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Expression, purification, and molecular analysis of the Necator americanus glutathione S-transferase 1 (Na-GST-1): A production process developed for a lead candidate recombinant hookworm vaccine antigen

机译:美洲轮虫谷胱甘肽S-转移酶1(Na-GST-1)的表达,纯化和分子分析:为候选候选重组钩虫疫苗抗原开发的生产工艺

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The enzyme Necator americanus glutathione S-transferase 1 (Na-GST-1) belongs to a unique Nu class of GSTs and is a lead candidate antigen in a bivalent human hookworm vaccine. Here we describe the expression of Na-GST-1 in the yeast Pichia pastoris at the 20 L manufacturing scale and its purification process performed by three chromatographic steps, comprised of a Q Sepharose XL anion exchange column, followed by a Butyl Sepharose HP hydrophobic affinity column and a Superdex 75 size-exclusion column. Approximately 1.5 g of recombinant protein was recovered at an overall process yield of 51%, with a purity grade of 98% and the absence of detectable host cell protein. By mass spectrometry the recombinant protein exhibits a mass of 23,676 Da, which closely matches the predicted molecular mass of the protein. The expression and purification methods described here are suitable for further scale-up product development and for its use to design formulation processes suitable to generate a vaccine for clinical testing.
机译:美洲轮虫谷胱甘肽S-转移酶1(Na-GST-1)酶属于独特的Nu类GST,是二价人钩虫疫苗中的主要候选抗原。在这里,我们描述了Na-GST-1在酵母毕赤酵母中以20 L的生产规模表达及其纯化过程,该过程由三个色谱步骤执行,包括Q Sepharose XL阴离子交换柱,然后是丁基Sepharose HP疏水亲和力色谱柱和Superdex 75尺寸排阻色谱柱。回收到约1.5 g重组蛋白,总工艺收率为51%,纯度为98%,并且没有可检测的宿主细胞蛋白。通过质谱分析,重组蛋白的质量为23676 Da,与预测的蛋白分子量非常匹配。本文所述的表达和纯化方法适用于进一步扩大规模的产品开发,并且适用于设计适合于产生用于临床测试的疫苗的配制过程。

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