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Bmoo FIBMP-I: A New Fibrinogenolytic Metalloproteinase from Bothrops moojeni Snake Venom

机译:Bmoo FIBMP-I:来自Bothrops moojeni蛇毒的新型纤维蛋白原分解金属蛋白酶

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摘要

A new fibrinogenolytic metalloproteinase (Bmoo FIBMP-I) was purified from Bothrops moojeni snake venom. This enzyme was isolated through a combination of three chromatographic steps (ion-exchange, molecular exclusion, and affinity chromatography). Analyses by reverse phase chromatography, followed by mass spectrometry, showed the presence of enzyme isoforms with average molecular mass of 22.8 kDa. The SDS-PAGE analyses showed a single chain of 27.6 kDa, in the presence and absence of reducing agent. The protein has a blocked N-terminal. One of the peptides obtained by enzymatic digestion of a reduced and S-alkylated isoform was completely sequenced by mass spectrometry (MS/MS). Bmoo FIBMP-I showed similarity with hemorrhagic factor and several metalloproteinases (MP). This enzyme degraded Aα-chain faster than the Bβ-chain and did not affect the γ-chain of bovine fibrinogen. The absence of proteolytic activity after treatment with EDTA, together with the observed molecular mass, led us to suggest that Bmoo FIBMP-I is a member of the P-I class of the snake venom MP family. Bmoo FIBMP-I showed pH-dependent proteolytic activity on azocasein, but was devoid of coagulant, defibrinating, or hemorrhagic activities. The kinetic parameters of proteolytic activity in azocasein were determined (V max = 0.4596 Uh−1nmol−1 ± 0.1031 and K m = 14.59 mg/mL ± 4.610).
机译:从Bothrops moojeni蛇毒中纯化出一种新的纤维蛋白原分解金属蛋白酶(Bmoo FIBMP-I)。通过三个色谱步骤(离子交换,分子排阻和亲和色谱)的组合来分离该酶。通过反相色谱分析,然后进行质谱分析,表明存在平均分子量为22.8 kDa的酶同工型。 SDS-PAGE分析显示在存在和不存在还原剂的情况下,单链为27.6 kDa。该蛋白质的N末端被封闭。通过质谱(MS / MS)对通过还原和还原的S-烷基化同工型进行酶消化而获得的一种肽进行了完全测序。 Bmoo FIBMP-1与出血性因子和几种金属蛋白酶(MP)相似。该酶降解Aα链的速度快于Bβ链,并且不影响牛纤维蛋白原的γ链。 EDTA处理后缺乏蛋白水解活性,再加上观察到的分子量,使我们认为Bmoo FIBMP-I是蛇毒MP家族P-I类的成员。 Bmoo FIBMP-1对偶氮酪蛋白显示出pH依赖的蛋白水解活性,但没有凝结,去纤维蛋白或出血活性。确定了偶氮酪蛋白中蛋白水解活性的动力学参数(V max = 0.4596 Uh -1 nmol -1 ±0.1031和K m = 14.59 mg / mL±4.610)。

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