Identification of novel inhibitory metabolites and impact verification on growth and protein synthesis in mammalian cells

IF 3.7 Q2 BIOTECHNOLOGY & APPLIED MICROBIOLOGY

Metabolic Engineering Communications Pub Date : 2021-12-01 DOI:10.1016/j.mec.2021.e00182

Bingyu Kuang , Venkata Gayatri Dhara , Duc Hoang , Jack Jenkins , Pranay Ladiwala , Yanglan Tan , Scott A. Shaffer , Shaun C. Galbraith , Michael J. Betenbaugh , Seongkyu Yoon

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引用次数: 7

Abstract

Mammalian cells consume large amount of nutrients during growth and production. However, endogenous metabolic inefficiencies often prevent cells to fully utilize nutrients to support growth and protein production. Instead, significant fraction of fed nutrients is diverted into extracellular accumulation of waste by-products and metabolites, further inhibiting proliferation and protein synthesis. In this study, an LC-MS/MS based metabolomics pipeline was used to screen Chinese hamster ovary (CHO) extracellular metabolites. Six out of eight identified inhibitory metabolites, caused by the inefficient cell metabolism, were not previously studied in CHO cells: aconitic acid, 2-hydroxyisocaproic acid, methylsuccinic acid, cytidine monophosphate, trigonelline, and n-acetyl putrescine. When supplemented back into a fed-batch culture, significant reduction in cellular growth was observed in the presence of each metabolite and all the identified metabolites were shown to impact the glycosylation of a model secreted antibody, with seven of these also reducing CHO cellular productivity (titer) and all eight inhibiting the formation of mono-galactosylated biantennary (G1F) and biantennary galactosylated (G2F) N-glycans. These inhibitory metabolites further impact the metabolism of cells, leading to a significant reduction in CHO cellular growth and specific productivity in fed-batch culture (maximum reductions of 27.2% and 40.6% respectively). In-depth pathway analysis revealed that these metabolites are produced when cells utilize major energy sources such as glucose and select amino acids (tryptophan, arginine, isoleucine, and leucine) for growth, maintenance, and protein production. Furthermore, these novel inhibitory metabolites were observed to accumulate in multiple CHO cell lines (CHO–K1 and CHO-GS) as well as HEK293 cell line. This study provides a robust and holistic methodology to incorporate global metabolomic analysis into cell culture studies for elucidation and structural verification of novel metabolites that participate in key metabolic pathways to growth, production, and post-translational modification in biopharmaceutical production.

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新型抑制代谢物的鉴定及其对哺乳动物细胞生长和蛋白质合成的影响验证

哺乳动物细胞在生长和生产过程中消耗大量的营养物质。然而，内源性代谢效率低下往往阻止细胞充分利用营养来支持生长和蛋白质生产。相反，大量的营养物质被转移到细胞外积累的废物副产品和代谢物中，进一步抑制了增殖和蛋白质合成。本研究采用基于LC-MS/MS的代谢组学方法筛选中国仓鼠卵巢(CHO)细胞外代谢物。由细胞代谢效率低下引起的8种已确定的抑制性代谢物中有6种以前未在CHO细胞中研究过:乌头酸、2-羟基异己酸、甲基琥珀酸、单磷酸胞苷、葫芦巴碱和n-乙酰腐胺。当补充回补料批培养时，观察到每种代谢物存在时细胞生长显著减少，所有鉴定的代谢物都显示影响模型分泌抗体的糖基化，其中7种也降低CHO细胞生产力(滴度)，所有8种都抑制单半乳糖化双天线(G1F)和双天线半乳糖化(G2F) n -聚糖的形成。这些抑制性代谢物进一步影响细胞的代谢，导致CHO细胞生长和比产率显著降低(最大降幅分别为27.2%和40.6%)。深入的途径分析表明，当细胞利用葡萄糖等主要能量来源和选择氨基酸(色氨酸、精氨酸、异亮氨酸和亮氨酸)进行生长、维持和蛋白质生产时，这些代谢物就会产生。此外，这些新的抑制性代谢物被观察到在多种CHO细胞系(CHO - k1和CHO- gs)以及HEK293细胞系中积累。本研究提供了一种强大而全面的方法，将全球代谢组学分析纳入细胞培养研究，以阐明和结构验证参与生物制药生产中生长，生产和翻译后修饰关键代谢途径的新型代谢物。

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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来源期刊

Metabolic Engineering Communications Medicine-Endocrinology, Diabetes and Metabolism

CiteScore

13.30

自引率

1.90%

发文量

审稿时长

18 weeks

期刊介绍： Metabolic Engineering Communications, a companion title to Metabolic Engineering (MBE), is devoted to publishing original research in the areas of metabolic engineering, synthetic biology, computational biology and systems biology for problems related to metabolism and the engineering of metabolism for the production of fuels, chemicals, and pharmaceuticals. The journal will carry articles on the design, construction, and analysis of biological systems ranging from pathway components to biological complexes and genomes (including genomic, analytical and bioinformatics methods) in suitable host cells to allow them to produce novel compounds of industrial and medical interest. Demonstrations of regulatory designs and synthetic circuits that alter the performance of biochemical pathways and cellular processes will also be presented. Metabolic Engineering Communications complements MBE by publishing articles that are either shorter than those published in the full journal, or which describe key elements of larger metabolic engineering efforts.