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首页> 外文期刊>Toxicon: An International Journal Devoted to the Exchange of Knowledge on the Poisons Derived from Animals, Plants and Microorganisms >Antibodies against synthetic epitopes inhibit the enzymatic activity of mutalysin II, a metalloproteinase from bushmaster snake venom
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Antibodies against synthetic epitopes inhibit the enzymatic activity of mutalysin II, a metalloproteinase from bushmaster snake venom

机译:针对合成表位的抗体可抑制muslysin II的酶活性,所述mutalysin II是来自Bushmaster蛇毒的金属蛋白酶

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摘要

Mutalysin II (mut-II), a 22.5kDa zinc endopeptidase isolated from bushmaster (Lachesis muta muta) snake venom, is a direct acting fibrin(ogen)olytic proteinase. It induces monoclonal and polyclonal antibodies which efficiently neutralize the hemorrhagic effect of L. muta and several Bothrops whole venoms. To characterize epitopes of protective antibodies we have used the Spot method of multiple peptide synthesis to prepare 64 overlapping dodecapeptides frameshifted by three residues, covering the complete amino acid sequence of mut-II. The rabbit anti-mut-II antibodies binding pattern to peptides revealed several continuous antigenic regions: one in the N-terminal part, two in the central region and the other in the C-terminal of mut-II. By using homology modelling, a three-dimensional model of mut-II was built which showed that epitopes are surface exposed. Anti-peptide antibodies were raised against three peptides (one representative of each epitope region) covalently coupled as a mixture to keyhole limpet hemocyanin. Purified IgG from the resulting anti- peptide antibodies cross-reacted with mut-II and induced a dose-dependent inhibition of the mut-II catalyzed proteolysis of fibrinogen.
机译:突变型溶血素II(mut-II)是一种22.5kDa的锌内肽酶,它是从树胶(Lachesis muta muta)蛇毒中分离出来的,是一种直接作用的纤维蛋白原水解酶。它诱导单克隆和多克隆抗体,可以有效地中和乳杆菌和几种Bothrops全毒液的止血作用。为了表征保护性抗体的表位,我们使用了多肽合成的Spot方法来制备64个重叠的十二肽,它们被三个残基移码,覆盖了mut-II的完整氨基酸序列。兔抗-mut-II抗体与肽的结合模式显示出几个连续的抗原区域:一个在mut-II的N末端部分,两个在中央区域,另一个在C-末端。通过使用同源性建模,建立了mut-II的三维模型,该模型表明表位是表面暴露的。产生针对共价偶联至匙孔血蓝蛋白的混合物的三种肽(每个表位区域的一个代表)的抗肽抗体。从得到的抗肽抗体中纯化的IgG与mut-II交叉反应,并诱导了mut-II催化的纤维蛋白原蛋白水解的剂量依赖性抑制。

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