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Effects of oligonucleotide immobilization density on selectivity of quantitative transduction of hybridization of immobilized DNA

机译:寡核苷酸固定化密度对固定化DNA杂交定量转导选择性的影响

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Immobilized single-stranded DNA (ssDNA) can be used as a selective "reagent" to bind complementary nucleic acids for applications including detection of pathogenic organisms and genetic mutations. The density of ssDNA on a surface will determine nearest neighbor interactions, surface interactions, and charge density due to ionizable phosphate groups. This may result in a local ionic strength, pH, and dielectric constant at the surface that is substantially different from that in bulk electrolyte solution. It is the local conditions that influence the thermodynamics of hybridization, and this can be studied by the melt temperature (T-m) of double-stranded DNA (dsDNA). Organosilane chemistry has been used to covalently immobilize hexaethylene glycol linkers and to control the subsequent density of dT(20) that was prepared by automated synthesis. Fiber-optic biosensors based on fused silica optical fibers that were coated with DNA were used in a total internal reflection fluorescence instrument to determine T-m from the dissociation of duplexes of mixtures of fluorescein-labeled and unlabeled dA(20) and d(A(9)GA(10)). Each thermal denaturation of dsDNA at the surface of the optical fibers was accompanied by a 2-3-fold reduction in standard enthalpy Change, relative to values determined for denaturation in bulk solution. The experimental results suggest that the thermodynamic stability of duplexes that are immobilized on a surface is dependent on the density of immobilized DNA. Additionally, the deviation in T-m, arising as a result of the presence of a centrally located single base-pair mismatch was significantly larger for thermal denaturation occurring at the surface of the optical fibers (Delta T-m = 6-10 degrees C) relative to that observed in bulk solution (Delta T-m = 3.8-6.1 degrees C). These results suggest that hybridization at an interface occurs in a significantly different physical environment in comparison to hybridization in bulk solution, and that surface density can be tuned to design analytical figures of merit. [References: 23]
机译:固定的单链DNA(ssDNA)可以用作结合互补核酸的选择性“试剂”,用于包括病原生物和遗传突变检测在内的各种应用。表面上ssDNA的密度将确定由于可电离的磷酸基团而引起的最邻近相互作用,表面相互作用和电荷密度。这可能导致表面的局部离子强度,pH和介电常数与本体电解质溶液中的离子强度,pH和介电常数显着不同。影响杂交热力学的是局部条件,可以通过双链DNA(dsDNA)的解链温度(T-m)进行研究。有机硅烷化学已用于共价固定六甘醇接头,并控制随后通过自动合成制备的dT(20)的密度。在全内反射荧光仪中使用基于涂有DNA的熔融石英光纤的光纤生物传感器,根据荧光素标记的和未标记的dA(20)和d(A(9)混合物的双链体解离确定Tm GA(10))。相对于在本体溶液中确定的变性值,在光纤表面上的dsDNA每次热变性都伴随着标准焓变降低2-3倍。实验结果表明,固定在表面上的双链体的热力学稳定性取决于固定的DNA的密度。此外,由于在光纤表面发生的热变性(ΔTm = 6-10摄氏度),相对于光纤表面发生的热变性,由位于中心的单个碱基对不匹配导致的Tm偏差要大得多。在本体溶液中观察到(ΔTm= 3.8-6.1℃)。这些结果表明,与本体溶液中的杂交相比,界面处的杂交发生在明显不同的物理环境中,并且可以调整表面密度以设计分析品质因数。 [参考:23]

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