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人唾液酸转移酶的共表达提高了非洲爪蟾内 N-糖基化水平,并优化了人源化治疗性糖蛋白 IFN-β的生产。

Co-expression of human sialyltransferase improves N-glycosylation in Leishmania tarentolae and optimizes the production of humanized therapeutic glycoprotein IFN-beta.

机构信息

Departamento de Bioquímica e Biologia Molecular, Universidade Federal de Viçosa, Av. P. H, Rolfs s/n, Viçosa 36570-900, Brazil.

Departamento de Bioquímica e Biologia Molecular, Universidade Federal de Viçosa, Av. P. H, Rolfs s/n, Viçosa 36570-900, Brazil.

出版信息

J Biotechnol. 2024 Nov 10;394:24-33. doi: 10.1016/j.jbiotec.2024.08.002. Epub 2024 Aug 4.

DOI:10.1016/j.jbiotec.2024.08.002
PMID:39103019
Abstract

The production of therapeutic glycoproteins is primarily expensive due to the necessity of culturing mammalian cells. These systems often require complex and costly culture media and typically yield low amounts of protein. Leishmania tarentolae, a non-pathogenic protozoan to mammals, has emerged as a cost-effective alternative system for heterologous glycoprotein expression due to its suitability for large-scale production using low-cost culture media, and its ability to perform mammalian-like post-translational modifications, including glycosylation. Nevertheless, differences in the carbohydrate residues at the end of N-glycan chains are observed in Leishmania compared to mammalian cells due to the absence of biosynthetic enzymes in Leishmania that are required for the incorporation of terminal sialic acid. In this study, a genetically optimized L. tarentolae cell line was engineered for the production of recombinant interferon-β (IFN-β) featuring a complete mammalian N-glycosylation profile. Genomic and metabolomic analyses revealed that heterologous expression of the sialyltransferase enzyme and cultivation in a medium containing sialic acid were sufficient to generate mammalian-like protein N-glycosylation. N-glycan mass spectrometry analysis demonstrated a glycosylation pattern compatible with the incorporation of sialic acid into the glycan structure. In vitro IFN-β activity indicated that the expressed protein exhibited reduced inflammatory effects compared to IFN-beta produced by other platforms, such as bacteria, non-optimized L. tarentolae, and mammalian cells.

摘要

治疗性糖蛋白的生产主要很昂贵,因为需要培养哺乳动物细胞。这些系统通常需要复杂且昂贵的培养基,并且通常产生低量的蛋白质。利什曼原虫(Leishmania tarentolae)是一种对哺乳动物无致病性的原生动物,由于其适合使用低成本培养基进行大规模生产,并且能够进行类似于哺乳动物的翻译后修饰,包括糖基化,因此已成为异源糖蛋白表达的具有成本效益的替代系统。然而,与哺乳动物细胞相比,利什曼原虫中 N-糖链末端的碳水化合物残基存在差异,这是由于利什曼原虫中缺乏用于掺入末端唾液酸的生物合成酶。在这项研究中,通过基因优化,构建了一种能够产生具有完整哺乳动物 N-糖基化特征的重组干扰素-β(IFN-β)的利什曼原虫细胞系。基因组和代谢组学分析表明,异源表达唾液酸转移酶和在含有唾液酸的培养基中培养足以产生类似于哺乳动物的蛋白 N-糖基化。N-糖链质谱分析表明,糖基化模式与糖链结构中唾液酸的掺入兼容。体外 IFN-β 活性表明,与其他平台(如细菌、非优化的利什曼原虫和哺乳动物细胞)产生的 IFN-β 相比,表达的蛋白表现出降低的炎症作用。

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