Cloning, Expression, Re-folding, and Purification of Protein Flic (salmonella Enteritidis) with Deletion of Amino Acids 220-320

VNU Journal of Science: Natural Sciences and Technology Pub Date : 2022-10-25 DOI:10.25073/2588-1140/vnunst.4966

N. Anh, Trần Huỳnh Bảo Châu, Nguyen Phuoc Khai Hoan, T. Hiếu

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Abstract

In order to develop high-performance subunit vaccines, many studies are currently aiming at the development of immunoadjuvants. Flagellin protein (FliC) contained in the Salmonella’s filament is one of the potential candidates for this purpose. However, the high antigenic property of FliC has made it difficult to apply for many vaccines. A variant with the deletion of amino acids from 220 to 320 of flagellin has been proven to have an adjuvant effect with lower immunogenicity. In this present study, we cloned and expressed FliCD220-320 recombinant in Escherichia coli system. The expression of FliCΔ220-320 was induced by IPTG and confirmed by SDS-PAGE and Western Blot probed with 6xHis tag antibody. Results showed that most of the expressed protein is insoluble. The targeted protein was then solubilized, re-folded and purified by affinity chromatography method with the purity of 80 %. With these results, we successfully expressed FliCD220-320 recombinant protein and this is a source for the evaluation and development of immune adjuvants.

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氨基酸缺失蛋白片段(肠炎沙门氏菌)的克隆、表达、重折叠和纯化

为了开发高性能的亚单位疫苗，目前许多研究都瞄准了免疫佐剂的开发。沙门氏菌丝中含有的鞭毛蛋白(FliC)是这一目的的潜在候选者之一。然而，FliC的高抗原性使其难以应用于许多疫苗。一种缺失鞭毛蛋白220到320个氨基酸的变体已被证明具有较低免疫原性的佐剂作用。本研究在大肠杆菌体系中克隆并表达了FliCD220-320重组蛋白。用IPTG诱导FliCΔ220-320表达，用SDS-PAGE和6xHis标记抗体检测Western Blot证实。结果表明，大部分表达蛋白是不溶性的。然后将目标蛋白溶解，重新折叠，用亲和层析法纯化，纯度为80%。根据这些结果，我们成功表达了FliCD220-320重组蛋白，这为免疫佐剂的评价和开发提供了一个来源。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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VNU Journal of Science: Natural Sciences and Technology

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