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3
A Stopped-Flow Light Scattering Methodology for Assessing the Osmotic Water Permeability of Whole Sertoli Cells.一种用于评估全支持细胞渗透水通透性的停流光散射方法。
Methods Mol Biol. 2018;1748:279-286. doi: 10.1007/978-1-4939-7698-0_19.
4
AQP2 in human urine is predominantly localized to exosomes with preserved water channel activities.人尿液中的水通道蛋白2主要定位于具有保留水通道活性的外泌体中。
Clin Exp Nephrol. 2018 Aug;22(4):782-788. doi: 10.1007/s10157-018-1538-6. Epub 2018 Feb 2.
5
Reproducible Preparation of Proteopolymersomes via Sequential Polymer Film Hydration and Membrane Protein Reconstitution.通过顺序聚合物膜水合和膜蛋白重构制备可重现的蛋白聚合物囊泡。
Langmuir. 2017 Oct 31;33(43):12336-12343. doi: 10.1021/acs.langmuir.7b02926. Epub 2017 Oct 19.
6
Dynamical modeling of liver Aquaporin-9 expression and glycerol permeability in hepatic glucose metabolism.肝葡萄糖代谢中肝水通道蛋白-9表达和甘油通透性的动力学建模。
Eur J Cell Biol. 2017 Jan;96(1):61-69. doi: 10.1016/j.ejcb.2016.12.003. Epub 2016 Dec 28.
7
Molecular cloning, overexpression and characterization of a novel water channel protein from Rhodobacter sphaeroides.球形红细菌一种新型水通道蛋白的分子克隆、过表达及特性分析
PLoS One. 2014 Jan 31;9(1):e86830. doi: 10.1371/journal.pone.0086830. eCollection 2014.
8
Preparative scale production and functional reconstitution of a human aquaglyceroporin (AQP3) using a cell free expression system.使用无细胞表达系统进行人水通道蛋白 3(AQP3)的制备规模生产和功能重建。
N Biotechnol. 2013 Jun 25;30(5):545-51. doi: 10.1016/j.nbt.2013.03.007. Epub 2013 Mar 26.
9
Biophysical assessment of aquaporin-9 as principal facilitative pathway in mouse liver import of glucogenetic glycerol.水通道蛋白-9 作为葡萄糖生成甘油在小鼠肝内摄取的主要易化途径的生物物理评估
Biol Cell. 2012 Jun;104(6):342-51. doi: 10.1111/boc.201100061. Epub 2012 Mar 23.
10
Aquaporin-9 protein is the primary route of hepatocyte glycerol uptake for glycerol gluconeogenesis in mice.水通道蛋白-9 蛋白是小鼠肝细胞甘油摄取用于甘油糖异生的主要途径。
J Biol Chem. 2011 Dec 30;286(52):44319-25. doi: 10.1074/jbc.M111.297002. Epub 2011 Nov 11.

红细胞甘油渗透性的停流光散射分析

Stopped-flow Light Scattering Analysis of Red Blood Cell Glycerol Permeability.

作者信息

Gena Patrizia, Portincasa Piero, Matera Sabino, Sonntag Yonathan, Rützler Michael, Calamita Giuseppe

机构信息

Department of Biosciences, Biotechnologies and Biopharmaceutics, University of Bari "Aldo Moro", Bari, Italy.

Clinica Medica "A. Murri", Department of Biomedical Sciences and Human Oncology, Medical School, University of Bari "Aldo Moro", Bari, Italy.

出版信息

Bio Protoc. 2020 Aug 20;10(16):e3723. doi: 10.21769/BioProtoc.3723.

DOI:10.21769/BioProtoc.3723
PMID:33659385
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC7842326/
Abstract

Stopped-Flow Light Scattering (SFLS) is a method devised to analyze the kinetics of fast chemical reactions that result in a significant change of the average molecular weight and/or in the shape of the reaction substrates. Several modifications of the original stopped-flow system have been made leading to a significant extension of its technical applications. One of these modifications allows the biophysical characterization of the water and solute permeability of biological and artificial membranes. Here, we describe a protocol of SFLS to measure the glycerol permeability of isolated human red blood cells (RBCs) and evaluate the pharmacokinetics properties (selectivity and potency) of isoform-specific inhibitors of AQP3, AQP7 and AQP9, three mammalian aquaglyceroporins allowing transport of glycerol across membranes. Suspensions of RBCs (1% hematocrit) are exposed to an inwardly directed gradient of 100 mM glycerol in a SFLS apparatus at 20 °C and the resulting changes in scattered light intensity are recorded at a monochromatic wavelength of 530 nm for 120 s. The SFLS apparatus is set up to have a dead time of 1.6-ms and 99% mixing efficiency in less than 1 ms. Data are fitted to a single exponential function and the related time constant (τ, seconds) of the cell-swelling phase of light scattering corresponding to the osmotic movement of water that accompanies the entry of glycerol into erythrocytes is measured. The coefficient of glycerol permeability ( , cm/s) of RBCs is calculated with the following equation: = 1/[(S/V)τ] where τ (s) is the fitted exponential time constant and S/V is the surface-to-volume ratio (cm) of the analyzed RBC specimen. Pharmacokinetics of the isoform-specific inhibitors of AQP3, AQP7 and AQP9 are assessed by evaluating the extent of RBC values resulting after the exposure to serial concentrations of the blockers.

摘要

停流光散射(SFLS)是一种用于分析快速化学反应动力学的方法,这些反应会导致平均分子量和/或反应底物形状发生显著变化。对原始停流系统进行了多次改进,从而显著扩展了其技术应用范围。其中一项改进使得能够对生物膜和人工膜的水和溶质渗透性进行生物物理表征。在此,我们描述了一种使用SFLS测量分离的人类红细胞(RBC)甘油渗透性的方案,并评估水通道蛋白3(AQP3)、水通道蛋白7(AQP7)和水通道蛋白9(AQP9)这三种允许甘油跨膜运输的哺乳动物水甘油通道蛋白的亚型特异性抑制剂的药代动力学特性(选择性和效力)。在20℃下,将红细胞悬液(血细胞比容为1%)置于SFLS装置中,使其暴露于100 mM甘油的内向梯度中,并在530 nm单色波长下记录120秒内散射光强度的变化。SFLS装置设置为死时间为1.6毫秒,在不到1毫秒内混合效率达到99%。数据拟合为单指数函数,并测量与甘油进入红细胞时伴随的水渗透运动相对应的光散射细胞肿胀阶段的相关时间常数(τ,秒)。红细胞的甘油渗透系数( ,cm/s)通过以下公式计算: = 1/[(S/V)τ],其中τ(s)是拟合的指数时间常数,S/V是分析的红细胞标本的表面积与体积比(cm)。通过评估暴露于系列浓度阻滞剂后红细胞 值的变化程度来评估AQP3、AQP水通道蛋白7和水通道蛋白9的亚型特异性抑制剂的药代动力学。