent ferrichrome transport rates than the corkless derivatives. Exceptions were the E. coli β-barrel/ Salmonella serovar Typhimurium cork hybrid protein and the Salmonella serovar Typhimurium β-barrel/ P. agglomerans cork hybrid protein, both of which were less active than the β-barrels alone. Each of the FhuA mutant proteins displayed activity for each of their ligands, except for phage T5, only when coupled to TonB. The hybrid FhuA proteins displayed a similar activity with the E. coli TonB protein as with their cognate TonB proteins. Sensitivity to phages T1, T5, and φ80, rifamycin CGP 4832, and colicin M was determined by the β-barrel, whereas sensitivity to phage ES18 and microcin J25 required both the β-barrel and cork domains. These results demonstrate that the β-barrel domain of FhuA confers activity and specificity and responds to TonB and that the cork domains of various FhuA proteins can be interchanged and contribute to the activities of the FhuA hybrids.

Materialart: Online-Ressource

ISSN: 0021-9193 , 1098-5530

URL: Article

DOI: 10.1128/JB.183.11.3476-3487.2001

Sprache: Englisch

Verlag: American Society for Microbiology

Publikationsdatum: 2001

ZDB Id: 1481988-0

SSG: 12

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7

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In Vivo Reconstitution of the FhuA Transport Protein of Escherichia coli K-12

Braun, Michael ; Endriss, Franziska ; Killmann, Helmut ; [weitere]

American Society for Microbiology ; 2003

In: Journal of Bacteriology Vol. 185, No. 18 ( 2003-09-15), p. 5508-5518

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In: Journal of Bacteriology, American Society for Microbiology, Vol. 185, No. 18 ( 2003-09-15), p. 5508-5518

Kurzfassung: The FhuA protein in the outer membrane of Escherichia coli actively transports ferrichrome and the antibiotics albomycin and rifamycin CGP 4832 and serves as a receptor for the phages T1, T5, and φ80 and for colicin M and microcin J25. The crystal structure reveals a β-barrel with a globular domain, the cork, which closes the channel formed by the barrel. Genetic deletion of the cork resulted in a β-barrel that displays no FhuA activity. A functional FhuA was obtained by cosynthesis of separately encoded cork and the β-barrel domain, each endowed with a signal sequence, which showed that complementation occurs after secretion of the fragments across the cytoplasmic membrane. Inactive complete mutant FhuA and an FhuA fragment containing 357 N-proximal amino acid residues complemented the separately synthesized wild-type β-barrel to form an active FhuA. Previous claims that the β-barrel is functional as transporter and receptor resulted from complementation by inactive complete FhuA and the 357-residue fragment. No complementation was observed between the wild-type cork and complete but inactive FhuA carrying cork mutations that excluded the exchange of cork domains. The data indicate that active FhuA is reconstituted extracytoplasmically by insertion of separately synthesized cork or cork from complete FhuA into the β-barrel, and they suggest that in wild-type FhuA the β-barrel is formed prior to the insertion of the cork.

Materialart: Online-Ressource

ISSN: 0021-9193 , 1098-5530

URL: Article

DOI: 10.1128/JB.185.18.5508-5518.2003

Sprache: Englisch

Verlag: American Society for Microbiology

Publikationsdatum: 2003

ZDB Id: 1481988-0

SSG: 12

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8

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Excretion of a protease by Serratia marcescens

Braun, Volkmar ; Schmitz, Gudrun

Springer Science and Business Media LLC ; 1980

In: Archives of Microbiology Vol. 124, No. 1 ( 1980-1), p. 55-61

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In: Archives of Microbiology, Springer Science and Business Media LLC, Vol. 124, No. 1 ( 1980-1), p. 55-61

Materialart: Online-Ressource

ISSN: 0302-8933 , 1432-072X

URL: Article

DOI: 10.1007/BF00407028

RVK:

WA 15000

Sprache: Englisch

Verlag: Springer Science and Business Media LLC

Publikationsdatum: 1980

ZDB Id: 1458451-7

ZDB Id: 477-7

ZDB Id: 124824-8

SSG: 12

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9

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Hemolytic activity of Serratia marcescens

Braun, Volkmar ; G�nther, Hannelore ; Neu�, Burkard ; [weitere]

Springer Science and Business Media LLC ; 1985

In: Archives of Microbiology Vol. 141, No. 4 ( 1985-5), p. 371-376

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In: Archives of Microbiology, Springer Science and Business Media LLC, Vol. 141, No. 4 ( 1985-5), p. 371-376

Materialart: Online-Ressource

ISSN: 0302-8933 , 1432-072X

URL: Article

DOI: 10.1007/BF00428852

RVK:

WA 15000

Sprache: Englisch

Verlag: Springer Science and Business Media LLC

Publikationsdatum: 1985

ZDB Id: 1458451-7

ZDB Id: 477-7

ZDB Id: 124824-8

SSG: 12

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10

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Colicins: structures, modes of action, transfer through membranes, and evolution

Braun, Volkmar ; Pilsl, Holger ; Gro�, Patricia

Springer Science and Business Media LLC ; 1994

In: Archives of Microbiology Vol. 161, No. 3 ( 1994-3), p. 199-206

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In: Archives of Microbiology, Springer Science and Business Media LLC, Vol. 161, No. 3 ( 1994-3), p. 199-206

Materialart: Online-Ressource

ISSN: 0302-8933 , 1432-072X

URL: Article

DOI: 10.1007/BF00248693

RVK:

WA 15000

Sprache: Englisch

Verlag: Springer Science and Business Media LLC

Publikationsdatum: 1994

ZDB Id: 1458451-7

ZDB Id: 477-7

ZDB Id: 124824-8

SSG: 12

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