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@ARTICLE{Fitter:4685,
author = {Fitter, J.},
title = {{T}he perspective of studying multi-domain protein folding},
journal = {Cellular and molecular life sciences},
volume = {66},
issn = {1420-682X},
address = {Basel},
publisher = {Birkhäuser},
reportid = {PreJuSER-4685},
pages = {1672 - 1681},
year = {2009},
note = {Record converted from VDB: 12.11.2012},
abstract = {Most of fundamental studies on protein folding have been
performed with small globular proteins consisting of a
single domain. In vitro many of these proteins are well
characterized by a reversible two-state folding scheme.
However, the majority of proteins in the cell belong to the
class of larger multi-domain proteins that often unfold
irreversibly under in vitro conditions. This makes folding
studies difficult or even impossible. In spite of these
problems for many multi-domain proteins, folding has been
investigated by classical refolding. Co-translational
folding of nascent polypeptide chains when synthesized by
ribosomes has also been studied. Single molecule techniques
represent a promising approach for future studies on the
folding of multi-domain proteins, and tremendous advances
have been made in these techniques in recent years. In
particular, fluorescence-based methods can contribute
significantly to an understanding of the fundamental
principles of multi-domain protein folding.},
keywords = {Animals / Humans / Models, Molecular / Protein Folding /
Protein Structure, Tertiary / Proteins: chemistry /
Spectrometry, Fluorescence / Proteins (NLM Chemicals) / J
(WoSType)},
cin = {ISB-2},
ddc = {570},
cid = {I:(DE-Juel1)ISB-2-20090406},
pnm = {Programm Biosoft},
pid = {G:(DE-Juel1)FUEK443},
shelfmark = {Biochemistry $\&$ Molecular Biology / Cell Biology},
typ = {PUB:(DE-HGF)16},
pubmed = {pmid:19183848},
UT = {WOS:000268003600004},
doi = {10.1007/s00018-009-8771-9},
url = {https://juser.fz-juelich.de/record/4685},
}