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Synergistic effect of orientation and lateral spacing of protein G on an on-chip immunoassay

  • Eung Sam Kim
  • , Chang Kyoon Shim
  • , Jae W. Lee
  • , Joon Won Park
  • , Kwan Yong Choi
  • Pohang University of Science and Technology

Research output: Contribution to journalArticlepeer-review

23 Scopus citations

Abstract

The proper orientation and lateral spacing of antibody molecules are a crucial element for an on-chip immunoassay in which the antibody or its antigen-binding fragments are immobilized on a solid surface. We covalently immobilized a modified protein G (Cys-protein G: protein G with only an N-terminal cysteine) on a dendron-coated surface to control its orientation and lateral spacing simultaneously. The cysteine-specific immobilization of Cys-protein G through the N-terminal cysteine resulted in 2.2-fold higher binding efficiency of Cys-protein G to IgG2a capture antibody than its random immobilization via lysine residues. The lateral spacing of 3.2 nm due to the surface modification with the 9-acid dendron molecule contributed to a 1.5-fold increase in the antibody-binding ability of Cys-protein G. Topographic images of atomic force microscopy exhibited a uniform coverage of Cys-protein G molecules immobilized on the thiol-reactive 9-acid dendron surface and homogeneous distribution of antibody bound to Cys-protein G. In the sandwich immunoassay, the control of the orientation of Cys-protein G led to 10-fold higher detection capability for rIL-2 compared with the randomly oriented protein G. The synergistic advantage of the unidirectional orientation and homogeneous lateral spacing of Cys-protein Gs on the dendron-coated surface can be applied to the development of more sensitive and reproducible antibody microarrays.

Original languageEnglish
Pages (from-to)2421-2430
Number of pages10
JournalAnalyst
Volume137
Issue number10
DOIs
StatePublished - May 21 2012

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