4.8 Article

Cascade Signal Amplification Strategy for Subattomolar Protein Detection by Rolling Circle Amplification and Quantum Dots Tagging

Journal

ANALYTICAL CHEMISTRY
Volume 82, Issue 8, Pages 3337-3342

Publisher

AMER CHEMICAL SOC
DOI: 10.1021/ac100144g

Keywords

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Funding

  1. National Science Funds for Creative Research Groups [20821063]
  2. NSFC [90713015]
  3. National Basic Research Program of China [2010CB732400]
  4. Important National S&T Specific Project of China [20097ZX10004-313]
  5. Department of Health of Jiangsu [RC2007069]
  6. Natural Science Foundation of Jiangsu [BK2008014]

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A cascade signal amplification strategy was proposed for detection of protein target at ultralow concentration by combining the rolling circle amplification (RCA) technique with oligonucleotide functionalized quantum dots (QDs), multiplex binding of the biotin-strepavidin system, and anodic stripping voltammetric detection. The RCA product containing tandem-repeat sequences could serve as excellent template for periodic assembly of QDs, which presented per protein recognition event to numerous quantum dot tags for electrochemical readout. Both the RCA and the multiplex binding system showed remarkable amplification efficiency, very little nonspecific adsorption, and low background signal. Using human vascular endothelial growth factor as a model protein, the designed strategy could quantitatively detect protein down to 16 molecules in a 100 mu L sample with a linear calibration range from 1 aM to 1 pM and was amenable to quantification of protein target in complex biological matrixes. The proposed cascade signal amplification strategy would become a powerful tool for proteomics research and clinical diagnostics.

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