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Rapid purification of recombinant dengue and West Nile virus envelope Domain III proteins by metal affinity membrane chromatography

机译:金属亲和膜色谱法快速纯化重组登革热和西尼罗河病毒包膜域III蛋白

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Arthropod-borne flaviviruses such as dengue virus (DENV) and West Nile virus (WNV) pose significant health threats to the global community. Due to escalating numbers of DENV and WNV infections worldwide, development of an effective vaccine remains a global health priority. As flavivirus envelope Domain III (DIII) protein is highly immunogenic and capable of inducing neutralizing antibodies against wild-type virus, it is both a potential protein subunit vaccine candidate and a suitable diagnostic reagent. Here, we describe the use of metal affinity membrane chromatography as a rapid and improved alternative for the purification of recombinant DIII (rDIII) antigens from DENV serotypes 1-4 and WNV - New York, Sarafend, Wengler and Kunjin strains. Optimum conditions for the expression, solubilization, renaturation and purification of these proteins were established. The purified proteins were confirmed by MALDI-TOF mass spectrometry and ELISA using antibodies raised against the respective viruses. Biological function of the purified rDIII proteins was confirmed by their ability to generate DIII-specific antibodies in mice that could neutralize the virus.
机译:节肢动物传播的黄病毒,例如登革热病毒(DENV)和西尼罗河病毒(WNV),对全球社会构成了严重的健康威胁。由于全世界DENV和WNV感染数量的增加,开发有效的疫苗仍然是全球健康的重点。由于黄病毒包膜域III(DIII)蛋白具有高度免疫原性,并且能够诱导针对野生型病毒的中和抗体,因此它既是潜在的蛋白亚基疫苗候选者,又是合适的诊断试剂。在这里,我们描述了使用金属亲和膜色谱作为从DENV血清型1-4和WNV-纽约,萨拉芬德,翁格勒和昆金菌株中纯化重组DIII(rDIII)抗原的快速和改良方法。建立了表达,溶解,复性和纯化这些蛋白的最佳条件。使用针对各个病毒的抗体,通过MALDI-TOF质谱和ELISA确认了纯化的蛋白质。纯化的rDIII蛋白的生物学功能通过其在小鼠中产生DIII特异性抗体的能力得以证实,该抗体可以中和病毒。

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