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Amplified Chemiluminescence Surface Detection of DNA and Telomerase Activity Using Catalytic Nucleic Acid Labels

机译:使用催化核酸标记的DNA和端粒酶活性的化学发光表面放大检测

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摘要

A G-rich nucleic acid sequence binds hemin and yields a biocatalytic complex (DNAzyme) of peroxidase activity, namely, the biocatalyzed generation of chemiluminescence in the presence of H_(2)O_(2) and luminol. The DNAzyme is used as a label for the amplified detection of DNA, or for the analysis of telomerase activity in cancer cells, using chemiluminescence as an output signal. In one configuration, the analyzed DNA is hybridized with a primer nucleic acid that is associated with a Au surface, and the DNAzyme label is hybridized with the surface-confined analyte DNA. The DNA is analyzed with a detection limit of ~1×10~(-9) M. In the second system, telomerase from HeLa cancer cells induces telomerization of a primer associated with a Au surface and the complementary DNAzyme units are hybridized with the telomere to yield the chemiluminescence. The detection limit of the system corresponds to 1000 HeLa cells in the analyzed sample.
机译:富含G的核酸序列与血红素结合,并产生具有过氧化物酶活性的生物催化复合物(DNA酶),即在H_(2)O_(2)和鲁米诺的存在下化学发光的化学催化生成。 DNAzyme用作标记物,用于放大检测DNA,或使用化学发光作为输出信号来分析癌细胞中的端粒酶活性。在一种构型中,将分析的DNA与与Au表面缔合的引物核酸杂交,并且将DNAzyme标记与表面受限的分析物DNA杂交。 DNA的检测限为〜1×10〜(-9)M。在第二种系统中,HeLa癌细胞的端粒酶诱导与Au表面相关的引物的端粒化,互补的DNAzyme单元与端粒杂交产生化学发光。该系统的检出限对应于分析样品中的1000个HeLa细胞。

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