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通过化学发光法测定生物体液中的亚硝基硫醇。

Determination of s-nitrosothiols in biological fluids by chemiluminescence.

作者信息

Nagababu Enika, Rifkind Joseph M

机构信息

Molecular Dynamics Section, National Institute on Aging, National Institutes of Health, 251 Bayview Blvd, Baltimore, MD, USA.

出版信息

Methods Mol Biol. 2011;704:27-37. doi: 10.1007/978-1-61737-964-2_3.

Abstract

S-nitrosothiols present in nanomolar concentrations in cells and body fluids play an important role in vasodilation, in preventing platelet aggregation, leukocyte adhesion, and for cellular signaling. However, because of the low levels of s-nitrosothiols and interference with other nitric oxide species, reliable assays that measure both high molecular weight and low molecular weight s-nitrosothiols in plasma and red blood cells red blood cells have been difficult to develop. We have previously developed a sensitive method using Cu(II)-ascorbic acid Cu(II)-ascorbic acid at a neutral pH, which was specific for s-nitrosothiols without interference of nitrite or other NOx species. However, due to neutral pH foaming, this method was not suitable for determinations in plasma or red blood cells with high protein content. This method has now been modified by using copper (II) chloride (CuCl(2)) and ascorbic acid in glacial acetic acid. The low pH solves the foaming problem. However, protonation of nitrite under acidic conditions facilitates the formation of s-nitrosothiols. For this method to specifically measure s-nitrosothiols in the sample, the unreacted thiols are blocked by reacting with N-ethylmaleimide and nitrite is blocked by reacting with acidified sulfanilamide before being analyzed by chemiluminescence. Using this method, s-nitrosothiols have been determined in the range of 2 nM to 26 nM (mean ± SE = 10.18±2.1) in plasma and up to 88.1 nM (mean ± SE = 51.27 ± 10.5) in red blood cells.

摘要

细胞和体液中纳摩尔浓度的S-亚硝基硫醇在血管舒张、防止血小板聚集、白细胞黏附以及细胞信号传导中发挥着重要作用。然而,由于S-亚硝基硫醇水平较低且会受到其他一氧化氮种类的干扰,因此很难开发出能够可靠测量血浆和红细胞中高分子量和低分子量S-亚硝基硫醇的检测方法。我们之前开发了一种在中性pH条件下使用Cu(II)-抗坏血酸的灵敏方法,该方法对S-亚硝基硫醇具有特异性,不会受到亚硝酸盐或其他氮氧化物的干扰。然而,由于中性pH会产生泡沫,这种方法不适用于高蛋白含量的血浆或红细胞的检测。现在通过在冰醋酸中使用氯化铜(CuCl₂)和抗坏血酸对该方法进行了改进。低pH解决了泡沫问题。然而,酸性条件下亚硝酸盐的质子化促进了S-亚硝基硫醇的形成。为了使该方法能够特异性测量样品中的S-亚硝基硫醇,在通过化学发光分析之前,未反应的硫醇通过与N-乙基马来酰亚胺反应进行阻断,亚硝酸盐通过与酸化的磺胺反应进行阻断。使用这种方法,血浆中S-亚硝基硫醇的测定范围为2 nM至26 nM(平均值±标准误=10.18±2.1),红细胞中高达88.1 nM(平均值±标准误=51.27±10.5)。

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