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DNA 液滴的酶促降解在相边界附近被调节。

Enzymatic degradation of liquid droplets of DNA is modulated near the phase boundary.

机构信息

Materials Department, University of California, Santa Barbara, CA 93106;

Materials Department, University of California, Santa Barbara, CA 93106.

出版信息

Proc Natl Acad Sci U S A. 2020 Jul 14;117(28):16160-16166. doi: 10.1073/pnas.2001654117. Epub 2020 Jun 29.

Abstract

Biomolecules can undergo liquid-liquid phase separation (LLPS), forming dense droplets that are increasingly understood to be important for cellular function. Analogous systems are studied as early-life compartmentalization mechanisms, for applications as protocells, or as drug-delivery vehicles. In many of these situations, interactions between the droplet and enzymatic solutes are important to achieve certain functions. To explore this, we carried out experiments in which a model LLPS system, formed from DNA "nanostar" particles, interacted with a DNA-cleaving restriction enzyme, SmaI, whose activity degraded the droplets, causing them to shrink with time. By controlling adhesion of the DNA droplet to a glass surface, we were able to carry out time-resolved imaging of this "active dissolution" process. We found that the scaling properties of droplet shrinking were sensitive to the proximity to the dissolution ("boiling") temperature of the dense liquid: For systems far from the boiling point, enzymes acted only on the droplet surface, while systems poised near the boiling point permitted enzyme penetration. This was corroborated by the observation of enzyme-induced vacuole-formation ("bubbling") events, which can only occur through enzyme internalization, and which occurred only in systems poised near the boiling point. Overall, our results demonstrate a mechanism through which the phase stability of a liquid affects its enzymatic degradation through modulation of enzyme transport properties.

摘要

生物分子可以发生液-液相分离 (LLPS),形成密集的液滴,这些液滴对于细胞功能越来越重要。类似的系统被作为早期生命分隔机制、原细胞或药物输送载体进行研究。在这些情况中的许多情况下,液滴和酶溶质之间的相互作用对于实现某些功能非常重要。为了探索这一点,我们进行了实验,其中模型 LLPS 系统由 DNA“纳米星”颗粒形成,与 DNA 切割限制酶 SmaI 相互作用,其活性降解液滴,导致它们随时间收缩。通过控制 DNA 液滴与玻璃表面的粘附,我们能够对这种“主动溶解”过程进行时间分辨成像。我们发现液滴收缩的标度性质对接近密集液体的溶解(“沸腾”)温度敏感:对于远离沸点的系统,酶仅在液滴表面起作用,而接近沸点的系统则允许酶渗透。这通过观察到酶诱导的空泡形成(“冒泡”)事件得到证实,空泡形成只能通过酶内化发生,并且仅在接近沸点的系统中发生。总的来说,我们的结果表明,通过调节酶的输运性质,液相的相稳定性会影响其酶降解的机制。

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