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从袋獾血清中分离和鉴定两种蛇毒金属蛋白酶抑制剂DM40和DM43。

Isolation and characterization of DM40 and DM43, two snake venom metalloproteinase inhibitors from Didelphis marsupialis serum.

作者信息

Neves-Ferreira A G, Cardinale N, Rocha S L, Perales J, Domont G B

机构信息

Depto. Fisiologia e Farmacodinâmica, Instituto Oswaldo Cruz, Fiocruz, 21045-900 Rio de Janeiro, Brazil

出版信息

Biochim Biophys Acta. 2000 May 1;1474(3):309-20. doi: 10.1016/s0304-4165(00)00022-2.

DOI:10.1016/s0304-4165(00)00022-2
PMID:10779682
Abstract

From Didelphis marsupialis serum, two antihemorrhagic proteins were isolated by DEAE-Sephacel, Phenyl-Sepharose and Superdex 200 and characterized. Their masses by mass spectrometry were 40318 AMU for DM40 and 42373 and 43010 AMU for DM43, indicating the presence of isoforms for the last. Molecular masses of 44.8 and 47.3 were obtained by SDS-PAGE, respectively for DM40 and DM43. Both inhibitors showed isoelectric points lower than 3.5 and glycosylation percentages varying from 20.5 to 29.0%, as estimated by chemical deglycosylation and amino acid analysis. N-terminal sequences of the first 17 residues of DM40 and DM43 were identical except for the exchange of R9 for P9. Both were homologous to oprin, a similar inhibitor from Didelphis virginiana serum. No evidence of complex formation between DM40 and DM43 was observed either by native PAGE or gel filtration chromatography. In addition to the antihemorrhagic activity, DM40 and DM43 inhibited the hydrolysis of casein, fibrinogen and fibronectin by Bothrops jararaca venom. DM43 also showed antilethal, antiedematogenic and antihyperalgesic activities. None of the inhibitors showed enzymatic activity on casein. Both proteins formed stable complexes with jararhagin and inhibited its hemorrhagic effect as well as the enzymatic activity of this toxin on fluorogenic substrate.

摘要

从绵毛负鼠血清中,通过DEAE-葡聚糖凝胶、苯基琼脂糖凝胶和Superdex 200分离出两种抗出血蛋白并对其进行了表征。通过质谱分析,DM40的质量为40318原子质量单位,DM43的质量为42373和43010原子质量单位,这表明后者存在异构体。通过SDS-PAGE分别测得DM40和DM43的分子量为44.8和47.3。通过化学去糖基化和氨基酸分析估计,两种抑制剂的等电点均低于3.5,糖基化百分比在20.5%至29.0%之间。DM40和DM43前17个残基的N端序列除了R9被P9替换外完全相同。两者均与弗吉尼亚负鼠血清中的一种类似抑制剂oprin同源。无论是非变性PAGE还是凝胶过滤色谱法,均未观察到DM40和DM43之间形成复合物的证据。除抗出血活性外,DM40和DM43还抑制了巴西矛头蝮蛇毒对酪蛋白、纤维蛋白原和纤连蛋白的水解。DM43还表现出抗致死、抗水肿和抗痛觉过敏活性。这些抑制剂均未对酪蛋白表现出酶活性。两种蛋白质均与矛头蝮蛇毒素形成稳定的复合物,并抑制其出血作用以及该毒素对荧光底物的酶活性。

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