Retro operation on the Trp-cage miniprotein sequence produces an unstructured molecule capable of folding similar to the original only upon 2,2,2-trifluoroethanol addition

Vymětal, Jiří; Bathula, S. R.; Černý, Jiří; Chaloupková, R.; Žídek, L.; Sklenář, V.; Vondrášek, Jiří

doi:https://dx.doi.org/10.1093/protein/gzu046

Počet záznamů: 1

Retro operation on the Trp-cage miniprotein sequence produces an unstructured molecule capable of folding similar to the original only upon 2,2,2-trifluoroethanol addition

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SYSNO ASEP	0438291
Druh ASEP	J - Článek v odborném periodiku
Zařazení RIV	J - Článek v odborném periodiku
Poddruh J	Článek ve WOS
Název	Retro operation on the Trp-cage miniprotein sequence produces an unstructured molecule capable of folding similar to the original only upon 2,2,2-trifluoroethanol addition
Tvůrce(i)	Vymětal, Jiří (UOCHB-X)_{RID, ORCID} Bathula, S. R. (CZ) Černý, Jiří (BTO-N)_{RID, ORCID} Chaloupková, R. (CZ) Žídek, L. (CZ) Sklenář, V. (CZ) Vondrášek, Jiří (UOCHB-X)_{RID, ORCID}
Celkový počet autorů	7
Zdroj.dok.	Protein Engineering Design and Selection - ISSN 1741-0126 Roč. 27, č. 12 (2014), s. 463-472
Poč.str.	10 s.
Jazyk dok.	eng - angličtina
Země vyd.	GB - Velká Británie
Klíč. slova	protein folding ; protein-structure prediction ; molecular dynamics ; NMR methods ; CD spectroscopy
Vědní obor RIV	CE - Biochemie
CEP	LH11020 GA MŠMT - Ministerstvo školství, mládeže a tělovýchovy
	GA203/08/0114 GA ČR - Grantová agentura ČR
Institucionální podpora	UOCHB-X - RVO:61388963 ; BTO-N - RVO:86652036
UT WOS	000345837300001
DOI	https://doi.org/10.1093/protein/gzu046
Anotace	Amino acid sequence and environment are the most important factors determining the structure, stability and dynamics of proteins. To evaluate their roles in the process of folding, we studied a retroversion of the well-described Trp-cage miniprotein in water and 2,2,2-trifluoroethanol (TFE) solution. We show, by circular dichroism spectroscopy and nuclear magnetic resonance (NMR) measurement, that the molecule has no stable structure under conditions in which the Trp-cage is folded. A detectable stable structure of the retro Trp-cage, with the architecture similar to that of the original Trp-cage, is established only upon addition of TFE to 30% of the total solvent volume. The retro Trp-cage structure shows a completely different pattern of stabilizing contacts between amino acid residues, involving the guanidinium group of arginine and the aromatic group of tryptophan. The commonly used online prediction methods for protein and peptide structures Robetta and PEP-FOLD failed to predict that the retro Trp-cage is unstructured under default prediction conditions. On the other hand, both methods provided structures with a fold similar to those of the experimentally determined NMR structure in water/TFE but with different contacts between amino acids.
Pracoviště	Ústav organické chemie a biochemie
Kontakt	asep@uochb.cas.cz ; Kateřina Šperková, Tel.: 232 002 584 ; Jana Procházková, Tel.: 220 183 418
Rok sběru	2015

Počet záznamů: 1