Functional peptide microarrays for specific and sensitive antibody diagnostics

被引:53
|
作者
Andresen, H
Grötzinger, C
Zarse, K
Kreuzer, OJ
Ehrentreich-Förster, E
Bier, FF
机构
[1] Fraunhofer Inst Biomed Engn, Dept Mol Bioanalyt & Bioelect, D-14558 Potsdam Nuthetal, Germany
[2] Peptides&elephants GmbH, Potsdam Nuthetal, Germany
[3] Charite Univ Med Berlin, Dept Gastroenterol & Hepatol, Berlin, Germany
[4] Univ Potsdam, Inst Biochem & Biol, Potsdam, Germany
关键词
antibody; microspot immunoassay; on-chip epitope mapping; peptide microarray; site-specific immobilization;
D O I
10.1002/pmic.200500343
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
Peptide microarrays displaying biologically active small synthetic peptides in a high-density format provide an attractive technology to probe complex samples for the presence and/or function of protein analytes. We present a new approach for manufacturing functional peptide microarrays for molecular immune diagnostics. Our method relies on the efficiency of site-specific solution-phase coupling of biotinylated synthetic peptides to NeutrAvidin (NA) and localized microdispensing of peptide-NA-complexes onto activated glass surfaces. Antibodies are captured in a sandwich manner between surface immobilized peptide probes and fluorescence-labeled secondary antibodies. Our work includes a total of 54 peptides derived from immunodominant linear epitopes of the T7 phage capsid protein, Herpes simplex virus glycoprotein D, c-myc protein, and three domains of the Human coronavirus polymerase polyprotein and their cognate mAbs. By using spacer molecules of different type and length for NA-mediated peptide presentation, we show that the incorporation of a minimum spacer length is imperative for antibody binding, whereas the peptide immobilization direction has only secondary importance for antibody affinity and binding. We further demonstrate that the peptide array is capable of detecting low-picomolar concentrations of mAbs in buffered solutions and diluted human serum with high specificity.
引用
收藏
页码:1376 / 1384
页数:9
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