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Titel: Trypsiligase-catalyzed labeling of proteins on living cells
Autor(en): Liebscher, Sandra
Mathea, Sebastian
Aumüller, Tobias
Pech, Andreas
Bordusa, Frank
Erscheinungsdatum: 2021
Art: Artikel
Sprache: Englisch
Zusammenfassung: Fluorescent fusion proteins are powerful tools for studying biological processes in living cells, but universal application is limited due to the voluminous size of those tags, which might have an impact on the folding, localization or even the biological function of the target protein. The designed biocatalyst trypsiligase enables site-directed linkage of small-sized fluorescence dyes on the N terminus of integral target proteins located in the outer membrane of living cells through a stable native peptide bond. The function of the approach was tested by using the examples of covalent derivatization of the transmembrane proteins CD147 as well as the EGF receptor, both presented on human HeLa cells. Specific trypsiligase recognition of the site of linkage was mediated by the dipeptide sequence Arg-His added to the proteins’ native N termini, pointing outside the cell membrane. The labeling procedure takes only about 5 minutes, as demonstrated for couplings of the fluorescence dye tetramethyl rhodamine and the affinity label biotin as well.
URI: https://opendata.uni-halle.de//handle/1981185920/78893
http://dx.doi.org/10.25673/76939
Open-Access: Open-Access-Publikation
Nutzungslizenz: (CC BY-NC-ND 4.0) Creative Commons Namensnennung - Nicht kommerziell - Keine Bearbeitungen 4.0 International(CC BY-NC-ND 4.0) Creative Commons Namensnennung - Nicht kommerziell - Keine Bearbeitungen 4.0 International
Sponsor/Geldgeber: Publikationsfonds MLU
Journal Titel: ChemBioChem
Verlag: Wiley-VCH
Verlagsort: Weinheim
Band: 22
Heft: 7
Originalveröffentlichung: 10.1002/cbic.202000718
Seitenanfang: 1201
Seitenende: 1204
Enthalten in den Sammlungen:Open Access Publikationen der MLU

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