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开发用于在色谱分离后分析蛇毒磷脂酶 A 活性的高通量筛选测定法。

Development of high-throughput screening assays for profiling snake venom phospholipase A activity after chromatographic fractionation.

机构信息

Division of BioAnalytical Chemistry, Amsterdam Institute of Molecular and Life Sciences, Vrije Universiteit Amsterdam, De Boelelaan 1085, 1081, HV, Amsterdam, the Netherlands; Centre for Analytical Sciences Amsterdam (CASA), the Netherlands.

Division of BioAnalytical Chemistry, Amsterdam Institute of Molecular and Life Sciences, Vrije Universiteit Amsterdam, De Boelelaan 1085, 1081, HV, Amsterdam, the Netherlands.

出版信息

Toxicon. 2020 Sep;184:28-38. doi: 10.1016/j.toxicon.2020.05.022. Epub 2020 Jun 2.

DOI:10.1016/j.toxicon.2020.05.022
PMID:32502555
Abstract

Many organisms, ranging from plants to mammals, contain phospholipase A enzymes (PLAs), which catalyze the production of lysophospholipids and fatty acid proinflammatory mediators. PLAs are also common constituents of animal venoms, including bees, scorpions and snakes, and they cause a wide variety of toxic effects including neuro-, myo-, cyto-, and cardio-toxicity, anticoagulation and edema. The aim of this study was to develop a generic method for profiling enzymatically active PLAs in snake venoms after chromatographic separation. For this, low-volume high-throughput assays for assessment of enzymatic PLA activity were evaluated and optimized. Subsequently, the assays were incorporated into a nanofractionation platform that combines high-resolution fractionation of crude venoms by liquid chromatography (LC) with bioassaying in 384-well plate format, and parallel mass spectrometric (MS) detection for toxin identification. The miniaturized assays developed are based on absorbance or fluorescence detection (respectively, using cresol red or fluorescein as pH indicators) to monitor the pH drop associated with free fatty acid formation by enzymatically active PLAs. The methodology was demonstrated for assessment of PLA activity profiles of venoms from the snake species Bothrops asper, Echis carinatus, Echis coloratus, Echis ocellatus, Oxyuranus scutellatus and Daboia russelii russelii.

摘要

许多生物体,从植物到哺乳动物,都含有磷脂酶 A 酶(PLA),它催化溶血磷脂和脂肪酸炎症介质的产生。PLA 也是动物毒液的常见成分,包括蜜蜂、蝎子和蛇,它们会引起多种毒性作用,包括神经毒性、肌肉毒性、细胞毒性和心脏毒性、抗凝和水肿。本研究的目的是开发一种在色谱分离后对蛇毒液中具有酶活性的 PLA 进行分析的通用方法。为此,评估和优化了用于评估酶 PLA 活性的小体积高通量测定法。随后,将这些测定法纳入纳分馏平台中,该平台将通过液相色谱(LC)对粗毒液进行高分辨率分馏与 384 孔板格式的生物测定相结合,并平行进行质谱(MS)检测以鉴定毒素。开发的微型测定法基于吸光度或荧光检测(分别使用甲酚红或荧光素作为 pH 指示剂)来监测与酶活性 PLA 形成游离脂肪酸相关的 pH 下降。该方法学已用于评估蛇种 Bothrops asper、Echis carinatus、Echis coloratus、Echis ocellatus、Oxyuranus scutellatus 和 Daboia russelii russelii 的毒液中 PLA 活性谱。

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