ACTION OF VENOM OF VIPERA SNAKE OF UKRAINE ON BLOOD COAGULATION in vitro

Biotechnologia Acta Pub Date : 2022-04-01 DOI:10.15407/biotech15.02.056

E. Iskandarov

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引用次数: 1

Abstract

Aim. In this study we focused on the search of fibrinogen-targeted proteases in the venom of Vipera renardi, Vipera nikolskii and Vipera berus. Venom of Vipera berus was also fractionated on Q-sepharose and action of separated fractions on human blood plasma, platelets and red cells was studied. Methods. Analysis of protein mixtures was performed using SDS-PAGE. Аction on the blood coagulation system was analyzed using the APTT assay. Identification of protein components with fibrinolytic activity was performed using enzyme-electrophoresis with fibrinogen as the substrate. Fractionation of V. berus venom was performed on Q-sepharose using FPLC system Acta Prime. Action of separated fractions on ADP-induced platelet aggregation in platelet rich blood plasma was analyzed using Aggregometer AP 2110. Hemolytic action of fractions was estimated using fresh human red cells. Amount of released hemoglobin was estimated by spectrophotometry on Optizen POP. Results. All studied venoms had different protein compositions with major protein fractions in the range from 25 kDa to 130 kDa. Both V. berus and V. nikolskii venoms taken in 1:200 dilutions reduced the time of clotting in APTT test from 25 to 13 s. In contrast, V. renardi venom in the same dilution prolonged the clotting time from 25 s to 180 s that we assumed as the result of fibrinogen-specific protease presence. According to enzyme-electrophoresis data all studied venoms contained fibrinogen-specific proteases with the apparent molecular weights for V. berus, V. nikolskii – 25-55 kDa. and V. renardi – 55-75 kDa. Fractionation of crude venom of V. berus allowed obtaining several fractions eluted at different concentrations of NaCl: 0.1; 0.2; 0.3; 0.5 М. Non-binded fraction was also collected. Conclusions. Thus, the components of Vipera venoms living in Ukraine can be used for basic biochemical research. At the same time, care should be taken in the case of envenomation, as the presence of fibrinogenolytic enzymes in the venom can lead to hemorrhage. Further characterization of fibrinogen-specific protease from V. berus venom is a promising task for biotechnology.

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乌克兰蝮蛇毒液对体外凝血的作用

的目标。在本研究中，我们主要研究了雷氏蝮蛇、尼古斯基蝮蛇和贝鲁斯蝮蛇毒液中纤维蛋白原靶向蛋白酶的研究。用Q-sepharose对蝰蛇毒液进行了分离，研究了分离物对人血浆、血小板和红细胞的作用。方法。用SDS-PAGE对蛋白混合物进行分析。应用APTT法分析Аction对凝血系统的影响。以纤维蛋白原为底物，采用酶电泳法鉴定具有纤溶活性的蛋白组分。采用FPLC系统对Q-sepharose进行分离。应用Aggregometer ap2110分析了分离组分对富血小板血浆中adp诱导血小板聚集的作用。用新鲜的人红细胞估计其溶血作用。Optizen POP分光光度法测定血红蛋白释放量。结果。所有研究的毒液都有不同的蛋白质组成，主要蛋白质含量在25 kDa到130 kDa之间。贝鲁斯弧菌和尼可氏弧菌毒液按1:200稀释后，APTT试验的凝血时间由25 s缩短至13 s。相比之下，在相同稀释度下，V. renardi毒液将凝血时间从25秒延长到180秒，我们认为这是纤维蛋白原特异性蛋白酶存在的结果。根据酶电泳数据，所有研究的毒液均含有纤维蛋白原特异性蛋白酶，其表观分子量为V. berus, V. nikolskii - 25-55 kDa。V. renardi - 55-75 kDa。对贝鲁斯的粗毒液进行分馏，得到不同浓度NaCl: 0.1洗脱的几个部分;0.2;0.3;0.5М。未结合部分也被收集。结论。因此，生活在乌克兰的毒蛇毒液成分可用于基础生化研究。同时，在毒液中毒的情况下要小心，因为毒液中纤维蛋白原溶解酶的存在会导致出血。进一步鉴定蛇毒纤维蛋白原特异性蛋白酶是一项有前景的生物技术任务。

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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Biotechnologia Acta

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20 weeks