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用编码矛头蝮蛇(Bothrops asper)一种新型P-II金属蛋白酶的质粒免疫产生的马抗体对蛇毒诱导的出血进行中和作用。

Neutralization of venom-induced hemorrhage by equine antibodies raised by immunization with a plasmid encoding a novel P-II metalloproteinase from the lancehead pitviper Bothrops asper.

作者信息

Arce-Estrada Viviana, Azofeifa-Cordero Gabriela, Estrada Ricardo, Alape-Girón Alberto, Flores-Díaz Marietta

机构信息

Instituto Clodomiro Picado, Facultad de Microbiología, Universidad de Costa Rica, San José, Costa Rica.

出版信息

Vaccine. 2009 Jan 14;27(3):460-6. doi: 10.1016/j.vaccine.2008.10.066. Epub 2008 Nov 12.

Abstract

In this work, the cDNA encoding a novel P-II type metalloproteinase from Bothrops asper venom glands was cloned, sequenced and used for DNA immunization of animals with accelerated DNA-coated tungsten microparticles and the helius Gene Gun system. Specific antibodies against B. asper venom antigens were induced in mice co-immunized with the plasmid encoding the P-II metalloproteinase together with an expression plasmid encoding the murine IL-2. Similarly, specific antibodies against B. asper venom antigens were also induced in a horse co-immunized with the plasmid encoding the P-II metalloproteinase, together with a plasmid encoding the equine IL-6. The equine antibodies induced by immunization with the P-II metalloproteinase encoding plasmid cross react with several proteins of B. asper, Crotalus durissus durissus, and Lachesis stenophrys venoms in western blot, demonstrating antigenic similarity between the cloned metalloproteinase and other metalloproteinases present in these venoms. Furthermore, the equine antibodies induced by immunization with the P-II metalloproteinase encoding plasmid completely neutralized the hemorrhagic activity of the whole B. asper venom and partially the hemorrhagic activity of C. durissus durissus venom. The neutralizing ability of the produced antibodies raises, for the first time, the possibility of developing therapeutic antivenoms in horses by DNA immunization using tungsten microparticles.

摘要

在本研究中,克隆并测序了编码来自矛头蝮蛇毒腺的一种新型P-II型金属蛋白酶的cDNA,并使用加速的包被DNA的钨微粒和氦气基因枪系统对动物进行DNA免疫。在用编码P-II金属蛋白酶的质粒与编码小鼠白细胞介素-2的表达质粒共同免疫的小鼠中,诱导产生了针对矛头蝮蛇毒抗原的特异性抗体。同样,在用编码P-II金属蛋白酶的质粒与编码马白细胞介素-6的质粒共同免疫的马中,也诱导产生了针对矛头蝮蛇毒抗原的特异性抗体。用编码P-II金属蛋白酶的质粒免疫诱导产生的马抗体在蛋白质印迹中与矛头蝮蛇、杜氏猪鼻蝮和窄头竹叶青蛇毒的几种蛋白质发生交叉反应,表明克隆的金属蛋白酶与这些蛇毒中存在的其他金属蛋白酶之间存在抗原相似性。此外,用编码P-II金属蛋白酶的质粒免疫诱导产生的马抗体完全中和了整个矛头蝮蛇毒的出血活性,并部分中和了杜氏猪鼻蝮蛇毒的出血活性。所产生抗体的中和能力首次提高了通过使用钨微粒进行DNA免疫在马中开发治疗性抗蛇毒血清的可能性。

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