Please use this identifier to cite or link to this item: http://hdl.handle.net/1942/23468
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dc.contributor.authorBILLEN, Brecht-
dc.contributor.authorVincke, Cécile-
dc.contributor.authorHANSEN, Rebekka-
dc.contributor.authorDevoogdt, Nick-
dc.contributor.authorMuyldermans, Serge-
dc.contributor.authorADRIAENSENS, Peter-
dc.contributor.authorGUEDENS, Wanda-
dc.date.accessioned2017-04-19T14:07:37Z-
dc.date.available2017-04-19T14:07:37Z-
dc.date.issued2017-
dc.identifier.citationPROTEIN EXPRESSION AND PURIFICATION, 133, p. 25-34-
dc.identifier.issn1046-5928-
dc.identifier.urihttp://hdl.handle.net/1942/23468-
dc.description.abstractSite-specific functionalization of nanobodies after introducing bioorthogonal groups offers the possibility to biofunctionalize surfaces with a uniformly oriented layer of nanobodies. In this paper, expressed protein ligation (EPL) was used for site-specific alkynation of the model nanobody NbBcII10. In contrast to EPL constructs, which are typically expressed in the cytoplasm, nanobodies are expressed in the periplasm where its oxidizing environment ensures a correct folding and disulfide bond formation. Different pathways were explored to express the EPL constructs in the periplasm but simultaneously, the effect of cytoplasmic expression on the functionality of NbBcII10 was also evaluated. By using Escherichia coli SHuffle®T7 cells, it was demonstrated that expression of the EPL complex in the cytoplasm was readily established and that site-specifically mono-alkynated nanobodies can be produced with the same binding properties as the non-modified NbBcII10 expressed in the periplasm. In conclusion, this paper shows that periplasmic expression of the EPL complex is quite challenging, but cytoplasmic expression has proven to be a valuable alternative.-
dc.description.sponsorshipThis research is funded by the FWO project G.0581.12N. The authors gratefully thank Prof. Andre Matagne (Universite de Liege, Belgium) for the BcII antigen, Prof. J-P. Noben and Mr. E. Royackers for the MS measurements, and drs. Ema Romao for the technical assistance during the SPR experiments. We further acknowledge the Hercules Foundation for the project "LC-MS@UHasselt: Linear Trap Quadrupole-Orbitrap mass spectrometer", and the Interreg IV-A project "BioMiMedics" which is financed by the EU and the province of Limburg (Belgium) (EMR INT4-1.2-2010-03/063). We further thank the Interuniversity Attraction Poles programme (P7/05) initiated by the Belgian Science Policy Office (BELSPO).-
dc.language.isoen-
dc.rights© 2017 Elsevier Inc. All rights reserved.-
dc.subject.othernanobodies; expressed protein ligation; periplasmic expression and extraction; click chemistry; CuAAC-
dc.titleCytoplasmic versus periplasmic expression of site-specifically and bioorthogonally functionalized nanobodies using expressed protein ligation-
dc.typeJournal Contribution-
dc.identifier.epage34-
dc.identifier.spage25-
dc.identifier.volume133-
local.bibliographicCitation.jcatA1-
dc.description.notesGuedens, W (reprint author), Hasselt Univ, Inst Mat Res IMO, Biomol Design Grp, BE-3590 Diepenbeek, Belgium. brecht.billen@uhasselt.be; cvincke@vub.ac.be; rebekka.hansen@uhasselt.be; ndevoogd@vub.ac.be; svmuylde@vub.ac.be; peter.adriaensens@uhasselt.be; wanda.guedens@uhasselt.be-
local.type.refereedRefereed-
local.type.specifiedArticle-
dc.identifier.doi10.1016/j.pep.2017.02.009-
dc.identifier.isi000401684400004-
item.validationecoom 2018-
item.contributorBILLEN, Brecht-
item.contributorVincke, Cécile-
item.contributorHANSEN, Rebekka-
item.contributorDevoogdt, Nick-
item.contributorMuyldermans, Serge-
item.contributorADRIAENSENS, Peter-
item.contributorGUEDENS, Wanda-
item.accessRightsOpen Access-
item.fullcitationBILLEN, Brecht; Vincke, Cécile; HANSEN, Rebekka; Devoogdt, Nick; Muyldermans, Serge; ADRIAENSENS, Peter & GUEDENS, Wanda (2017) Cytoplasmic versus periplasmic expression of site-specifically and bioorthogonally functionalized nanobodies using expressed protein ligation. In: PROTEIN EXPRESSION AND PURIFICATION, 133, p. 25-34.-
item.fulltextWith Fulltext-
crisitem.journal.issn1046-5928-
crisitem.journal.eissn1096-0279-
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