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Investigating fast folding of RNA pseudoknot VPK with an ultrafast microfluidic mixer.

机译:用超快速微流体混合器研究RNA假结VPK的快速折叠。

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摘要

Despite advances in understanding the theory behind RNA folding, ab initio prediction of the folding process has not been achieved yet. Given only the sequence information we still cannot tell the precise three-dimensional structure of neither RNA nor protein. Knowing the kinetics of folding we hope to learn more about the arrangement of secondary and tertiary structure.;For that reason we investigated the folding process of RNA pseudoknot VPK with our microfluidic mixing device. VPK (variant pseudoknot) is a variant of the mouse mammary tumor virus (MMTV) pseudoknot and it was specifically designed to prevent the formation of alternative base pairings in the stem regions. Using two differently labeled samples, VPK-2AP and F-VPK, and high and low salt folding conditions, we analyzed the folding process and determined the different folding rates. Our results match very well with recently published findings, but they also raise the possible existence of folding transitions not seen in T-jump experiments. The measured folding times are in the range of 0.5 to several milliseconds. The folding process seems to have different pathways with one of the stems of the pseudoknot forming before, perhaps even initiating the folding of the other.
机译:尽管在理解RNA折叠背后的理论方面有进步,但尚未实现对折叠过程的从头开始的预测。仅给出序列信息,我们仍然无法分辨出RNA和蛋白质的精确三维结构。了解折叠的动力学过程后,我们希望进一步了解二级和三级结构的排列方式。因此,我们使用微流体混合装置研究了RNA假结VPK的折叠过程。 VPK(变型假结)是小鼠乳腺肿瘤病毒(MMTV)假结的变体,它经过专门设计,可以防止在茎区域中形成其他碱基配对。使用两种不同标记的样品VPK-2AP和F-VPK,以及高盐和低盐折叠条件,我们分析了折叠过程并确定了不同的折叠速率。我们的结果与最近发表的发现非常吻合,但它们也增加了T型跳跃实验中未发现的折叠过渡的可能。测得的折叠时间为0.5到几毫秒。折叠过程似乎具有不同的路径,假结的茎之一在此之前形成,甚至可能开始了另一个的折叠。

著录项

  • 作者

    Meindl, Andreas John.;

  • 作者单位

    Michigan State University.;

  • 授予单位 Michigan State University.;
  • 学科 Physics General.;Biophysics General.
  • 学位 M.S.
  • 年度 2012
  • 页码 58 p.
  • 总页数 58
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类
  • 关键词

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