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首页> 外文期刊>Analytical and bioanalytical chemistry >Molecular beacon-based fluorescence biosensor for the detection of gene fragment and PCR amplification products related to chronic myelogenous leukemia
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Molecular beacon-based fluorescence biosensor for the detection of gene fragment and PCR amplification products related to chronic myelogenous leukemia

机译:基于分子信标的荧光生物传感器,用于检测与慢性粒细胞性白血病相关的基因片段和PCR扩增产物

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摘要

A novel fluorescence method has been established for the determination of gene fragment and PCR amplification products related to chronic myelogenous leukemia (CML). A molecular beacon (MB) which comprises a DNA loop section, a pair of fluorophore (tetramethoxyl rhodamine, TAMRA), and a quencher (4-(2-methyl-on-amino-azobenzene) benzoate, DABCYL) was designed. The loop sequence of MB was designed according to the DNA sequence relating to CML (type b3a2) which contained a single-stranded oligonucleotide. Before hybridization, the fluorescence from the TAMRA had been quenched by the DABCYL. After hybridization with the complementary DNA, the quencher will become far away from the TAMRA, and the fluorescence intensity detected will increase. Changes in the fluorescence intensity have a linear relationship with the concentration of complementary DNA (C) in the range of 4.0∈×∈10 ~(-9)-3.2∈×∈10 ~(-8) mol/L, with a correlation coefficient of 0.9973; the detection limit was 6.0∈×∈10 ~(-10) mol/L (S/N∈=∈3). The developed method has high selectivity, which can be used to discriminate single-base mismatch sequence. The method has been applied to detect the short-stranded CML DNA fragment (278 bp) with high sensitivity. This approach is a promising method for the detection of CML in real samples for medical diagnostics.
机译:建立了一种新型的荧光方法,用于测定与慢性粒细胞性白血病(CML)相关的基因片段和PCR扩增产物。设计了分子信标(MB),其包含DNA环部分,一对荧光团(四甲氧基罗丹明,TAMRA)和淬灭剂(4-(2-甲基-氨基-偶氮苯)苯甲酸酯,DABCYL)。 MB的环序列是根据与CML(b3a2型)相关的DNA序列设计的,该序列包含单链寡核苷酸。在杂交之前,来自TAMRA的荧光已被DABCYL淬灭。与互补DNA杂交后,淬灭剂将远离TAMRA,并且检测到的荧光强度将增加。荧光强度的变化与互补DNA(C)的浓度在4.0∈×∈10〜(-9)-3.2∈×∈10〜(-8)mol / L范围内呈线性关系,具有相关性系数0.9973;检出限为6.0∈×∈10〜(-10)mol / L(S /N∈=∈3)。所开发的方法具有很高的选择性,可用于区分单碱基错配序列。该方法已用于高灵敏度检测短链CML DNA片段(278 bp)。该方法是用于医学诊断中实际样品中CML检测的有前途的方法。

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