Antigen-specific T cell phenotyping microarrays using grating coupled surface plasmon resonance imaging and surface plasmon coupled emission

被引:30
|
作者
Rice, James M. [1 ]
Stern, Lawrence J. [2 ,3 ]
Guignon, Ernest F. [4 ]
Lawrence, David A. [5 ]
Lynes, Michael A. [1 ]
机构
[1] Univ Connecticut, Dept Mol & Cell Biol, Storrs, CT 06269 USA
[2] Univ Massachusetts, Sch Med, Dept Pathol, Worcester, MA 01655 USA
[3] Univ Massachusetts, Sch Med, Dept Biochem & Mol Pharmacol, Worcester, MA 01655 USA
[4] Ciencia Inc, E Hartford, CT 06108 USA
[5] New York State Dept Hlth, Wadsworth Ctr, Albany, NY 12201 USA
来源
BIOSENSORS & BIOELECTRONICS | 2012年 / 31卷 / 01期
关键词
T cell microarray; SPR; SPCE; PERIPHERAL-BLOOD; BINDING; PEPTIDE; IDENTIFICATION; RECOGNITION; PREDICTION; MOLECULES; CYTOMETRY; TETRAMERS; RESPONSES;
D O I
10.1016/j.bios.2011.10.029
中图分类号
Q6 [生物物理学];
学科分类号
071011 ;
摘要
The circulating population of peripheral T lymphocytes obtained from a blood sample can provide a large amount of information about an individual's medical status and history. Recent evidence indicates that the detection and functional characterization of antigen-specific T cell subsets within the circulating population may provide a diagnostic indicator of disease and has the potential to predict an individual's response to therapy. In this report, a microarray detection platform that combines grating-coupled surface plasmon resonance imaging (GCSPRI) and grating-coupled surface plasmon coupled emission (SPCE) fluorescence detection modalities were used to detect and characterize CD4+ T cells. The microspot regions of interest (ROIs) printed on the array consisted of immobilized antibodies or peptide loaded MHC monomers (p/MHC) as T cell capture ligands mixed with additional antibodies as cytokine capture ligands covalently bound to the surface of a corrugated gold sensor chip. Using optimized parameters, an unlabeled influenza peptide reactive T cell clone could be detected at a frequency of 0.1% in a mixed T cell sample using GCSPRI. Additionally, after cell binding was quantified, differential TH1 cytokine secretion patterns from a T cell clone cultured under TH1 or TH2 inducing conditions was detected using an SPCE fluorescence based assay. Differences in the secretion patterns of 3 cytokines, characteristic of the inducing conditions, indicated that differences were a consequence of the functional status of the captured cells. A dual mode GCSPRI/SPCE assay can provide a rapid, high content T cell screening/characterization tool that is useful for diagnosing disease, evaluating vaccination efficacy, or assessing responses to immunotherapeutics. (C) 2011 Elsevier B.V. All rights reserved.
引用
收藏
页码:264 / 269
页数:6
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