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运用单分子成像技术探索细胞内的异质性。

Using single molecule imaging to explore intracellular heterogeneity.

机构信息

Oregon Health and Science University, Quantitative and Systems Biology Program in BME and The Knight Cancer Institute, Portland, OR 97239, USA.

出版信息

Int J Biochem Cell Biol. 2023 Oct;163:106455. doi: 10.1016/j.biocel.2023.106455. Epub 2023 Aug 15.

Abstract

Despite more than 100 years of study, it is unclear if the movement of proteins inside the cell is best described as a mosh pit or an exquisitely choreographed dance. Recent studies suggest the latter. Local interactions induce molecular condensates such as liquid-liquid phase separations (LLPSs) or non-liquid, functionally significant molecular aggregates, including synaptic densities, nucleoli, and Amyloid fibrils. Molecular condensates trigger intracellular signaling and drive processes ranging from gene expression to cell division. However, the descriptions of condensates tend to be qualitative and correlative. Here, we indicate how single-molecule imaging and analyses can be applied to quantify condensates. We discuss the pros and cons of different techniques for measuring differences between transient molecular behaviors inside and outside condensates. Finally, we offer suggestions for how imaging and analyses from different time and space regimes can be combined to identify molecular behaviors indicative of condensates within the dynamic high-density intracellular environment.

摘要

尽管已经进行了 100 多年的研究,但蛋白质在细胞内的运动是更像是一场乱舞,还是一场精心编排的舞蹈,目前仍不清楚。最近的研究表明,更倾向于后者。局部相互作用诱导分子凝聚物,如液-液相分离(LLPS)或非液相、具有功能意义的分子聚集体,包括突触密度、核仁、和淀粉样纤维。分子凝聚物触发细胞内信号转导,并驱动从基因表达到细胞分裂等过程。然而,凝聚物的描述往往是定性和相关的。在这里,我们指出如何应用单分子成像和分析来定量凝聚物。我们讨论了测量凝聚物内外瞬态分子行为差异的不同技术的优缺点。最后,我们提出了如何将来自不同时间和空间范围的成像和分析相结合,以识别在动态高密度细胞内环境中具有凝聚物特征的分子行为的建议。

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