Publication:

Contrasting the excited-state dynamics of the photoactive yellow protein chromophore: Protein versus solvent environments

cris.lastimport.scopus

2025-06-03T18:14:22Z

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2024-08-02T08:25:31Z

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80587

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PH-SB

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ISIC

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SB

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EPFL

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161474

cris.virtual.sciperId

122830

cris.virtual.unitId

10862

cris.virtual.unitManager

Dyson, Paul Joseph

cris.virtual.unitManager

Cramer, Nicolai

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36bfab9f-a1c3-4afa-aba6-e644fcc4b202

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36bfab9f-a1c3-4afa-aba6-e644fcc4b202

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88c8659d-7346-49fc-8051-42deb18c4f3b

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a8b46ec9-d7ff-4557-a462-2837a43a00d2

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36bfab9f-a1c3-4afa-aba6-e644fcc4b202

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88c8659d-7346-49fc-8051-42deb18c4f3b

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36bfab9f-a1c3-4afa-aba6-e644fcc4b202

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88c8659d-7346-49fc-8051-42deb18c4f3b

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datacite.rights

metadata-only

dc.contributor.author

Vengris, Mikas

dc.contributor.author

van der Horst, Michael A.

dc.contributor.author

Zgrablic, Goran

dc.contributor.author

van Stokkum, Ivo H. M.

dc.contributor.author

Haacke, Stefan

dc.contributor.author

Chergui, Majed

dc.contributor.author

Hellingwerf, Klaas J.

dc.contributor.author

van Grondelle, Rienk

dc.contributor.author

Larsen, Delmar S.

dc.date.accessioned

2006-02-27T10:18:07

dc.date.available

2006-02-27T10:18:07

dc.date.created

2006-02-27

dc.date.issued

2004

dc.date.modified

2025-04-30T12:08:55.821874Z

dc.description.abstract

Wavelength- and time-resolved fluorescence expts. have been performed on the photoactive yellow protein, the E46Q mutant, the hybrids of these proteins contg. a nonisomerizing "locked" chromophore, and the native and locked chromophores in aq. soln. The ultrafast dynamics of these six systems is compared and spectral signatures of isomerization and solvation are discussed. We find that the ultrafast red-shifting of fluorescence is assocd. mostly with solvation dynamics, whereas isomerization manifests itself as quenching of fluorescence. The obsd. multiexponential quenching of the protein samples differs from the single-exponential lifetimes of the chromophores in soln. The locked chromophore in the protein environment decays faster than in soln. This is due to addnl. channels of excited-state energy dissipation via the covalent and hydrogen bonds with the protein environment. The obsd. large dispersion of quenching timescales obsd. in the protein samples that contain the native pigment favors both an inhomogeneous model and an excited-state barrier for isomerization. [on SciFinder (R)]

dc.description.sponsorship

LSU

dc.identifier.dar

5573

dc.identifier.doi

10.1529/biophysj.104.043224

dc.identifier.isi

WOS:000223668500042

dc.identifier.uri

https://infoscience.epfl.ch/handle/20.500.14299/225834

dc.relation.journal

Biophysical Journal

dc.title

Contrasting the excited-state dynamics of the photoactive yellow protein chromophore: Protein versus solvent environments

dc.type

text::journal::journal article::research article

dspace.entity.type

Publication

dspace.legacy.oai-identifier

oai:infoscience.tind.io:80587

epfl.legacy.itemtype

Journal Articles

epfl.legacy.submissionform

ARTICLE

epfl.oai.currentset

SB

epfl.oai.currentset

OpenAIREv4

epfl.oai.currentset

article

epfl.peerreviewed

REVIEWED

epfl.publication.version

http://purl.org/coar/version/c_970fb48d4fbd8a85

epfl.writtenAt

EPFL

oaire.citation.endPage

1857

oaire.citation.issue

3

oaire.citation.startPage

1848

oaire.citation.volume

87

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