Hauptseite > Publikationsdatenbank > A thermostable flavin-based fluorescent protein from Chloroflexus aggregans : a framework for ultra-high resolution structural studies
 
Journal Article FZJ-2019-05390
http://join2-wiki.gsi.de/foswiki/pub/Main/Artwork/join2_logo100x88.png
A thermostable flavin-based fluorescent protein from Chloroflexus aggregans : a framework for ultra-high resolution structural studies

 ;  ;  ;  ;  ;  ;  ;  ;  ;  ;  ;  ;  ;  ;  ;  ;  ;

2019
Royal Society of Chemistry Cambridge

Photochemical & photobiological sciences 18(7), 1793 - 1805 () [10.1039/C9PP00067D]

This record in other databases:      

Please use a persistent id in citations:   doi:

Abstract: Light-Oxygen-Voltage (LOV) domains are conserved parts of photoreceptors in plants, bacteria and fungi that bind flavins as chromophores and detect blue light. In the past, LOV domain variants have been developed as fluorescent reporter proteins (called flavin-based fluorescent proteins; FbFPs), which due to their ability to fluoresce under anaerobic conditions, fast folding kinetics and a small size of ∼12–16 kDa are a promising reporter system for quantitative real-time analysis of biological processes. Here, we present a small thermostable flavin-based fluorescent protein CagFbFP derived from a soluble LOV domain-containing histidine kinase from the thermophilic bacterium Chloroflexus aggregans. CagFbFP is composed of 107 amino acids with a molecular weight of 11.6 kDa and consists only of the conserved LOV core domain. The protein is thermostable with a melting point of about 68 °C. It crystallizes easily and its crystals diffract to 1.07 Å. Both the crystal structure and small angle scattering data show that the protein is a dimer. Unexpectedly, glutamine 148, which in LOV photoreceptor proteins is the key residue responsible for signal transduction, occupies two conformations. Molecular dynamics simulations show that the two conformations interconvert rapidly. The crystal structure of the wild-type Chloroflexus aggregans LOV domain determined at 1.22 Å resolution confirmed the presence of two alternative conformations of the glutamine 148 side chain. Overall, this protein, due to its stability and ease of crystallization, appears to be a promising model for ultra-high resolution structural studies of LOV domains and for application as a fluorescent reporter.

Classification:
Contributing Institute(s):
  1. Institut für Molekulare Enzymtechnologie (HHUD) (IMET)
  2. Strukturbiochemie (ICS-6)
  3. Biotechnologie (IBG-1)
Research Program(s):
  1. 581 - Biotechnology (POF3-581) (POF3-581)

Appears in the scientific report 2019
Database coverage:
Medline ; Embargoed OpenAccess ; Allianz-Lizenz / DFG ; BIOSIS Previews ; Clarivate Analytics Master Journal List ; Current Contents - Physical, Chemical and Earth Sciences ; Ebsco Academic Search ; IF < 5 ; JCR ; NCBI Molecular Biology Database ; National-Konsortium ; NationallizenzNationallizenz ; SCOPUS ; Science Citation Index ; Science Citation Index Expanded ; Web of Science Core Collection
Click to display QR Code for this record

The record appears in these collections:
Dokumenttypen > Aufsätze > Zeitschriftenaufsätze
Institutssammlungen > IBI > IBI-7
Institutssammlungen > IBG > IBG-1
Workflowsammlungen > Öffentliche Einträge
Institutssammlungen > IMET
ICS > ICS-6
Publikationsdatenbank
Open Access
 Datensatz erzeugt am 2019-11-08, letzte Änderung am 2021-01-30
Ähnliche Datensätze


Published on 2019-05-01. Available in OpenAccess from 2020-05-01.:
Volltext herunterladen PDF Volltext herunterladen PDF (PDFA)
(zusätzliche Dateien)
Externer link:
Volltext herunterladenFulltext by OpenAccess repository
Dieses Dokument bewerten:

Rate this document:
1
2
3
4
5
 
(Bisher nicht rezensiert)
JuSER :: Suchen :: Absenden :: Personalisieren :: Hilfe
Powered by Invenio v1.1.7 | join2_v2508-8-g6303aad
Verwaltet von juser@fz-juelich.de

Impressum | Data Privacy Policy
Diese Seite gibt es auch in den folgenden Sprachen:
Deutsch  English