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MeSH: interakční proteinové domény a motivy-fyziologie

3 záznamů v Články Filtry

Článek

structural characterization of the interaction between the C-terminal domain of the influenza polymerase PA subunit and an optimized small peptide inhibitor

Hejdánek, Jakub
Autor Hejdánek, Jakub Institute of Organic Chemistry and Biochemistry of the Czech Academy of Sciences, Gilead Sciences and IOCB Research Center, Flemingovo n. 2, 16610, Prague 6, Czech Republic
Radilová, Kateřina
Autor Radilová, Kateřina Institute of Organic Chemistry and Biochemistry of the Czech Academy of Sciences, Gilead Sciences and IOCB Research Center, Flemingovo n. 2, 16610, Prague 6, Czech Republic First Faculty of Medicine, Charles University, Kateřinská 1660/32, 12108, Prague 2, Czech Republic
Pachl, Petr
Autor Pachl, Petr Institute of Organic Chemistry and Biochemistry of the Czech Academy of Sciences, Gilead Sciences and IOCB Research Center, Flemingovo n. 2, 16610, Prague 6, Czech Republic
Hodek, Jan
Autor Hodek, Jan Institute of Organic Chemistry and Biochemistry of the Czech Academy of Sciences, Gilead Sciences and IOCB Research Center, Flemingovo n. 2, 16610, Prague 6, Czech Republic
Machara, Aleš
Autor Machara, Aleš Institute of Organic Chemistry and Biochemistry of the Czech Academy of Sciences, Gilead Sciences and IOCB Research Center, Flemingovo n. 2, 16610, Prague 6, Czech Republic Department of Organic Chemistry, Faculty of Science, Charles University, Hlavova 8, 12800, Prague 2, Czech Republic
Weber, Jan
Autor Weber, Jan Institute of Organic Chemistry and Biochemistry of the Czech Academy of Sciences, Gilead Sciences and IOCB Research Center, Flemingovo n. 2, 16610, Prague 6, Czech Republic
Řezáčová, Pavlína
Autor Řezáčová, Pavlína Institute of Organic Chemistry and Biochemistry of the Czech Academy of Sciences, Gilead Sciences and IOCB Research Center, Flemingovo n. 2, 16610, Prague 6, Czech Republic Institute of Molecular Genetics of the Czech Academy of Sciences, Vídeňská 1083, 14000, Prague 4, Czech Republic
Konvalinka, Jan
Autor Konvalinka, Jan Institute of Organic Chemistry and Biochemistry of the Czech Academy of Sciences, Gilead Sciences and IOCB Research Center, Flemingovo n. 2, 16610, Prague 6, Czech Republic Department of Biochemistry, Faculty of Science, Charles University, Hlavova 8, 12800, Prague 2, Czech Republic
Kožíšek, Milan
Autor Kožíšek, Milan Institute of Organic Chemistry and Biochemistry of the Czech Academy of Sciences, Gilead Sciences and IOCB Research Center, Flemingovo n. 2, 16610, Prague 6, Czech Republic. Electronic address: milan.kozisek@uochb.cas.cz

Antiviral research. 2021 ; 185 (-) : 104971. [pub] 20201106

Antiviral Res
ISSN 1872-9096
Medvik
Zdroj

Influenza viruses can cause severe respiratory infections in humans, leading to nearly half a million deaths worldwide each year. Improved antiviral drugs are needed to address the threat of development of novel pandemic strains. Current therapeutic interventions target three key proteins in the viral life cycle: neuraminidase, the M2 channel and RNA-dependent-RNA polymerase. Protein-protein interactions between influenza polymerase subunits are potential new targets for drug development. Using a newly developed assay based on AlphaScreen technology, we screened a peptide panel for protein-protein interaction inhibitors to identify a minimal PB1 subunit-derived peptide that retains high inhibition potential and can be further modified. Here, we present an X-ray structure of the resulting decapeptide bound to the C-terminal domain of PA polymerase subunit from pandemic isolate A/California/07/2009 H1N1 at 1.6 Å resolution and discuss its implications for the design of specific, potent influenza polymerase inhibitors.

MeSH
antivirové látky farmakologie MeSH
interakční proteinové domény a motivy účinky léků fyziologie MeSH
krystalizace MeSH
lidé MeSH
RNA-dependentní RNA-polymerasa chemie metabolismus MeSH
vazba proteinů MeSH
virové proteiny antagonisté a inhibitory chemie metabolismus MeSH
virus chřipky A, podtyp H1N1 účinky léků enzymologie metabolismus MeSH
Check Tag
lidé MeSH
Publikační typ
časopisecké články MeSH
práce podpořená grantem MeSH

Článek

An inter-subunit protein-peptide interface that stabilizes the specific activity and oligomerization of the AAA+ chaperone Reptin

Journal of proteomics. 2019 ; 199 (-) : 89-101. [pub] 20190309

J Proteomics
ISSN 1876-7737
Medvik
Zdroj

Reptin is a member of the AAA+ superfamily whose members can exist in equilibrium between monomeric apo forms and ligand bound hexamers. Inter-subunit protein-protein interfaces that stabilize Reptin in its oligomeric state are not well-defined. A self-peptide binding assay identified a protein-peptide interface mapping to an inter-subunit "rim" of the hexamer bridged by Tyrosine-340. A Y340A mutation reduced ADP-dependent oligomer formation using a gel filtration assay, suggesting that Y340 forms a dominant oligomer stabilizing side chain. The monomeric ReptinY340A mutant protein exhibited increased activity to its partner protein AGR2 in an ELISA assay, further suggesting that hexamer formation can preclude certain protein interactions. Hydrogen-deuterium exchange mass spectrometry (HDX-MS) demonstrated that the Y340A mutation attenuated deuterium suppression of Reptin in this motif in the presence of ligand. By contrast, the tyrosine motif of Reptin interacts with a shallower pocket in the hetero-oligomeric structure containing Pontin and HDX-MS revealed no obvious role of the Y340 side chain in stabilizing the Reptin-Pontin oligomer. Molecular dynamic simulations (MDS) rationalized how the Y340A mutation impacts upon a normally stabilizing inter-subunit amino acid contact. MDS also revealed how the D299N mutation can, by contrast, remove oligomer de-stabilizing contacts. These data suggest that the Reptin interactome can be regulated by a ligand dependent equilibrium between monomeric and hexameric forms through a hydrophobic inter-subunit protein-protein interaction motif bridged by Tyrosine-340. SIGNIFICANCE: Discovering dynamic protein-protein interactions is a fundamental aim of research in the life sciences. An emerging view of protein-protein interactions in higher eukaryotes is that they are driven by small linear polypeptide sequences; the linear motif. We report on the use of linear-peptide motif screens to discover a relatively high affinity peptide-protein interaction for the AAA+ and pro-oncogenic protein Reptin. This peptide interaction site was shown to form a 'hot-spot' protein-protein interaction site, and validated to be important for ligand-induced oligomerization of the Reptin protein. These biochemical data provide a foundation to understand how single point mutations in Reptin can impact on its oligomerization and protein-protein interaction landscape.

MeSH
AAA doména * MeSH
ATPázy spojené s různými buněčnými aktivitami chemie metabolismus MeSH
DNA-helikasy chemie metabolismus MeSH
interakční proteinové domény a motivy fyziologie MeSH
lidé MeSH
molekulární chaperony chemie metabolismus MeSH
multimerizace proteinu * MeSH
mutace MeSH
simulace molekulární dynamiky MeSH
transportní proteiny chemie metabolismus MeSH
tyrosin genetika MeSH
Check Tag
lidé MeSH
Publikační typ
časopisecké články MeSH
práce podpořená grantem MeSH

Článek

The Role of Protein-Protein and Protein-Membrane Interactions on P450 Function

Drug metabolism and disposition. 2016 ; 44 (4) : 576-90. [pub] 20160205

Drug Metab Dispos
ISSN 1521-009X
Medvik
Zdroj

This symposium summary, sponsored by the ASPET, was held at Experimental Biology 2015 on March 29, 2015, in Boston, Massachusetts. The symposium focused on: 1) the interactions of cytochrome P450s (P450s) with their redox partners; and 2) the role of the lipid membrane in their orientation and stabilization. Two presentations discussed the interactions of P450s with NADPH-P450 reductase (CPR) and cytochrome b5. First, solution nuclear magnetic resonance was used to compare the protein interactions that facilitated either the hydroxylase or lyase activities of CYP17A1. The lyase interaction was stimulated by the presence of b5 and 17α-hydroxypregnenolone, whereas the hydroxylase reaction was predominant in the absence of b5. The role of b5 was also shown in vivo by selective hepatic knockout of b5 from mice expressing CYP3A4 and CYP2D6; the lack of b5 caused a decrease in the clearance of several substrates. The role of the membrane on P450 orientation was examined using computational methods, showing that the proximal region of the P450 molecule faced the aqueous phase. The distal region, containing the substrate-access channel, was associated with the membrane. The interaction of NADPH-P450 reductase (CPR) with the membrane was also described, showing the ability of CPR to "helicopter" above the membrane. Finally, the endoplasmic reticulum (ER) was shown to be heterogeneous, having ordered membrane regions containing cholesterol and more disordered regions. Interestingly, two closely related P450s, CYP1A1 and CYP1A2, resided in different regions of the ER. The structural characteristics of their localization were examined. These studies emphasize the importance of P450 protein organization to their function.

MeSH
buněčná membrána metabolismus MeSH
endoplazmatické retikulum metabolismus MeSH
interakční proteinové domény a motivy fyziologie MeSH
jaterní mikrozomy metabolismus MeSH
lidé MeSH
sekundární struktura proteinů MeSH
systém (enzymů) cytochromů P-450 chemie fyziologie MeSH
výzkumná zpráva * MeSH
zvířata MeSH
Check Tag
lidé MeSH
zvířata MeSH
Publikační typ
časopisecké články MeSH
práce podpořená grantem MeSH
přehledy MeSH
Research Support, N.I.H., Extramural MeSH

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