膜联蛋白A5稳定基质囊泡仿生脂质膜:揭示膜联蛋白在钙化中的新作用。

IF 2.2 4区 生物学 Q3 BIOPHYSICS European Biophysics Journal Pub Date : 2023-11-08 DOI:10.1007/s00249-023-01687-4
Claudio R. Ferreira, Marcos Antônio E. Cruz, Maytê Bolean, Luiz Henrique da S. Andrilli, José Luis Millan, Ana Paula Ramos, Massimo Bottini, Pietro Ciancaglini
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引用次数: 0

摘要

基质小泡是一类特殊的细胞外小泡,被认为对生理和病理矿化都有积极贡献。蛋白质组学研究表明,基质小泡具有大量的膜联蛋白A5,这表明该蛋白可能在钙化部位发挥多种作用。目前,膜联蛋白A5被认为可以促进富含磷脂酰丝氨酸和Ca2+的基质囊泡膜内小叶附近的磷灰石矿物的成核。在此,我们旨在通过研究膜联蛋白A5在不存在和存在Ca2+的情况下吸附在基质囊泡仿生脂质体和由二棕榈酰磷脂酰丝氨酸(DPPS)和二棕榈酰膦酰胆碱(DPPC)制成的Langmuir单层上的能力,揭示膜联蛋白A5。差示扫描量热法和动态光散射测量表明,浓度在0.5-2.0mM范围内的Ca2+可能由于DPPS富集结构域的形成而诱导脂质体的聚集。然而,膜联蛋白A5在Ca2+浓度低于1.0mM时避免了脂质体的聚集。表压-表面积等温线显示,膜联素A5在由DPPC和DPPS的混合物制成的单层上的吸附导致过量面积与理论值相比减少,这证实了蛋白质有利于膜脂质之间的有吸引力的相互作用。膜联蛋白A5对脂质膜的稳定性也通过记录表面压力随时间的变化来验证。最后,脂质单层的荧光显微镜图像显示,在膜联蛋白A5存在的情况下,形成了未定形且更大的球形脂质凝聚结构域。我们的数据支持这样的模型,即基质囊泡中的膜联蛋白A5在富含磷脂酰丝氨酸和Ca2+的膜位点被募集,不仅有助于管腔内矿物质的形成,而且有助于稳定囊泡的膜并防止其过早破裂。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

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Annexin A5 stabilizes matrix vesicle-biomimetic lipid membranes: unravelling a new role of annexins in calcification

Matrix vesicles are a special class of extracellular vesicles thought to actively contribute to both physiologic and pathologic mineralization. Proteomic studies have shown that matrix vesicles possess high amounts of annexin A5, suggesting that the protein might have multiple roles at the sites of calcification. Currently, Annexin A5 is thought to promote the nucleation of apatitic minerals close to the inner leaflet of the matrix vesicles’ membrane enriched in phosphatidylserine and Ca2+. Herein, we aimed at unravelling a possible additional role of annexin A5 by investigating the ability of annexin A5 to adsorb on matrix-vesicle biomimetic liposomes and Langmuir monolayers made of dipalmitoylphosphatidylserine (DPPS) and dipalmitoylphosphatidylcholine (DPPC) in the absence and in the presence of Ca2+. Differential scanning calorimetry and dynamic light scattering measurements showed that Ca2+ at concentrations in the 0.5–2.0 mM range induced the aggregation of liposomes probably due to the formation of DPPS-enriched domains. However, annexin A5 avoided the aggregation of liposomes at Ca2+ concentrations lower than 1.0 mM. Surface pressure versus surface area isotherms showed that the adsorption of annexin A5 on the monolayers made of a mixture of DPPC and DPPS led to a reduction in the area of excess compared to the theoretical values, which confirmed that the protein favored attractive interactions among the membrane lipids. The stabilization of the lipid membranes by annexin A5 was also validated by recording the changes with time of the surface pressure. Finally, fluorescence microscopy images of lipid monolayers revealed the formation of spherical lipid-condensed domains that became unshaped and larger in the presence of annexin A5. Our data support the model that annexin A5 in matrix vesicles is recruited at the membrane sites enriched in phosphatidylserine and Ca2+ not only to contribute to the intraluminal mineral formation but also to stabilize the vesicles’ membrane and prevent its premature rupture.

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来源期刊
European Biophysics Journal
European Biophysics Journal 生物-生物物理
CiteScore
4.30
自引率
0.00%
发文量
43
审稿时长
6-12 weeks
期刊介绍: The journal publishes papers in the field of biophysics, which is defined as the study of biological phenomena by using physical methods and concepts. Original papers, reviews and Biophysics letters are published. The primary goal of this journal is to advance the understanding of biological structure and function by application of the principles of physical science, and by presenting the work in a biophysical context. Papers employing a distinctively biophysical approach at all levels of biological organisation will be considered, as will both experimental and theoretical studies. The criteria for acceptance are scientific content, originality and relevance to biological systems of current interest and importance. Principal areas of interest include: - Structure and dynamics of biological macromolecules - Membrane biophysics and ion channels - Cell biophysics and organisation - Macromolecular assemblies - Biophysical methods and instrumentation - Advanced microscopics - System dynamics.
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