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Binding of 7-methoxy-4-(aminomethyl)-coumarin to wild-type and W128F mutant cytochrome P450 2D6 studied by time-resolved fluorescence spectroscopy.
Biochem J. 2006 Feb 01; 393(Pt 3):635-43.BJ

Abstract

Enzyme structure and dynamics may play a main role in substrate binding and the subsequent steps in the CYP (cytochrome P450) catalytic cycle. In the present study, changes in the structure of human CYP2D6 upon binding of the substrate are studied using steady-state and time-resolved fluorescence methods, focusing not only on the emission of the tryptophan residues, but also on emission of the substrate. As a substrate, MAMC [7-methoxy-4-(aminomethyl)-coumarin] was selected, a compound exhibiting native fluorescence. As well as the wild-type, the W128F (Trp128-->Phe) mutant of CYP2D6 was studied. After binding, a variety of energy transfer possibilities exist, and molecular dynamics simulations were performed to calculate distances and relative orientations of donors and acceptors. Energy transfer from Trp128 to haem appeared to be important; its emission was related to the shortest of the three average tryptophan fluorescence lifetimes observed for CYP2D6. MAMC to haem energy transfer was very efficient as well: when bound in the active site, the emission of MAMC was fully quenched. Steady-state anisotropy revealed that besides the MAMC in the active site, another 2.4% of MAMC was bound outside of the active site to wild-type CYP2D6. The tryptophan residues in CYP2D6 appeared to be less accessible for the external quenchers iodide and acrylamide in presence of MAMC, indicating a tightening of the enzyme structure upon substrate binding. However, the changes in the overall enzyme structure were not very large, since the emission characteristics of the enzyme were not very different in the presence of MAMC.

Authors+Show Affiliations

Laser Centre VU, Department of Analytical Chemistry and Applied Spectroscopy, Vrije Universiteit, De Boelelaan 1083, 1081 HV Amsterdam, The Netherlands.No affiliation info availableNo affiliation info availableNo affiliation info availableNo affiliation info availableNo affiliation info availableNo affiliation info availableNo affiliation info availableNo affiliation info available

Pub Type(s)

Journal Article

Language

eng

PubMed ID

16190863

Citation

Stortelder, Aike, et al. "Binding of 7-methoxy-4-(aminomethyl)-coumarin to Wild-type and W128F Mutant Cytochrome P450 2D6 Studied By Time-resolved Fluorescence Spectroscopy." The Biochemical Journal, vol. 393, no. Pt 3, 2006, pp. 635-43.
Stortelder A, Keizers PH, Oostenbrink C, et al. Binding of 7-methoxy-4-(aminomethyl)-coumarin to wild-type and W128F mutant cytochrome P450 2D6 studied by time-resolved fluorescence spectroscopy. Biochem J. 2006;393(Pt 3):635-43.
Stortelder, A., Keizers, P. H., Oostenbrink, C., De Graaf, C., De Kruijf, P., Vermeulen, N. P., Gooijer, C., Commandeur, J. N., & Van der Zwan, G. (2006). Binding of 7-methoxy-4-(aminomethyl)-coumarin to wild-type and W128F mutant cytochrome P450 2D6 studied by time-resolved fluorescence spectroscopy. The Biochemical Journal, 393(Pt 3), 635-43.
Stortelder A, et al. Binding of 7-methoxy-4-(aminomethyl)-coumarin to Wild-type and W128F Mutant Cytochrome P450 2D6 Studied By Time-resolved Fluorescence Spectroscopy. Biochem J. 2006 Feb 1;393(Pt 3):635-43. PubMed PMID: 16190863.
* Article titles in AMA citation format should be in sentence-case
TY - JOUR T1 - Binding of 7-methoxy-4-(aminomethyl)-coumarin to wild-type and W128F mutant cytochrome P450 2D6 studied by time-resolved fluorescence spectroscopy. AU - Stortelder,Aike, AU - Keizers,Peter H J, AU - Oostenbrink,Chris, AU - De Graaf,Chris, AU - De Kruijf,Petra, AU - Vermeulen,Nico P E, AU - Gooijer,Cees, AU - Commandeur,Jan N M, AU - Van der Zwan,Gert, PY - 2005/9/30/pubmed PY - 2006/3/25/medline PY - 2005/9/30/entrez SP - 635 EP - 43 JF - The Biochemical journal JO - Biochem J VL - 393 IS - Pt 3 N2 - Enzyme structure and dynamics may play a main role in substrate binding and the subsequent steps in the CYP (cytochrome P450) catalytic cycle. In the present study, changes in the structure of human CYP2D6 upon binding of the substrate are studied using steady-state and time-resolved fluorescence methods, focusing not only on the emission of the tryptophan residues, but also on emission of the substrate. As a substrate, MAMC [7-methoxy-4-(aminomethyl)-coumarin] was selected, a compound exhibiting native fluorescence. As well as the wild-type, the W128F (Trp128-->Phe) mutant of CYP2D6 was studied. After binding, a variety of energy transfer possibilities exist, and molecular dynamics simulations were performed to calculate distances and relative orientations of donors and acceptors. Energy transfer from Trp128 to haem appeared to be important; its emission was related to the shortest of the three average tryptophan fluorescence lifetimes observed for CYP2D6. MAMC to haem energy transfer was very efficient as well: when bound in the active site, the emission of MAMC was fully quenched. Steady-state anisotropy revealed that besides the MAMC in the active site, another 2.4% of MAMC was bound outside of the active site to wild-type CYP2D6. The tryptophan residues in CYP2D6 appeared to be less accessible for the external quenchers iodide and acrylamide in presence of MAMC, indicating a tightening of the enzyme structure upon substrate binding. However, the changes in the overall enzyme structure were not very large, since the emission characteristics of the enzyme were not very different in the presence of MAMC. SN - 1470-8728 UR - https://www.unboundmedicine.com/medline/citation/16190863/Binding_of_7_methoxy_4__aminomethyl__coumarin_to_wild_type_and_W128F_mutant_cytochrome_P450_2D6_studied_by_time_resolved_fluorescence_spectroscopy_ L2 - https://portlandpress.com/biochemj/article-lookup/doi/10.1042/BJ20051169 DB - PRIME DP - Unbound Medicine ER -