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首页> 外文期刊>The Analyst: The Analytical Journal of the Royal Society of Chemistry: A Monthly International Publication Dealing with All Branches of Analytical Chemistry >Isothermal double-cycle catalytic system using DNAzyme and RNase H for the highly selective one-pot detection of oligonucleotides
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Isothermal double-cycle catalytic system using DNAzyme and RNase H for the highly selective one-pot detection of oligonucleotides

机译:等温双循环催化系统使用DNAzyme和RNase H用于寡核苷酸的高选择性单罐检测

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With the use of a double-cycle system involving two catalytic reactions by RNase H and DNAzyme, the signal of oligoDNAs has been specifically amplified in an isothermal mode. The precursor of DNAzyme was introduced to the system as a ring-structured and inactivated form, which involves the 6-nt RNA portion being complementary to target oligoDNA. In the presence of target oligoDNA, the RNA portion forms a DNA/RNA hetero-duplex and is cut by RNase H. This scission converts the precursor to catalytically active DNAzyme, which in turn disconnects the molecular beacon to produce the amplified signal. Because the covalent bonds were disconnected to provide discrete structural changes in both cycles, high sensitivity and specificity are obtained, indicating the strong potential of this double catalytic cycle method for versatile applications.
机译:通过使用RNase H和DNazyme涉及两个催化反应的双循环系统,已经在等温模式下具体放大了oligoDNA的信号。 将DNAzyme的前体作为环状结构和灭活形式引入系统,其涉及与靶oligoDNA互补的6-NT RNA部分。 在靶oligoDNA的存在下,RNA部分形成DNA / RNA杂 - 双链体,并通过RNase H切割。该裂殖将前体转化为催化活性的DNAzyme,其又断开分子信标以产生扩增的信号。 因为在循环中断开共价键以提供离散结构变化,因此获得了高灵敏度和特异性,表明这种双催化循环方法对多功能应用的强势。

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