Bacterial Chaperone Domain Insertions Convert Human FKBP12 into an Excellent Protein-Folding Catalyst—A Structural and Functional Analysis-Reference-Cited by-同舟云学术

Bacterial Chaperone Domain Insertions Convert Human FKBP12 into an Excellent Protein-Folding Catalyst—A Structural and Functional Analysis

Published:2024-03-23 Issue:7 Volume:29 Page:1440
ISSN:1420-3049
Container-title:Molecules
language:en
Short-container-title:Molecules

Author:

Žoldák Gabriel¹^ORCID,Knappe Thomas A.²,Geitner Anne-Juliane²,Scholz Christian³,Dobbek Holger⁴,Schmid Franz X.²,Jakob Roman P.⁵^ORCID

Affiliation:

1. Center for Interdisciplinary Biosciences, Technology and Innovation Park, Pavol Jozef Šafárik University in Košice, 040 11 Kosice, Slovakia

2. Laboratorium für Biochemie und Bayreuther Zentrum für Molekulare Biowissenschaften, Universität Bayreuth, 95447 Bayreuth, Germany

3. Roche Diagnostics GmbH, Nonnenwald 2, 82377 Penzberg, Germany

4. Institut für Biologie, Strukturbiologie/Biochemie, Humboldt-Universität zu Berlin, Unter den Linden 6, 10099 Berlin, Germany

5. Departement Biozentrum, University of Basel, Spitalstrasse 41, 4056 Basel, Switzerland

Abstract

Many folding enzymes use separate domains for the binding of substrate proteins and for the catalysis of slow folding reactions such as prolyl isomerization. FKBP12 is a small prolyl isomerase without a chaperone domain. Its folding activity is low, but it could be increased by inserting the chaperone domain from the homolog SlyD of E. coli near the prolyl isomerase active site. We inserted two other chaperone domains into human FKBP12: the chaperone domain of SlpA from E. coli, and the chaperone domain of SlyD from Thermococcus sp. Both stabilized FKBP12 and greatly increased its folding activity. The insertion of these chaperone domains had no influence on the FKBP12 and the chaperone domain structure, as revealed by two crystal structures of the chimeric proteins. The relative domain orientations differ in the two crystal structures, presumably representing snapshots of a more open and a more closed conformation. Together with crystal structures from SlyD-like proteins, they suggest a path for how substrate proteins might be transferred from the chaperone domain to the prolyl isomerase domain.

Funder

Fonds der Chemischen Industrie and the Deutsche Forschungsgemeinschaft

Publisher

MDPI AG

Link

https://www.mdpi.com/1420-3049/29/7/1440/pdf

Reference57 articles.

1. Extremely rapid folding in the absence of intermediates: The cold-shock protein from Bacillus subtilis;Schindler;Nat. Struct. Biol.,1995

2. Early events in protein folding;Ferguson;Curr. Opin. Struct. Biol.,2003

3. Submillisecond folding of monomeric lambda repressor;Huang;Proc. Natl. Acad. Sci. USA,1995

4. Protein folding and unfolding in microseconds to nanoseconds by experiment and simulation;Mayor;Proc. Natl. Acad. Sci. USA,2000

5. Prolyl isomerization and its catalysis in protein folding and protein function;Schmidpeter;J. Mol. Biol.,2015