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溶菌酶光化学与温度的关系。纳米颗粒对溶菌酶光稳定性的保护作用。

Lysozyme Photochemistry as a Function of Temperature. The Protective Effect of Nanoparticles on Lysozyme Photostability.

作者信息

Oliveira Silva Catarina, Petersen Steffen B, Pinto Reis Catarina, Rijo Patrícia, Molpeceres Jesús, Vorum Henrik, Neves-Petersen Maria Teresa

机构信息

Research Center for Biosciences & Health Technologies, Universidade Lusófona, Lisboa, 1749-024, Portugal.

Department of Biomedical Sciences, Faculty of Pharmacy, University of Alcalá, 28871 Alcalá de Henares, Spain.

出版信息

PLoS One. 2015 Dec 14;10(12):e0144454. doi: 10.1371/journal.pone.0144454. eCollection 2015.

Abstract

The presence of aromatic residues and their close spatial proximity to disulphide bridges makes hen egg white lysozyme labile to UV excitation. UVB induced photo-oxidation of tryptophan and tyrosine residues leads to photochemical products, such as, kynurenine, N-formylkynurenine and dityrosine and to the disruption of disulphide bridges in proteins. We here report that lysozyme UV induced photochemistry is modulated by temperature, excitation power, illumination time, excitation wavelength and by the presence of plasmonic quencher surfaces, such as gold, and by the presence of natural fluorescence quenchers, such as hyaluronic acid and oleic acid. We show evidence that the photo-oxidation effects triggered by 295 nm at 20°C are reversible and non-reversible at 10°C, 25°C and 30°C. This paper provides evidence that the 295 nm damage threshold of lysozyme lies between 0.1 μW and 0.3 μW. Protein conformational changes induced by temperature and UV light have been detected upon monitoring changes in the fluorescence emission spectra of lysozyme tryptophan residues and SYPRO® Orange. Lysozyme has been conjugated onto gold nanoparticles, coated with hyaluronic acid and oleic acid (HAOA). Steady state and time resolved fluorescence studies of free and conjugated lysozyme onto HAOA gold nanoparticles reveals that the presence of the polymer decreased the rate of the observed photochemical reactions and induced a preference for short fluorescence decay lifetimes. Size and surface charge of the HAOA gold nanoparticles have been determined by dynamic light scattering and zeta potential measurements. TEM analysis of the particles confirms the presence of a gold core surrounded by a HAOA matrix. We conclude that HAOA gold nanoparticles may efficiently protect lysozyme from the photochemical effects of UVB light and this nanocarrier could be potentially applied to other proteins with clinical relevance. In addition, this study confirms that the temperature plays a critical role in the photochemical pathways a protein enters upon UV excitation.

摘要

芳香族残基的存在及其与二硫键的紧密空间 proximity 使得鸡蛋清溶菌酶对紫外线激发不稳定。UVB 诱导的色氨酸和酪氨酸残基的光氧化导致光化学产物,如犬尿氨酸、N-甲酰犬尿氨酸和二酪氨酸,并导致蛋白质中二硫键的破坏。我们在此报告,溶菌酶紫外线诱导的光化学受到温度、激发功率、光照时间、激发波长以及等离子体猝灭剂表面(如金)的存在以及天然荧光猝灭剂(如透明质酸和油酸)的存在的调节。我们表明,在 20°C 下由 295 nm 触发的光氧化效应在 10°C、25°C 和 30°C 下是可逆的和不可逆的。本文提供了证据表明溶菌酶的 295 nm 损伤阈值在 0.1 μW 和 0.3 μW 之间。通过监测溶菌酶色氨酸残基和 SYPRO® Orange 的荧光发射光谱的变化,检测到温度和紫外线诱导的蛋白质构象变化。溶菌酶已与涂有透明质酸和油酸(HAOA)的金纳米颗粒缀合。对游离和缀合到 HAOA 金纳米颗粒上的溶菌酶进行稳态和时间分辨荧光研究表明,聚合物的存在降低了观察到的光化学反应速率,并导致对短荧光衰减寿命的偏好。通过动态光散射和 zeta 电位测量确定了 HAOA 金纳米颗粒的尺寸和表面电荷。对颗粒的 TEM 分析证实了存在被 HAOA 基质包围的金核。我们得出结论,HAOA 金纳米颗粒可以有效地保护溶菌酶免受 UVB 光的光化学影响,并且这种纳米载体可能潜在地应用于其他具有临床相关性的蛋白质。此外,本研究证实温度在蛋白质受到紫外线激发时进入的光化学途径中起着关键作用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/cbc4/4682814/d57612e15268/pone.0144454.g001.jpg

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