A Nearly Isosteric Photosensitive Amide-Backbone Substitution Allows Enzyme Activity Switching in Ribonuclease S

Wildemann, Dirk; Schiene‐Fischer, Cordelia; Aumüller, Tobias; Bachmann, Annett; Kiefhaber, Thomas; Lücke, Christian; Fischer, Gunter

doi:10.1021/ja069048o

Cited by 74 publications

(77 citation statements)

References 58 publications

(141 reference statements)

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“…Deuteration of amide protons destabilizes helical structures, but the effect is very small (14). A near isosteric change in the polypeptide backbone can be achieved by introducing a thioxopeptide bond, i.e., by replacing an amide oxygen by sulfur (15).…”

mentioning

confidence: 99%

Mapping backbone and side-chain interactions in the transition state of a coupled protein folding and binding reaction

Bachmann

Wildemann

Praetorius

et al. 2011

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

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116

147

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Understanding the mechanism of protein folding requires a detailed knowledge of the structural properties of the barriers separating unfolded from native conformations. The S-peptide from ribonuclease S forms its α-helical structure only upon binding to the folded S-protein. We characterized the transition state for this binding-induced folding reaction at high resolution by determining the effect of site-specific backbone thioxylation and side-chain modifications on the kinetics and thermodynamics of the reaction, which allows us to monitor formation of backbone hydrogen bonds and side-chain interactions in the transition state. The experiments reveal that α-helical structure in the S-peptide is absent in the transition state of binding. Recognition between the unfolded S-peptide and the S-protein is mediated by loosely packed hydrophobic side-chain interactions in two well defined regions on the S-peptide. Close packing and helix formation occurs rapidly after binding. Introducing hydrophobic residues at positions outside the recognition region can drastically slow down association.phi-value analysis | protein-protein interaction | encounter complex formation | thioxo peptide bond C onformational changes in proteins play an important role in many biological processes. A detailed understanding of the mechanism of conformational transitions requires knowledge of the structural and dynamic properties of the initial and final states as well as the characterization of the transition barrier separating them. Site-directed mutagenesis proved a powerful tool to determine the properties of transition states for reactions involving proteins. Comparing the effect of amino acid replacements on kinetics and thermodynamics of a reaction identifies the interactions that are important for the rate-limiting step of a process. This method has been successfully applied to characterize transition states for protein folding (1, 2), for proteinprotein interactions (3-5) and for conformational changes in folded proteins (6). Protein folding transition states were shown to have native-like topology in the whole protein or in major parts of the structure (7-9) and it is commonly assumed that this includes the presence of native-like secondary structure (10, 11). Because site-directed mutagenesis can only modify amino acid side chains, it is still unclear at which stage of a folding reaction backbone hydrogen bonds in secondary structure elements are formed. Several approaches have been applied to test for secondary structure in protein folding transition states. Replacing amino acids by glycyl and prolyl residues leads to changes in backbone conformation, which was used to probe α-helix formation (12), but these replacements introduce additional effects due to altered side-chain interactions. Introducing ester bonds into the polypeptide backbone (13) also has multiple effects because it leads to the loss of a backbone hydrogen bonding donor and strongly increases conformational flexibility of the polypeptide backbone. Deuteration of a...

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mentioning

confidence: 99%

Mapping backbone and side-chain interactions in the transition state of a coupled protein folding and binding reaction

Bachmann

Wildemann

Praetorius

et al. 2011

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

Self Cite

116

147

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“…[48,49] It has recently been shown that this isomerization near the N-terminus of the S peptide in the protein complex ribonuclease S induces conformational changes sufficient to switch off enzymatic activity. [50] In many of these examples photo-excitation of a significant fraction of molecules is possible, resulting in large conformational changes and transient VCD signal levels can be similar to those observed in the Co(sp)Cl 2 model compound. In addition, the development of alternative detection schemes is about to further improve signal to noise levels in transient circular dichroism measurements.…”

Section: Photo-triggered Conformational Transitions Of Peptidesmentioning

confidence: 88%

Time-Resolved Chiral Vibrational Spectroscopy

Helbing¹,

Bonmarin²

2009

Chimia

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Advances in infrared laser technology and detection sensitivity have made time-resolved chiral vibrational spectroscopy experimentally feasible. Here we describe our recent efforts in detecting, for the first time, transient vibrational circular dichroism (VCD) signals with picosecond time resolution. The absorption changes of the cobalt (−)-sparteine complex Co(sp)Cl2 after visible excitation of a d-d excited state was probed in the CH-stretch region by alternating left-and right-handed circular polarized mid IR laser pulses. VCD spectra can be sensitive reporters of peptide and protein secondary structure or the absolute configuration of chiral organic compounds in solution. Recent developments are presented, which may in the future allow us to access this information in the course of fast chemical reactions.128 CHIMIA 2009, 63, No. 3 Young AcAdemics in switzerlAnd PArt ii doi:10.2533doi:10. /chimia.2009doi:10. .128 Chimia 63 (2009

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“…The N-terminal peptide comprising residues 1-20 (MjCM [1][2][3][4][5][6][7][8][9][10][11][12][13][14][15][16][17][18][19][20] ) was prepared by solid-phase peptide synthesis (SPPS) methods, and purified by HPLC. The C-terminal portion containing the additional mutation I77R to disfavor homodimerization 18 (MjCM * 22-93 ) was produced by heterologous expression in the CM-deficient Escherichia Coli strain KA13 27 with a C-terminal His 6 -tag and purified on a Ni-NTA column.…”

Section: Design Of a Heterodimeric Chorismate Mutasementioning

confidence: 99%

“…Solid-phase peptide synthesis mMjCM [1][2][3][4][5][6][7][8][9][10][11][12][13][14][15][16][17][18][19][20] was synthesized on a Wang resin preloaded with Fmoc-Leu (0.68 mmol/g) on a 433A peptide synthesizer (Applied Biosystems) on a 0.1 mmol scale with standard Fmoc-protected amino acids (Novabiochem). The peptide was cleaved from the resin and amino acid protecting groups were removed by incubation in 95% TFA, 2.5% H 2 O, and 2.5% TIS for 2 h. The resin was filtered off, excess TFA was evaporated, and the peptide was precipitated and washed with cold ether and dried under vacuum.…”

Section: In Vivo Complementation Experimentsmentioning

confidence: 99%

“…1,2 Split enzymes permit facile incorporation of synthetic peptide fragments into enzymes, which enabled structure-activity studies long before molecular cloning became a standard method for mutational analysis of proteins. 3 In addition, a wide variety of unnatural building blocks containing photoisomerizable groups, 4 environmentally sensitive dyes, 5 and modified backbones 6 could easily be incorporated into the peptide fragment of RNase S for biophysical studies.…”

Section: Introductionmentioning

confidence: 99%

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Design, selection, and characterization of a split chorismate mutase

et al. 2010

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Split proteins are versatile tools for detecting protein-protein interactions and studying protein folding. Here, we report a new, particularly small split enzyme, engineered from a thermostable chorismate mutase (CM). Upon dissecting the helical-bundle CM from Methanococcus jannaschii into a short N-terminal helix and a 3-helix segment and attaching an antiparallel leucine zipper dimerization domain to the individual fragments, we obtained a weakly active heterodimeric mutase. Using combinatorial mutagenesis and in vivo selection, we optimized the short linker sequences connecting the leucine zipper to the enzyme domain. One of the selected CMs was characterized in detail. It spontaneously assembles from the separately inactive fragments and exhibits wild-type like CM activity. Owing to the availability of a well characterized selection system, the simple 4-helix bundle topology, and the small size of the N-terminal helix, the heterodimeric CM could be a valuable scaffold for enzyme engineering efforts and as a split sensor for specifically oriented protein-protein interactions.

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A Nearly Isosteric Photosensitive Amide-Backbone Substitution Allows Enzyme Activity Switching in Ribonuclease S

Cited by 74 publications

References 58 publications

Mapping backbone and side-chain interactions in the transition state of a coupled protein folding and binding reaction

Mapping backbone and side-chain interactions in the transition state of a coupled protein folding and binding reaction

Time-Resolved Chiral Vibrational Spectroscopy

Design, selection, and characterization of a split chorismate mutase

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