Site-specific and covalent attachment of his-tagged proteins by chelation assisted photoimmobilization : a strategy for microarraying of protein ligands

A novel strategy for site-specific and covalent attachment of proteins has been developed, intended for robust and controllable immobilization of histidine (His)-tagged ligands in protein microarrays. The method is termed chelation assisted photoimmobilization (CAP) and was demonstrated using human...

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Veröffentlicht in:Langmuir : the ACS journal of surfaces and colloids. - 1999. - 29(2013), 37 vom: 17. Sept., Seite 11687-94
1. Verfasser: Ericsson, Emma M (VerfasserIn)
Weitere Verfasser: Enander, Karin, Bui, Lan, Lundström, Ingemar, Konradsson, Peter, Liedberg, Bo
Format: Online-Aufsatz
Sprache:English
Veröffentlicht: 2013
Zugriff auf das übergeordnete Werk:Langmuir : the ACS journal of surfaces and colloids
Schlagworte:Journal Article Research Support, Non-U.S. Gov't Chelating Agents Immunoglobulin Fc Fragments Ligands Histidine 4QD397987E
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520 |a A novel strategy for site-specific and covalent attachment of proteins has been developed, intended for robust and controllable immobilization of histidine (His)-tagged ligands in protein microarrays. The method is termed chelation assisted photoimmobilization (CAP) and was demonstrated using human IgG-Fc modified with C-terminal hexahistidines (His-IgGFc) as the ligand and protein A as the analyte. Alkanethiols terminated with either nitrilotriacetic acid (NTA), benzophenone (BP), or oligo(ethylene glycol) were synthesized and mixed self-assembled monolayers (SAMs) were prepared on gold and thoroughly characterized by infrared reflection absorption spectroscopy (IRAS), ellipsometry, and contact angle goniometry. In the process of CAP, NTA chelates Ni(2+) and the complex coordinates the His-tagged ligand in an oriented assembly. The ligand is then photoimmobilized via BP, which forms covalent bonds upon UV light activation. In the development of affinity biosensors and protein microarrays, site-specific attachment of ligands in a fashion where analyte binding sites are available is often preferred to random coupling. Analyte binding performance of ligands immobilized either by CAP or by standard amine coupling was characterized by surface plasmon resonance in combination with IRAS. The relative analyte response with randomly coupled ligand was 2.5 times higher than when site-specific attachment was used. This is a reminder that also when immobilizing ligands via residues far from the binding site, there are many other factors influencing availability and activity. Still, CAP provides a valuable expansion of protein immobilization techniques since it offers attractive microarraying possibilities amenable to applications within proteomics 
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650 4 |a Research Support, Non-U.S. Gov't 
650 7 |a Chelating Agents  |2 NLM 
650 7 |a Immunoglobulin Fc Fragments  |2 NLM 
650 7 |a Ligands  |2 NLM 
650 7 |a Histidine  |2 NLM 
650 7 |a 4QD397987E  |2 NLM 
700 1 |a Enander, Karin  |e verfasserin  |4 aut 
700 1 |a Bui, Lan  |e verfasserin  |4 aut 
700 1 |a Lundström, Ingemar  |e verfasserin  |4 aut 
700 1 |a Konradsson, Peter  |e verfasserin  |4 aut 
700 1 |a Liedberg, Bo  |e verfasserin  |4 aut 
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