Near-native, site-specific and purification-free protein labeling for quantitative protein interaction analysis by MicroScale Thermophoresis

DC FieldValueLanguage
dc.contributor.authorBartoschik, Tanja
dc.contributor.authorGalinec, Stefanie
dc.contributor.authorKleusch, Christian
dc.contributor.authorWalkiewicz, Katarzyna
dc.contributor.authorBreitsprecher, Dennis
dc.contributor.authorWeigert, Sebastian
dc.contributor.authorMuller, Yves A.
dc.contributor.authorYou, Changjiang
dc.contributor.authorPiehler, Jacob
dc.contributor.authorVercruysse, Thomas
dc.contributor.authorDaelemans, Dirk
dc.contributor.authorTschammer, Nuska
dc.date.accessioned2021-12-23T16:18:38Z-
dc.date.available2021-12-23T16:18:38Z-
dc.date.issued2018
dc.identifier.issn20452322
dc.identifier.urihttps://osnascholar.ub.uni-osnabrueck.de/handle/unios/12780-
dc.description.abstractMicroScale Thermophoresis (MST) is a frequently used method for the quantitative characterization of intermolecular interactions with several advantages over other technologies. One of these is its capability to determine equilibrium constants in solution including complex biological matrices such as cell lysates. MST requires one binding partner to be fluorescent, which is typically achieved by labeling target proteins with a suitable fluorophore. Here, we present a near-native, site-specific in situ labeling strategy for MST experiments that enables reliable measurements in cell lysates and that has distinct advantages over routine covalent labeling techniques. To this end, we exploited the high-affinity interaction of tris-NTA with oligohistidine-tags, which are popular for purification, immobilization or detection of recombinant proteins. We used various DYE-tris-NTA conjugates to successfully label His-tagged proteins that were either purified or a component of cell lysate. The RED-tris-NTA was identified as the optimal dye conjugate with a high affinity towards oligohistidine-tags, a high fluorescence signal and an optimal signal-to-noise ratio in MST binding experiments. Owing to its emission in the red region of the spectrum, it also enables reliable measurements in complex biological matrices such as cell lysates allowing a more physiologically realistic assessment and eliminating the need for protein purification.
dc.language.isoen
dc.publisherNATURE PUBLISHING GROUP
dc.relation.ispartofSCIENTIFIC REPORTS
dc.subjectAFFINITY
dc.subjectAMINO-ACIDS
dc.subjectBINDING
dc.subjectCELLS
dc.subjectDRUG DISCOVERY
dc.subjectHISTIDINE-TAGGED PROTEINS
dc.subjectINHIBITOR
dc.subjectMultidisciplinary Sciences
dc.subjectNONCOVALENT
dc.subjectNUCLEAR EGRESS COMPLEX
dc.subjectScience & Technology - Other Topics
dc.subjectSENSOR CHIP
dc.titleNear-native, site-specific and purification-free protein labeling for quantitative protein interaction analysis by MicroScale Thermophoresis
dc.typejournal article
dc.identifier.doi10.1038/s41598-018-23154-3
dc.identifier.isiISI:000427926500021
dc.description.volume8
dc.contributor.orcid0000-0001-7092-1153
dc.contributor.orcid0000-0002-7839-6397
dc.contributor.orcid0000-0002-8649-777X
dc.contributor.orcid0000-0002-0469-1545
dc.contributor.orcid0000-0003-0519-8928
dc.contributor.orcid0000-0003-2433-3355
dc.contributor.researcheridAAK-8879-2020
dc.contributor.researcheridP-7923-2017
dc.contributor.researcheridL-3901-2014
dc.contributor.researcheridR-5397-2016
dc.contributor.researcheridA-7359-2008
dc.publisher.placeMACMILLAN BUILDING, 4 CRINAN ST, LONDON N1 9XW, ENGLAND
dcterms.isPartOf.abbreviationSci Rep
dcterms.oaStatusgold, Green Published
crisitem.author.deptSonderforschungsbereich 944: Physiologie und Dynamik zellulärer Mikrokompartimente-
crisitem.author.deptFB 05 - Biologie/Chemie-
crisitem.author.deptidorganisation19-
crisitem.author.deptidfb05-
crisitem.author.orcid0000-0002-7839-6397-
crisitem.author.orcid0000-0002-2143-2270-
crisitem.author.parentorgFB 05 - Biologie/Chemie-
crisitem.author.parentorgUniversität Osnabrück-
crisitem.author.grandparentorgUniversität Osnabrück-
crisitem.author.netidYoCh745-
crisitem.author.netidPiJa938-
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