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Unzipping and binding of small interfering RNA with single walled carbon nanotube: A platform for small interfering RNA delivery

机译:小干扰RNA与单壁碳纳米管的解链和结合:小干扰RNA传递的平台

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摘要

In an effort to design efficient platform for siRNA delivery, we combine all atom classical and quantum simulations to study the binding of small interfering RNA (siRNA) by pristine single wall carbon nanotube (SWCNT). Our results show that siRNA strongly binds to SWCNT surface via unzipping its base-pairs and the propensity of unzipping increases with the increase in the diameter of the SWCNTs. The unzipping and subsequent wrapping events are initiated and driven by van der Waals interactions between the aromatic rings of siRNA nucleobases and the SWCNT surface. However, molecular dynamics (MD) simulations of double strand DNA (dsDNA) of the same sequence show that the dsDNA undergoes much less unzipping and wrapping on the SWCNT in the simulation time scale of 70 ns. This interesting difference is due to smaller interaction energy of thymidine of dsDNA with the SWCNT compared to that of uridine of siRNA, as calculated by dispersion corrected density functional theory (DFT) methods. After the optimal binding of siRNA to SWCNT, the complex is very stable which serves as one of the major mechanisms of siRNA delivery for biomedical applications. Since siRNA has to undergo unwinding process with the effect of RNA-induced silencing complex, our proposed delivery mechanism by SWCNT possesses potential advantages in achieving RNA interference.
机译:为了设计有效的siRNA传递平台,我们将所有原子经典和量子模拟相结合,以研究原始单壁碳纳米管(SWCNT)对小干扰RNA(siRNA)的结合。我们的结果表明,siRNA通过拉开其碱基对的拉链与SWCNT表面牢固结合,并且随着SWCNTs直径的增加,拉开拉链的倾向也随之增加。 siRNA核碱基的芳香环与SWCNT表面之间的范德华相互作用引发并推动了解压缩和随后的包裹事件。但是,相同序列的双链DNA(dsDNA)的分子动力学(MD)模拟表明,在70 ns的模拟时间内,dsDNA在SWCNT上的解压缩和包裹少得多。这种有趣的差异是由于通过分散校正密度泛函理论(DFT)方法计算得出,与siRNA的尿苷相比,dsDNA的胸苷与SWCNT的相互作用能更小。 siRNA与SWCNT最佳结合后,该复合物非常稳定,是生物医学应用中siRNA传递的主要机制之一。由于siRNA在RNA诱导的沉默复合物的作用下必须经过解链过程,因此我们提出的SWCNT传递机制在实现RNA干扰方面具有潜在优势。

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