Efficient factors in protein modification: ADenosine deaminase esterification by woodward reagent K

Mahnam, Karim; Moosavi‐Movahedi, Ali Akbar; Bahrami, Homayoon; Hakimelahi, G. H.; Ataie, G.; Jalili, Seifollah; Saboury, Ali Akbar; Ahmad, Faizan; Safarian, Shahrokh; Amanlou, Massoud; Moshiri, Behzad

doi:10.1007/bf03246004

Cited by 3 publications

(3 citation statements)

References 33 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…The modification of the ␤-casein by WRK showed a new absorption peak in the wavelength range 340-350 nm, establishing the modification of aspartate and glutamate residues [33,48]. The first step in WRK reaction is the formation of ketoketenimine, which then reacts with carboxylate groups to produce an enol ester [49] with an absorbance peak at 340-350 nm. CD spectra of WRK-modified ␤-casein showed more negative ellipticity relative to native ␤-casein in the range of 250-204 nm (Fig.…”

Section: Resultsmentioning

confidence: 99%

Acidic residue modifications restore chaperone activity of β-casein interacting with lysozyme

Moosavi-Movahedi

Rajabzadeh

Amani

et al. 2011

International Journal of Biological Macromolecules

Self Cite

View full text Add to dashboard Cite

Section: Resultsmentioning

confidence: 99%

Acidic residue modifications restore chaperone activity of β-casein interacting with lysozyme

Moosavi-Movahedi

Rajabzadeh

Amani

et al. 2011

International Journal of Biological Macromolecules

Self Cite

View full text Add to dashboard Cite

“…As such it is stable, but it can be activated by bases initiating a rearrangement to form a ketenimine that reacts with carboxylic acids to form enol esters. Due to this reactivity, WRK has also been employed in enzymology for analysis of enzyme mechanisms through covalent modification of key carboxylic acids and other amino acids (Bustos et al, 1996;Carvajal et al, 2004;Komissarov et al, 1995;Mahnam et al, 2008;Sinha and Brewer, 1985).…”

Section: Discussionmentioning

confidence: 99%

“…Woodward's reagent K (WRK) (Kemp and Chien, 1967;) ( Figure 1A) has been employed in protein chemistry to covalently modify nucleophilic cysteine (Bustos et al, 1996), histidine (Carvajal et al, 2004), and carboxylic acid residues (Bodlaender et al, 1969;Feinstein et al, 1969;Komissarov et al, 1995;Mahnam et al, 2008;Pé tra and Neurath, 1971;Pé tra, 1971;Sinha and Brewer, 1985) in order to study enzymatic activity. We have recently described that ABPP probes based on WRK can be surprisingly selective and covalently modify the N-terminal proline of macrophage migration inhibitory factor (Qian et al, 2016).…”

Section: Introductionmentioning

confidence: 99%

Covalent Protein Labeling at Glutamic Acids

Martín‐Gago

Fansa

Winzker

et al. 2017

Cell Chemical Biology

View full text Add to dashboard Cite

Covalent labeling of amino acids in proteins by reactive small molecules, in particular at cysteine SH and lysine NH groups, is a powerful approach to identify and characterize proteins and their functions. However, for the less-reactive carboxylic acids present in Asp and Glu, hardly any methodology is available. Employing the lipoprotein binding chaperone PDE6δ as an example, we demonstrate that incorporation of isoxazolium salts that resemble the structure and reactivity of Woodward's reagent K into protein ligands provides a novel method for selective covalent targeting of binding site carboxylic acids in whole proteomes. Covalent adduct formation occurs via rapid formation of enol esters and the covalent bond is stable even in the presence of strong nucleophiles. This new method promises to open up hitherto unexplored opportunities for chemical biology research.

show abstract

Molecular dynamic simulations of nanomechanic chaperone peptide and effects of in silico His mutations on nanostructured function

Barzegar

Moosavi-Movahedi

Mahnam

et al. 2008

Journal of Peptide Science

View full text Add to dashboard Cite

The nanoscale peptide YSGVCHTDLHAWHGDWPLPVK exhibits molecular chaperone activity and prevents protein aggregation under chemical and/or thermal stress. Here, His mutations of this peptide and their impact on chaperone activity were evaluated using theoretical techniques. Molecular dynamic (MD) simulations with simulated annealing (SA) of different mutant nanopeptides were employed to determine the contribution of the scaffolding His residues (H45, H49, H52), when mutated to Pro, on chaperone action in vitro. The in silico mutations of His residues to Pro (H45P, H49P, H52P) revealed loss of secondary ordered strand structure. However, a small part of the strand conformation was formed in the middle region of the native chaperone peptide. The His-to-Pro mutations resulted in decreased gyration radius (Rg) values and surface accessibility of the mutant peptides under the simulation times. The invariant dihedral angle (phi) values and the disrupting effects of the Pro residues indicated the coil conformation of mutant peptides. The failure of the chaperone-like action in the Pro mutant peptides was consistent with their decreased effective accessible surfaces. The high variation of Phi value for His residues in native chaperone peptide leads to high flexibility, such as a minichaperone acting as a nanomachine at the molecular level. Our findings demonstrate that the peptide strand conformation motif with high flexibility at nanoscale is critical for chaperone activity.

show abstract

Efficient factors in protein modification: ADenosine deaminase esterification by woodward reagent K

Cited by 3 publications

References 33 publications

Acidic residue modifications restore chaperone activity of β-casein interacting with lysozyme

Acidic residue modifications restore chaperone activity of β-casein interacting with lysozyme

Covalent Protein Labeling at Glutamic Acids

Molecular dynamic simulations of nanomechanic chaperone peptide and effects of in silico His mutations on nanostructured function

Contact Info

Product

Resources

About