Issue 1, 2015
From the journal:

Chemical Science

Diagnosing the miR-141 prostate cancer biomarker using nucleic acid-functionalized CdSe/ZnS QDs and telomerase

Amily Fang-ju Jou,a   Chun-Hua Lu,b   Yen-Chuan Ou,*c   Shian-Shiang Wang,c   Shih-Lan Hsu,d   Itamar Willner*b  and  Ja-an Annie Ho*a  

* Corresponding authors

a BioAnalytical Chemistry and Nanobiomedicine Laboratory, Department of Biochemical Science & Technology, National Taiwan University, Taipei 10617, Taiwan
E-mail: jaho@ntu.edu.tw

b Institute of Chemistry, The Hebrew University of Jerusalem, Jerusalem 91904, Israel
E-mail: willnea@vms.huji.ac.il

c VACRS Division of Urology, Department of Surgery, Taichung Veterans General Hospital, Taichung 40705, Taiwan
E-mail: ycou228@gmail.com

d Department of Education and Research, Taichung Veterans General Hospital, Taichung 40705, Taiwan

Abstract

The microRNA, miR-141, is a promising biomarker for prostate cancer. We implement here a two-step sensing platform for the sensitive detection of miR-141. The first step involves the use of semiconductor CdSe/ZnS quantum dots (QDs) modified by FRET quencher-functionalized nucleic acids, that include the recognition sequence for miR-141 and a telomerase primer sequence for the second step of the analytical platform. Subjecting the probe-modified QDs to miR-141, in the presence of duplex specific nuclease, DSN, leads to the formation of a miR-141/probe duplex and to its DSN-mediated cleavage, while regenerating the miR-141. The DSN-induced cleavage of the quencher units leads to the activation of the fluorescence of the QDs, thus allowing the optical detection of miR-141 with a sensitivity corresponding to 1.0 × 10−12 M. The nucleic acid residues associated with the QDs after cleavage of the probe nucleic acids by DSN act as primers for telomerase. The subsequent telomerase/dNTPs-stimulated elongation of the primer units forms G-quadruplex telomer chains. Incorporation of hemin in the resulting G-quadruplex telomer chains yields horseradish peroxidase-mimicking DNAzyme units, that catalyze the generation of chemiluminescence in the presence of luminol/H2O2. The resulting chemiluminescence intensities provide a readout signal for miR-141, DL = 2.8 × 10−13 M. The first step of the sensing platform is non-selective toward miR-141 and the resulting fluorescence may be considered only as an indicator for the existence of miR-141. The second step in the sensing protocol, involving telomerase, provides a selective chemiluminescence signal for the existence of miR-141. The two-step sensing platform is implemented for the analysis of miR-141 in serum samples from healthy individuals and prostate cancer carriers. Impressive discrimination between healthy individuals and prostate cancer carriers is demonstrated.

Graphical abstract: Diagnosing the miR-141 prostate cancer biomarker using nucleic acid-functionalized CdSe/ZnS QDs and telomerase

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Article information

DOI
https://doi.org/10.1039/C4SC02104E
Article type
Edge Article
Submitted
16 Jul 2014
Accepted
28 Aug 2014
First published
09 Sep 2014
This article is Open Access

All publication charges for this article have been paid for by the Royal Society of Chemistry
Creative Commons BY-NC license

Chem. Sci., 2015,6, 659-665

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Diagnosing the miR-141 prostate cancer biomarker using nucleic acid-functionalized CdSe/ZnS QDs and telomerase

A. F. Jou, C. Lu, Y. Ou, S. Wang, S. Hsu, I. Willner and J. A. Ho, Chem. Sci., 2015, 6, 659 DOI: 10.1039/C4SC02104E

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