Multiplexed Detection of Small Analytes by Structure-Switching Aptamer-Based Capillary Electrophoresis

被引:27
作者
Zhu, Zhenyu [1 ]
Ravelet, Corinne [1 ]
Perrier, Sandrine [1 ]
Guieu, Valerie [1 ]
Roy, Beatrice [2 ]
Perigaud, Christian [2 ]
Peyrin, Eric [1 ]
机构
[1] Univ Grenoble 1, CNRS, ICMG FR 2607, UMR 5063,Dept Pharmacochim Mol, F-38402 St Martin Dheres, France
[2] Univ Montpellier 2, CNRS, UMR 5247, Inst Biomol Max Mousseron, Montpellier, France
关键词
LASER-INDUCED FLUORESCENCE; MOLECULAR RECOGNITION; COMPETITIVE-BINDING; DNA SEPARATIONS; IMMUNOASSAY; ASSAY; AMPHIPHILES; ADENOSINE; SENSORS; LENGTH;
D O I
10.1021/ac100755q
中图分类号
O65 [分析化学];
学科分类号
070302 ; 081704 ;
摘要
Affinity probe capillary electrophoresis (APCE) assays, combining the separation power of CE with the specificity of interactions occurring between a target and a molecular recognition element (MRE), have become important analytical tools in many application fields. In this report, a rationalized strategy, derived from the structure-switching aptamer concept, is described for the design of a novel APCE mode dedicated to small molecule detection. Two assay configurations were reported. The first one, developed for the single-analyte determination, was based on the use of a cholesteryl-tagged aptamer (Chol-Apt) as the MRE and its fluorescein-labeled complementary strand (CS*) as the tracer (laser-induced fluorescence detection). Under micellar electrokinetic chromatography (MEKC) conditions, free CS* and the hybrid formed with Choi-Apt (duplex*) were efficiently separated (and then quantified) through the specific shift of the electrophoretic mobility of the cholesteryl-tagged species in the presence of a neutral micellar phase. When the target was introduced into the preincubated sample, the hybridized form was destabilized, resulting in a decrease in the duplex* peak area and a concomitant increase in the free CS* peak area. The second format, especially designed for multianalyte sensing, employed dually cholesteryl- and fluorescein-labeled complementary strands (Chol-CS*) of different lengths and unmodified aptamers (Apt). The size-dependent electrophoretic separation of different Chol-CS* forms from each other and from their corresponding duplexes* was also accomplished under MEKC conditions. The simultaneous detection of multiple analytes in a single capillary was performed by monitoring accurately each target-induced duplex-to-complex change. This method could expand significantly the potential of small solute APCE analysis in terms of simplicity, adaptability, generalizability, and high-throughput analysis capability.
引用
收藏
页码:4613 / 4620
页数:8
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