Alvandi Ehsan, Koohdani Fariba
Diabetes Research Center, Endocrinology and Metabolism Clinical Sciences Institute, Tehran University of Medical Sciences, Tehran, Iran.
J Diabetes Metab Disord. 2014 Feb 4;13(1):26. doi: 10.1186/2251-6581-13-26.
TaqMan genotyping with real-time PCR is a reliable method for single nucleotide polymorphism detection, which is done by probes. These oligonucleotides should be short enough to avoid mismatch hybridization, as well as having 5-10°C higher melting temperature than the primers of real-time PCR reaction. One approach for these qualities is to conjugate the probe with minor groove binder (MGB). Having no access to MGB probes, we searched for an alternative. In the current study, we used Zip Nucleic Acids (ZNA) as probes to increase its stability and melting temperature. Our aim was to genotype the -265 T/C changes of Apolipoprotein A-2 gene. We set up the real-time PCR reaction with ZNA probes, and by repeating the reactions, we confirmed the reliability of this new approach. It is now recommended to use ZNA probes, as an alternative to MGB probes, to increase the probe Tm value and its binding to target DNA.
使用实时荧光定量PCR的TaqMan基因分型是一种通过探针进行单核苷酸多态性检测的可靠方法。这些寡核苷酸应足够短以避免错配杂交,并且其解链温度应比实时荧光定量PCR反应的引物高5-10°C。实现这些特性的一种方法是将探针与小沟结合物(MGB)缀合。由于无法获得MGB探针,我们寻找了一种替代方法。在本研究中,我们使用Zip核酸(ZNA)作为探针来提高其稳定性和解链温度。我们的目的是对载脂蛋白A-2基因的-265 T/C变化进行基因分型。我们用ZNA探针建立了实时荧光定量PCR反应,并通过重复反应,证实了这种新方法的可靠性。现在建议使用ZNA探针作为MGB探针的替代品,以提高探针Tm值及其与靶DNA的结合。
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