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反光蛋白结合并重组合成磷脂囊泡。

Reflectin Proteins Bind and Reorganize Synthetic Phospholipid Vesicles.

作者信息

Song Junyi, Levenson Robert, Santos Jerome, Velazquez Lourdes, Zhang Fan, Fygenson Deborah, Wu Wenjian, Morse Daniel E

机构信息

Department of Molecular, Cellular and Developmental Biology, University of California, Santa Barbara, California 93106-5100, United States.

Physics Department and California Nanosystems Institute, University of California, Santa Barbara, California 93106, United States.

出版信息

Langmuir. 2020 Mar 17;36(10):2673-2682. doi: 10.1021/acs.langmuir.9b03632. Epub 2020 Mar 9.

DOI:10.1021/acs.langmuir.9b03632
PMID:32097553
Abstract

The reflectin proteins have been extensively studied for their role in reflectance in cephalopods. In the recently evolved Loliginid squids, these proteins and the structural color they regulate are dynamically tunable, enhancing their effectiveness for camouflage and communication. In these species, the reflectins are found in highest concentrations within the structurally tunable, membrane enclosed, periodically stacked lamellae of subcellular Bragg reflectors and in the intracellular vesicles of specialized skin cells known as iridocytes and leuocophores, respectively. To better understand the interactions between the reflectins and the membrane structures that encompass them, we analyzed the interactions of two purified reflectins with synthetic phospholipid membrane vesicles similar in composition to cellular membranes, using confocal fluorescence microscopy and dynamic light scattering. The purified recombinant reflectins were found to drive multivalent vesicle agglomeration in a ratio-dependent and saturable manner. Extensive proteolytic digestion terminated with PMSF of the reflectin A1-vesicle complexes triggered energetic membrane rearrangement, resulting in vesicle fusion, fission, and tubulation. This behavior contrasted markedly with that of vesicles complexed with reflectin C, from which PMSF-terminated proteolysis only released the original size vesicles. Clues to the basis for this difference, residing in significant differences between the structures of the two reflectins, led to the suggestion that specific reflectin-membrane interactions may play a role in the ontogenetic formation, long-term maintenance, and/or dynamic behavior of their biophotonically active host membrane nanostructures. Similar energetic remodeling has been associated with osmotic stress in other membrane systems, suggesting a path to reconstitution of the biophotonic system .

摘要

反射蛋白因其在头足类动物反射中的作用而受到广泛研究。在最近进化的枪乌贼科鱿鱼中,这些蛋白及其调节的结构色是动态可调的,增强了它们在伪装和通讯方面的有效性。在这些物种中,反射蛋白在亚细胞布拉格反射器的结构可调、膜包裹、周期性堆叠的薄片中浓度最高,分别在称为虹彩细胞和白色素细胞的特殊皮肤细胞的细胞内小泡中浓度最高。为了更好地理解反射蛋白与包围它们的膜结构之间的相互作用,我们使用共聚焦荧光显微镜和动态光散射分析了两种纯化的反射蛋白与组成与细胞膜相似的合成磷脂膜囊泡的相互作用。发现纯化的重组反射蛋白以比例依赖性和饱和方式驱动多价囊泡聚集。用苯甲基磺酰氟(PMSF)终止对反射蛋白A1-囊泡复合物的广泛蛋白水解作用会引发剧烈的膜重排,导致囊泡融合、裂变和形成微管。这种行为与与反射蛋白C复合的囊泡的行为形成明显对比,用PMSF终止对其的蛋白水解作用只会释放出原始大小的囊泡。这两种反射蛋白结构上的显著差异为这种差异的基础提供了线索,这表明特定的反射蛋白-膜相互作用可能在其生物光子活性宿主膜纳米结构的个体发育形成、长期维持和/或动态行为中发挥作用。类似的剧烈重塑与其他膜系统中的渗透压应激有关,这为生物光子系统的重构提供了一条途径。

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引用本文的文献

1
Protein Charge Neutralization Is the Proximate Driver Dynamically Tuning Reflectin Assembly.蛋白质电荷中和是动态调节反射素组装的直接驱动力。
Int J Mol Sci. 2024 Aug 17;25(16):8954. doi: 10.3390/ijms25168954.
2
A colloidal model for the equilibrium assembly and liquid-liquid phase separation of the reflectin A1 protein.一种胶体模型,用于反射蛋白 A1 的平衡组装和液-液相分离。
Biophys J. 2024 Sep 17;123(18):3065-3079. doi: 10.1016/j.bpj.2024.07.004. Epub 2024 Jul 4.
3
Synthetic peptides for the precise transportation of proteins of interests to selectable subcellular areas.
用于将目标蛋白质精确转运至可选择亚细胞区域的合成肽。
Front Bioeng Biotechnol. 2023 Feb 20;11:1062769. doi: 10.3389/fbioe.2023.1062769. eCollection 2023.
4
A Mini-Review on Reflectins, from Biochemical Properties to Bio-Inspired Applications.关于反射蛋白的综述:从生化特性到仿生应用
Int J Mol Sci. 2022 Dec 10;23(24):15679. doi: 10.3390/ijms232415679.
5
Tunable Cellular Localization and Extensive Cytoskeleton-Interplay of Reflectins.反射蛋白的可调细胞定位及广泛的细胞骨架相互作用
Front Cell Dev Biol. 2022 Jun 23;10:862011. doi: 10.3389/fcell.2022.862011. eCollection 2022.