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首页> 外文期刊>Mikrochimica Acta: An International Journal for Physical and Chemical Methods of Analysis >The mechanism of the adsorption of dsDNA on citrate-stabilized gold nanoparticles and a colorimetric and visual method for detecting the V600E point mutation of the BRAF gene
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The mechanism of the adsorption of dsDNA on citrate-stabilized gold nanoparticles and a colorimetric and visual method for detecting the V600E point mutation of the BRAF gene

机译:DSDNA对柠檬酸盐稳定金纳米颗粒的吸附机理及比色和视觉方法检测BRAF基因的V600E点突变

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摘要

A study is presented on the binding kinetics and mechanism of the adsorption of dsDNA on citrate-capped gold nanoparticles (AuNPs). Methods include fluorescence titration, isothermal calorimetry (ITC) titration, dynamic light scattering and gel electrophoresis. It is found that the fluorescence of probe DNA (labeled with Rhodamine Green and measured at excitation/emission peaks of 498/531 nm) is quenched by addition of AuNPs. The Stern-Volmer quenching constant (Ksv) is 1.67 x 10^9 L.mol(-1) at 308 K and drops with increasing temperature. The quenching mechanism is mainly static. The results of both fluorescence titrations and ITC show negative values for Delta H and Delta S values. This shows ion-induced dipole-dipole interaction to be the main attractive forces between dsDNA and AuNPs, while electrostatic interactions result in repulsion. The repulsive forces lead to a lower affinity between dsDNA and AuNPs (compared to single-strand DNA). It is also found that dsDNA can prevent the aggregation of AuNPs which is accompanied by a color change from red into blue. The visual detection limit with bare eyes for dsDNA(1) is 36 pM. Based on these findings, a colorimetric method was developed to detect the proto-oncogene of serine/threonine-protein kinase B-Raf V600E point mutation in HT29, Ec109, A549, Huh-7 and SW480 cell lines.
机译:提出了对柠檬酸盐覆盖金纳米颗粒(AUNP)对DSDNA吸附的结合动力学和机理研究。方法包括荧光滴定,等温度量热(ITC)滴定,动态光散射和凝胶电泳。发现探针DNA的荧光(用Rhodamine绿色标记并在498/531nm的激发/发射峰值下测量)通过添加AUNP来淬灭。泰铢淬火常数(KSV)为1.67×10℃,在308 k下为1.67×10℃,温度升高。淬火机制主要是静态的。荧光滴定和ITC的结果显示了Delta H和Delta S值的负值。这显示离子诱导的偶极子 - 偶极子相互作用,成为DSDNA和AUNP之间的主要吸引力,而静电相互作用会导致排斥。排斥力导致DSDNA和AUNPS(与单链DNA相比)较低的亲和力。还发现DSDNA可以防止AUNP的聚集,伴随着从红色变为蓝色的颜色变化。 DSDNA(1)裸眼睛的视觉检测限是36下午。基于这些发现,开发了比色法检测HT29,EC109,A549,HUH-7和SW480细胞系中丝氨酸/苏氨酸 - 蛋白激酶B-RAF V600E点突变的原癌基因。

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