NMR solution structure of SlyD from Escherichia coli: Spatial Separation of Prolyl Isomerase and Chaperone Function

Publikation: Beitrag in FachzeitschriftArtikelForschungPeer-Review

Autoren

  • Ulrich Weininger
  • Caroline Haupt
  • Kristian Schweimer
  • Wenke Graubner
  • Michael Kovermann
  • Thomas Brüser
  • Christian Scholz
  • Peter Schaarschmidt
  • Gabriel Zoldak
  • Franz X. Schmid
  • Jochen Balbach

Externe Organisationen

  • Martin-Luther-Universität Halle-Wittenberg
  • Universität Bayreuth
  • Roche Diagnostics GmbH
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Details

OriginalspracheEnglisch
Seiten (von - bis)295-305
Seitenumfang11
FachzeitschriftJournal of Molecular Biology
Jahrgang387
Ausgabenummer2
PublikationsstatusVeröffentlicht - 27 März 2009
Extern publiziertJa

Abstract

SlyD (sensitive to lysis D) is a putative folding helper from the bacterial cytosol and harbors prolyl isomerase and chaperone activities. We determined the solution NMR structure of a truncated version of SlyD (1-165) from Escherichia coli (SlyD*) that lacks the presumably unstructured C-terminal tail. SlyD* consists of two well-separated domains: the FKBP domain, which harbors the prolyl isomerase activity, and the insert-in-flap (IF) domain, which harbors the chaperone activity. The IF domain is inserted into a loop of the FKBP domain near the prolyl isomerase active site. The NMR structure of SlyD* showed no distinct orientation of the two domains relative to each other. In the FKBP domain, Tyr68 points into the active site, which might explain the lowered intrinsic prolyl isomerase activity and the much lower FK506 binding affinity of the protein compared with archetype human FKBP12 (human FK506 binding protein with 12 kDa). The thermodynamics and kinetics of substrate binding by SlyD* were quantified by fluorescence resonance energy transfer. NMR titration experiments revealed that the IF domain recognizes and binds unfolded or partially folded proteins and peptides. Insulin aggregation is markedly slowed by SlyD* as evidenced by two-dimensional NMR spectroscopy in real time, probably due to SlyD* binding to denatured insulin. The capacity of the IF domain to establish an initial encounter-collision complex, together with the flexible orientation of the two interacting domains, makes SlyD* a very powerful catalyst of protein folding.

ASJC Scopus Sachgebiete

Zitieren

NMR solution structure of SlyD from Escherichia coli: Spatial Separation of Prolyl Isomerase and Chaperone Function. / Weininger, Ulrich; Haupt, Caroline; Schweimer, Kristian et al.
in: Journal of Molecular Biology, Jahrgang 387, Nr. 2, 27.03.2009, S. 295-305.

Publikation: Beitrag in FachzeitschriftArtikelForschungPeer-Review

Weininger, U, Haupt, C, Schweimer, K, Graubner, W, Kovermann, M, Brüser, T, Scholz, C, Schaarschmidt, P, Zoldak, G, Schmid, FX & Balbach, J 2009, 'NMR solution structure of SlyD from Escherichia coli: Spatial Separation of Prolyl Isomerase and Chaperone Function', Journal of Molecular Biology, Jg. 387, Nr. 2, S. 295-305. https://doi.org/10.1016/j.jmb.2009.01.034
Weininger, U., Haupt, C., Schweimer, K., Graubner, W., Kovermann, M., Brüser, T., Scholz, C., Schaarschmidt, P., Zoldak, G., Schmid, F. X., & Balbach, J. (2009). NMR solution structure of SlyD from Escherichia coli: Spatial Separation of Prolyl Isomerase and Chaperone Function. Journal of Molecular Biology, 387(2), 295-305. https://doi.org/10.1016/j.jmb.2009.01.034
Weininger U, Haupt C, Schweimer K, Graubner W, Kovermann M, Brüser T et al. NMR solution structure of SlyD from Escherichia coli: Spatial Separation of Prolyl Isomerase and Chaperone Function. Journal of Molecular Biology. 2009 Mär 27;387(2):295-305. doi: 10.1016/j.jmb.2009.01.034
Weininger, Ulrich ; Haupt, Caroline ; Schweimer, Kristian et al. / NMR solution structure of SlyD from Escherichia coli : Spatial Separation of Prolyl Isomerase and Chaperone Function. in: Journal of Molecular Biology. 2009 ; Jahrgang 387, Nr. 2. S. 295-305.
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title = "NMR solution structure of SlyD from Escherichia coli: Spatial Separation of Prolyl Isomerase and Chaperone Function",
abstract = "SlyD (sensitive to lysis D) is a putative folding helper from the bacterial cytosol and harbors prolyl isomerase and chaperone activities. We determined the solution NMR structure of a truncated version of SlyD (1-165) from Escherichia coli (SlyD*) that lacks the presumably unstructured C-terminal tail. SlyD* consists of two well-separated domains: the FKBP domain, which harbors the prolyl isomerase activity, and the insert-in-flap (IF) domain, which harbors the chaperone activity. The IF domain is inserted into a loop of the FKBP domain near the prolyl isomerase active site. The NMR structure of SlyD* showed no distinct orientation of the two domains relative to each other. In the FKBP domain, Tyr68 points into the active site, which might explain the lowered intrinsic prolyl isomerase activity and the much lower FK506 binding affinity of the protein compared with archetype human FKBP12 (human FK506 binding protein with 12 kDa). The thermodynamics and kinetics of substrate binding by SlyD* were quantified by fluorescence resonance energy transfer. NMR titration experiments revealed that the IF domain recognizes and binds unfolded or partially folded proteins and peptides. Insulin aggregation is markedly slowed by SlyD* as evidenced by two-dimensional NMR spectroscopy in real time, probably due to SlyD* binding to denatured insulin. The capacity of the IF domain to establish an initial encounter-collision complex, together with the flexible orientation of the two interacting domains, makes SlyD* a very powerful catalyst of protein folding.",
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author = "Ulrich Weininger and Caroline Haupt and Kristian Schweimer and Wenke Graubner and Michael Kovermann and Thomas Br{\"u}ser and Christian Scholz and Peter Schaarschmidt and Gabriel Zoldak and Schmid, {Franz X.} and Jochen Balbach",
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TY - JOUR

T1 - NMR solution structure of SlyD from Escherichia coli

T2 - Spatial Separation of Prolyl Isomerase and Chaperone Function

AU - Weininger, Ulrich

AU - Haupt, Caroline

AU - Schweimer, Kristian

AU - Graubner, Wenke

AU - Kovermann, Michael

AU - Brüser, Thomas

AU - Scholz, Christian

AU - Schaarschmidt, Peter

AU - Zoldak, Gabriel

AU - Schmid, Franz X.

AU - Balbach, Jochen

N1 - Funding Information: This research was supported by grants from the Deutsche Forschungsgemeinschaft (BA 1821/4-1, SCHM 444/19-1 and GRK 1026 “Conformational Transitions in Macromolecular Interactions”) and the European Regional Development Fund (ERDF). G.Z. was supported by a Deutsche Akademische Austauschdienst postdoctoral fellowship in the program “Modern Applications of Biotechnology.” We thank Paul Rösch for NMR spectrometer time at 700 and 800 MHz and Christian Löw for very helpful discussions. We also thank Laurence Thirault, Franz Wagner, Sima Hassanzadeh-Makooi and Nicole Amtmann (Roche, Penzberg) for excellent technical assistance and Dr. Martin Humeník for matrix-assisted laser desorption/ionization time-of-flight measurements. Copyright: Copyright 2020 Elsevier B.V., All rights reserved.

PY - 2009/3/27

Y1 - 2009/3/27

N2 - SlyD (sensitive to lysis D) is a putative folding helper from the bacterial cytosol and harbors prolyl isomerase and chaperone activities. We determined the solution NMR structure of a truncated version of SlyD (1-165) from Escherichia coli (SlyD*) that lacks the presumably unstructured C-terminal tail. SlyD* consists of two well-separated domains: the FKBP domain, which harbors the prolyl isomerase activity, and the insert-in-flap (IF) domain, which harbors the chaperone activity. The IF domain is inserted into a loop of the FKBP domain near the prolyl isomerase active site. The NMR structure of SlyD* showed no distinct orientation of the two domains relative to each other. In the FKBP domain, Tyr68 points into the active site, which might explain the lowered intrinsic prolyl isomerase activity and the much lower FK506 binding affinity of the protein compared with archetype human FKBP12 (human FK506 binding protein with 12 kDa). The thermodynamics and kinetics of substrate binding by SlyD* were quantified by fluorescence resonance energy transfer. NMR titration experiments revealed that the IF domain recognizes and binds unfolded or partially folded proteins and peptides. Insulin aggregation is markedly slowed by SlyD* as evidenced by two-dimensional NMR spectroscopy in real time, probably due to SlyD* binding to denatured insulin. The capacity of the IF domain to establish an initial encounter-collision complex, together with the flexible orientation of the two interacting domains, makes SlyD* a very powerful catalyst of protein folding.

AB - SlyD (sensitive to lysis D) is a putative folding helper from the bacterial cytosol and harbors prolyl isomerase and chaperone activities. We determined the solution NMR structure of a truncated version of SlyD (1-165) from Escherichia coli (SlyD*) that lacks the presumably unstructured C-terminal tail. SlyD* consists of two well-separated domains: the FKBP domain, which harbors the prolyl isomerase activity, and the insert-in-flap (IF) domain, which harbors the chaperone activity. The IF domain is inserted into a loop of the FKBP domain near the prolyl isomerase active site. The NMR structure of SlyD* showed no distinct orientation of the two domains relative to each other. In the FKBP domain, Tyr68 points into the active site, which might explain the lowered intrinsic prolyl isomerase activity and the much lower FK506 binding affinity of the protein compared with archetype human FKBP12 (human FK506 binding protein with 12 kDa). The thermodynamics and kinetics of substrate binding by SlyD* were quantified by fluorescence resonance energy transfer. NMR titration experiments revealed that the IF domain recognizes and binds unfolded or partially folded proteins and peptides. Insulin aggregation is markedly slowed by SlyD* as evidenced by two-dimensional NMR spectroscopy in real time, probably due to SlyD* binding to denatured insulin. The capacity of the IF domain to establish an initial encounter-collision complex, together with the flexible orientation of the two interacting domains, makes SlyD* a very powerful catalyst of protein folding.

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