dc.contributor.author
Daublebsky von Eichhain, Mareike
dc.date.accessioned
2018-06-07T23:25:18Z
dc.date.available
2000-12-14T00:00:00.649Z
dc.identifier.uri
https://refubium.fu-berlin.de/handle/fub188/10466
dc.identifier.uri
http://dx.doi.org/10.17169/refubium-14664
dc.description
Die komplette Dissertation im :
diss.pdf
dc.description.abstract
Membrane fusion is an important property of biological systems in general and
has been the subject of many investigations. Influenza hemagglutinin (HA) is
often used as a model system for these studies. For this reason HA was chosen
as a target for a His-Tag introduction by recombinant DNA technologies for use
as a step in protein purification. The refinement and simplification of HA
purification has potential value, not only in the general study of membrane
fusion, but also in the equally important use in different medical
applications, such as highly fusogenic liposomes for drug targeting.
Six histidine residues were introduced into the HA protein by DNA mutagenesis
of the HA gene of A/FPV/Rostock/34, which codes for the wildtype HA protein
(HAwt) of 545 amino acids. Amino acids 198-203, situated in the global head
region of HA, were changed into histidine residues. This location of a His-Tag
within the protein is unusual since it is in contrast to the typical terminal
placement of a His-Tag.
The genes of HAwt and HA-His were expressed in insect cells
(Baculovirussystem), as well as in mammalian cells
(Vaccinia-T7-Expressionsystem). In all tests, HA-His was compared to HAwt.
Both proteins were characterized using several criteria in order to ensure
that the integrity of HA-His was not different to that of HAwt. Neither the
glycosylation nor the trimerisation of HAwt and HA-His showed any difference.
Receptor binding and induction of membrane fusion for both proteins were also
identical.
HA-His was purified by using affinity chromatography on a Ni-NTA-Agarose
column, which selectively binds proteins that contain stretches of histidine
residues. The conditions for this purification were optimized so that HA-His
from the starting membranes could be concentrated.
The results of this study show that addition of a His-Tag within the exposed
head region of the HA protein has no influence on the biochemical or
functional characteristics that were examined in this study. In addition, it
was shown that purification of a protein by metal ion affinity chromatography
is possible even with the untypical internal placement of a His-Tag within the
amino acid sequence.
en
dc.rights.uri
http://www.fu-berlin.de/sites/refubium/rechtliches/Nutzungsbedingungen
dc.subject
haemagglutinins
dc.subject
viral-proteins
dc.subject.ddc
600 Technik, Medizin, angewandte Wissenschaften::630 Landwirtschaft::630 Landwirtschaft und verwandte Bereiche
dc.title
Untersuchungen zur Anreicherung von Influenza Hämagglutinin mit einer
Hexahistidinsequenz durch Affinitätschromatographie
dc.contributor.firstReferee
Univ.-Prof. Dr. Michael F.G. Schmidt
dc.contributor.furtherReferee
Univ.-Prof. Dr. Hans-Jörg Risse
dc.date.accepted
1997-11-28
dc.date.embargoEnd
2001-01-15
dc.identifier.urn
urn:nbn:de:kobv:188-1998000401
dc.title.translated
Investigations on the enrichment of a histagged Influenza Hemagglutinin using
affinity chromatography
en
refubium.affiliation
Veterinärmedizin
de
refubium.mycore.fudocsId
FUDISS_thesis_000000000012
refubium.mycore.transfer
http://www.diss.fu-berlin.de/1998/40/
refubium.mycore.derivateId
FUDISS_derivate_000000000012
dcterms.accessRights.dnb
free
dcterms.accessRights.openaire
open access
