Fibrinogenolytic activity of protease from the culture fluid of Pleurotus ostreatus

S. Ye, Chernyshenko, Kucheriavyi Ye
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引用次数: 1

Abstract

The use of proteases makes it possible to obtain partially hydrolyzed forms of macromolecules with unique properties. The importance of proteases for studying the structure and functions of fibrinogen forces scientists to search for new sources of highly specific proteases. Thus, the aim of this work was to study the content of the Pleurotus ostreatus culture fluid in search of fibrinogen- specific proteases. P. ostreatus was cultured for 14 days at 27°C. The culture fluid was collected and the protein fraction was salted out with NaCl and then dialyzed. Fibrinogen hydrolysis products by P. ostreatus protease were characterized using SDS PAGE under reducing conditions followed by immunoprobing using murine monoclonal antibodies I-5A (anti-Aα505-610) and 2d2a (anti-Bβ26-42). The study of turbidity and platelet aggregation was performed using a Multiskan FC spectrophotometric microplate reader and a SOLAR-2110 aggregometer, respectively. Electron microscopy of fibrils formed by truncated compared with native fibrins was performed using a transmission electron microscope N-600. Analysis of the products of fibrinogen hydrolysis with a fungal protease using SDS-PAGE demonstrated the cleavage of the alpha chain of fibrinogen exclusively with the formation of a truncated form of fibrinogen in which there are no C-terminal portions of αC regions with a molecular weight of 25 kDa. A study of turbidity showed that the polymerization of truncated fibrin is significantly impaired. The rate of lateral association of protofibrils significantly decreased from 1.5 to 2.2 times in the case of truncated fibrinogen compared to the native one depending on the initial concentration of fibrinogen. It was shown that platelet aggregation in the presence of fibrinogen without 25 kDa fragments of αC regions was less effective than in the presence of native fibrinogen. Application of the preparation of the fungal protease allows us to obtain high molecular forms of the fibrinogen molecule with cleaved 25 kDa peptides, which provide new information on the role of these peptides in the fibrinogen functioning.
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平菇培养液蛋白酶的纤维蛋白原溶解活性
蛋白酶的使用使得获得具有独特性质的部分水解形式的大分子成为可能。蛋白酶对研究纤维蛋白原结构和功能的重要性迫使科学家们寻找高度特异性蛋白酶的新来源。因此,本研究的目的是研究平菇培养液中纤维蛋白原特异性蛋白酶的含量。P. ostreatus在27℃下培养14天。收集培养液,用NaCl盐腌出蛋白质部分,然后透析。在还原条件下,利用SDS - PAGE对纤维蛋白原水解产物进行了表征,然后用小鼠单克隆抗体I-5A(抗a α505-610)和2d2a(抗b β26-42)进行了免疫探针检测。浊度和血小板聚集的研究分别使用Multiskan FC分光光度微孔板仪和SOLAR-2110聚集仪进行。用N-600透射电子显微镜对截断的纤维蛋白与天然纤维蛋白形成的原纤维进行电镜观察。利用SDS-PAGE对真菌蛋白酶水解纤维蛋白原的产物进行分析,发现纤维蛋白原α链完全断裂,形成截断形式的纤维蛋白原,其中αC区没有c端部分,分子量为25 kDa。浊度的研究表明,截断纤维蛋白的聚合明显受损。根据纤维蛋白原的初始浓度,截断纤维蛋白原的原原纤维的横向结合率显著降低,从1.5倍到2.2倍。结果表明,没有αC区25 kDa片段的纤维蛋白原存在时,血小板聚集的效果不如天然纤维蛋白原存在时。真菌蛋白酶的制备使我们能够获得纤维蛋白原分子的高分子形式,这为这些肽在纤维蛋白原功能中的作用提供了新的信息。
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