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Photothermal release of single-stranded DNA from the surface of gold nanoparticles through controlled denaturating and Au-S bond breaking

机译:通过受控的变性和Au-S键断裂从金纳米颗粒表面光热释放单链DNA

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Photothermal release of DNA from gold nanoparticles either by thermolysis of the Au-S bonds used to anchor the oligonucleotides to the nanoparticle or by thermal denaturation has great therapeutic potential, however, both processes have limitations (a decreased particle stability for the former process and a prohibitively slow rate of release for the latter). Here we show that these two mechanisms are not mutually exclusive and can be controlled by adjusting laser power and ionic strength. We show this using two different double-stranded (ds)DNA-nanoparticle conjugates, in which either the anchored sense strand or the complementary antisense strand was labeled with a fluorescent marker. The amounts of release due to the two mechanisms were evaluated using fluorescence spectroscopy and capillary electrophoresis, which showed that irradiation of the decorated particles in 200 mM NaOAc containing 10 mM Mg(OAc)_2 with a pulsed 532 nm laser operating at 100 mW favors denaturation over Au-S cleavage to an extent of more than six-to-one. Due to the use of a pulsed laser, the process occurs on the order of minutes rather than hours, which is typical for continuous wave lasers. These findings encourage continued research toward developing photothermal gene therapeutics.
机译:通过热分解用于将寡核苷酸固定在纳米颗粒上的Au-S键或通过热变性从金纳米颗粒中光热释放DNA具有巨大的治疗潜力,但是,这两种方法都有局限性(前一种方法的颗粒稳定性降低,并且后者的释放速度太慢了)。在这里,我们表明这两种机制不是互相排斥的,可以通过调节激光功率和离子强度来控制。我们使用两种不同的双链(ds)DNA-纳米粒子偶联物显示了这一点,其中锚定的有义链或互补的反义链都用荧光标记物标记。使用荧光光谱法和毛细管电泳法评估了由于两种机理引起的释放量,结果表明,用100 mW脉冲532 nm激光在200 mM含10 mM Mg(OAc)_2的NaOAc中照射装饰颗粒有助于变性。 Au-S裂解的比例超过六比一。由于使用了脉冲激光,该过程发生的时间大约是几分钟而不是几个小时,这对于连续波激光器来说是典型的。这些发现鼓励继续进行研究以开发光热基因疗法。

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