Cottonseed hydrolysate supplementation alters metabolic and proteomics responses in Chinese hamster ovary cell cultures

Dhara, Venkata Gayatri; Kumar, Swetha; DeVine, Lauren R.; Naik, Harnish Mukesh; Cole, Robert N.; More, Abbie J; Lau, Eduardo C.; Betenbaugh, Michael J.

doi:10.1002/biot.202200243

Cited by 3 publications

(4 citation statements)

References 101 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…There were numerous publications demonstrated the continuous supply of nutrients through the fed-batch possibly promoted glycolysis, aminoacyl-tRNA biosynthesis and TCA cycle, which might be considered to be responsible for increased mAb production. [36][37][38][39] The main pathways involved in the HS016 CHO-S cell culture process were also supported by these previous studies. Analysis of the correlated metabolic pathways of each phase was performed using the MetaboAnalyst web-server (http:// www.metaboanalyst.ca/MetaboAnalyst/) to characterize the important metabolic pathways.…”

Section: Analysis Of Metabolic Pathways For Three Cell Growth Phasessupporting

confidence: 74%

¹H NMR‐based process understanding and biochemical marker identification methodology for monitoring CHO cell culture process during commercial‐scale manufacturing

Zhao

Wan

Nie

et al. 2023

Biotechnology Journal

View full text Add to dashboard Cite

Controlling the process of CHO cell fed-batch culture is critical for biologics quality control. However, the biological complexity of cells has hampered the reliable process understanding for industrial manufacturing. In this study, a workflow was developed for the consistency monitoring and biochemical marker identification of the commercial-scale CHO cell culture process through 1 H NMR assisted with multivariate data analysis (MVDA). Firstly, a total of 63 metabolites were identified in this study object in 1 H NMR spectra of the CHO cell-free supernatants. Secondly, multivariate statistical process control (MSPC) charts were used to evaluate process consistency.According to MSPC charts, the batch-to-batch quality consistency was high, indicating the CHO cell culture process at the commercial scale was well-controlled and stable.Then, the biochemical marker identification was provided through orthogonal partial least square discriminant analysis (OPLS-DA) based S-line plots during the cell logarithmic expansion, stable growth, and decline phases. Identified biochemical markers of the three cell growth phases were as follows: L-glutamine, pyroglutamic acid, 4hydroxyproline, choline, glucose, lactate, alanine, and proline were of the logarithmic growth phase; isoleucine, leucine, valine, acetate, and alanine were of the stable growth phase; acetate, glycine, glycerin, and gluconic acid were of the cell decline phase.Additional potential metabolic pathways that might influence the cell culture phase transitions were demonstrated. The workflow proposed in this study demonstrates that the combination of MVDA tools and 1 H NMR technology is highly appealing to the research of the biomanufacturing process, and applies well to provide guidance in future work on consistency evaluation and biochemical marker monitoring of the production of other biologics.

show abstract

Section: Analysis Of Metabolic Pathways For Three Cell Growth Phasessupporting

confidence: 74%

¹H NMR‐based process understanding and biochemical marker identification methodology for monitoring CHO cell culture process during commercial‐scale manufacturing

Zhao

Wan

Nie

et al. 2023

Biotechnology Journal

View full text Add to dashboard Cite

show abstract

“…Spent media collected were subjected to metabolite profiling using GC‐MS (Agilent 7890 GC with 5977 MSD). Extracellular concentrations of pyruvate, alanine, glycine, serine, aspartate, asparagine, and glutamate were measured using a GC‐MS‐based method used in previous studies (Dhara et al, 2023; Long & Antoniewicz, 2019; Y. Chen et al, 2019). Estimation of cell‐specific consumption rates ( q s ) were calculated using the following equation (Pan et al, 2017):

{C}_{s}(t)-{C}_{s}(0)={q}_{s}{IVCD}

, where

{C}_{s}(t)

is the concentration of substrate S at time t,

{C}_{s}(0)

is the concentration of substrate S at the start of the culture.…”

Section: Methodsmentioning

confidence: 99%

“…Extracellular concentrations of pyruvate, alanine, glycine, serine, aspartate, asparagine, and glutamate were measured using a GC-MSbased method used in previous studies (Dhara et al, 2023;Long & Antoniewicz, 2019;. Estimation of cell-specific consumption rates (q s ) were calculated using the following equation (Pan et al, 2017):…”

Section: Extracellular and Intracellular Metabolite Profilingmentioning

confidence: 99%

Chemical inhibitors of hexokinase‐2 enzyme reduce lactate accumulation, alter glycosylation processing, and produce altered glycoforms in CHO cell cultures

Naik

Kumar

Reddy

et al. 2023

Biotech & Bioengineering

Self Cite

View full text Add to dashboard Cite

Chinese hamster ovary (CHO) cells, predominant hosts for recombinant biotherapeutics production, generate lactate as a major glycolysis by‐product. High lactate levels adversely impact cell growth and productivity. The goal of this study was to reduce lactate in CHO cell cultures by adding chemical inhibitors to hexokinase‐2 (HK2), the enzyme catalyzing the conversion of glucose to glucose 6‐phosphate, and examine their impact on lactate accumulation, cell growth, protein titers, and N‐glycosylation. Five inhibitors of HK2 enzyme at different concentrations were evaluated, of which 2‐deoxy‐ d‐glucose (2DG) and 5‐thio‐ d‐glucose (5TG) successfully reduced lactate accumulation with only limited impacts on CHO cell growth. Individual 2DG and 5TG supplementation led to a 35%–45% decrease in peak lactate, while their combined supplementation resulted in a 60% decrease in peak lactate. Inhibitor supplementation led to at least 50% decrease in moles of lactate produced per mol of glucose consumed. Recombinant EPO‐Fc titers peaked earlier relative to the end of culture duration in supplemented cultures leading to at least 11% and as high as 32% increase in final EPO‐Fc titers. Asparagine, pyruvate, and serine consumption rates also increased in the exponential growth phase in 2DG and 5TG treated cultures, thus, rewiring central carbon metabolism due to low glycolytic fluxes. N‐glycan analysis of EPO‐Fc revealed an increase in high mannose glycans from 5% in control cultures to 25% and 37% in 2DG and 5TG‐supplemented cultures, respectively. Inhibitor supplementation also led to a decrease in bi‐, tri‐, and tetra‐antennary structures and up to 50% lower EPO‐Fc sialylation. Interestingly, addition of 2DG led to the incorporation of 2‐deoxy‐hexose (2DH) on EPO‐Fc N‐glycans and addition of 5TG resulted in the first‐ever observed N‐glycan incorporation of 5‐thio‐hexose (5TH). Six percent to 23% of N‐glycans included 5TH moieties, most likely 5‐thio‐mannose and/or 5‐thio‐galactose and/or possibly 5‐thio‐N‐acetylglucosamine, and 14%–33% of N‐glycans included 2DH moieties, most likely 2‐deoxy‐mannose and/or 2‐deoxy‐galactose, for cultures treated with different concentrations of 5TG and 2DG, respectively. Our study is the first to evaluate the impact of these glucose analogs on CHO cell growth, protein production, cell metabolism, N‐glycosylation processing, and formation of alternative glycoforms.

show abstract

“…This continued until both the nutrients in the culture were completely exhausted leading to the stopping of cell growth and subsequently cell death.Typically, commercial media are designed to sustain growth for a wide range of CHO cell lines and thus contain relatively standard amounts of different nutrients utilized as part of normal cellular metabolism. Knowledge about the amino acid concentrations over the duration of the batch culture will provide us with useful information about amino acid consumption patterns of the CHO cells in culture(Dhara et al, 2023). Therefore, shown in Figure2is a heat map profile of relative levels of amino acids in CHO cells (normalized to 100%) over time for a batch cell culture process using medium A supplemented with 6 mM L-Glutamine.…”

mentioning

confidence: 99%

Addressing amino acid‐derived inhibitory metabolites and enhancing CHO cell culture performance through DOE‐guided media modifications

Ladiwala

Dhara

Jenkins

et al. 2023

Biotech & Bioengineering

Self Cite

View full text Add to dashboard Cite

Previously, we identified six inhibitory metabolites (IMs) accumulating in Chinese hamster ovary (CHO) cultures using AMBIC 1.0 community reference medium that negatively impacted culture performance. The goal of the current study was to modify the medium to control IM accumulation through design of experiments (DOE). Initial over‐supplementation of precursor amino acids (AAs) by 100% to 200% in the culture medium revealed positive correlations between initial AA concentrations and IM levels. A screening design identified 5 AA targets, Lys, Ile, Trp, Leu, Arg, as key contributors to IMs. Response surface design analysis was used to reduce initial AA levels between 13% and 33%, and these were then evaluated in batch and fed‐batch cultures. Lowering AAs in basal and feed medium and reducing feed rate from 10% to 5% reduced inhibitory metabolites HICA and NAP by up to 50%, MSA by 30%, and CMP by 15%. These reductions were accompanied by a 13% to 40% improvement in peak viable cell densities and 7% to 50% enhancement in IgG production in batch and fed‐batch processes, respectively. This study demonstrates the value of tuning specific AA levels in reference basal and feed media using statistical design methodologies to lower problematic IMs.

show abstract

Cottonseed hydrolysate supplementation alters metabolic and proteomics responses in Chinese hamster ovary cell cultures

Cited by 3 publications

References 101 publications

¹H NMR‐based process understanding and biochemical marker identification methodology for monitoring CHO cell culture process during commercial‐scale manufacturing

¹H NMR‐based process understanding and biochemical marker identification methodology for monitoring CHO cell culture process during commercial‐scale manufacturing

Chemical inhibitors of hexokinase‐2 enzyme reduce lactate accumulation, alter glycosylation processing, and produce altered glycoforms in CHO cell cultures

Addressing amino acid‐derived inhibitory metabolites and enhancing CHO cell culture performance through DOE‐guided media modifications

Contact Info

Product

Resources

About

Cottonseed hydrolysate supplementation alters metabolic and proteomics responses in Chinese hamster ovary cell cultures

Cited by 3 publications

References 101 publications

1H NMR‐based process understanding and biochemical marker identification methodology for monitoring CHO cell culture process during commercial‐scale manufacturing

1H NMR‐based process understanding and biochemical marker identification methodology for monitoring CHO cell culture process during commercial‐scale manufacturing

Chemical inhibitors of hexokinase‐2 enzyme reduce lactate accumulation, alter glycosylation processing, and produce altered glycoforms in CHO cell cultures

Addressing amino acid‐derived inhibitory metabolites and enhancing CHO cell culture performance through DOE‐guided media modifications

Contact Info

Product

Resources

About

¹H NMR‐based process understanding and biochemical marker identification methodology for monitoring CHO cell culture process during commercial‐scale manufacturing

¹H NMR‐based process understanding and biochemical marker identification methodology for monitoring CHO cell culture process during commercial‐scale manufacturing