Influence of protein and carbohydrate contents of soy protein hydrolysates on cell density and IgG production in animal cell cultures

Gupta, Abhishek; Wierenga, Peter A.; Gruppen, Harry; Boots, Jan-Willem P.

doi:10.1002/btpr.2121

Cited by 11 publications

(3 citation statements)

References 38 publications

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“…Exopeptidases were not chosen in order to avoid the production of free amino acids. Improved CHO cell growth and/or productivity were so far reported for commercial or in-house produced protein hydrolysates made from soy [20][21][22], wheat [21][22][23], cotton [22], rice [23,24], and rapeseeds [25]. CHO cells were applied for the assessment of antioxidant potential of perilla seeds' protein hydrolysate [26] as well as for chemometric analysis of metabolized soy protein hydrolysate [27].…”

Section: Introductionmentioning

confidence: 99%

Protein Hydrolysates from Flaxseed Oil Cake as a Media Supplement in CHO Cell Culture

et al. 2021

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This is the first report about flaxseed protein hydrolysates applied as media supplements in CHO cell culture. The hydrolysates were produced by three separate enzymatic digestions of proteins isolated from flaxseed oil cake. The enzymes used were Alcalase, Neutrase, and Protamex, and the most efficient hydrolysis was achieved with Alcalase. The three hydrolysates were first tested as a partial substitute for serum in basal media in order to evaluate their effects on the adherent IgG-producing CHO cell line. The cells that grew in such media reached higher density than the cells in media supplemented with serum only. Consequently, the increased cell number improved the final IgG titer. In the next experiment, the impact of hydrolysates was evaluated in suspension CHO culture adapted to chemically defined media. In this preliminary investigation, the cells showed no response to the hydrolysate addition concerning the growth rate and productivity. Despite this outcome, we speculate that low molecular mass components in the hydrolysates, besides nutritive, may have a cell-protective function.

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Section: Introductionmentioning

confidence: 99%

Protein Hydrolysates from Flaxseed Oil Cake as a Media Supplement in CHO Cell Culture

et al. 2021

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“…Many kinds of materials have replaced the role of serum in cell culture (Zhao et al 2017), but most of these materials contain undefined raw materials that were derived from microbes, such as hydrolysates (Gupta et al 2015). Therefore, we focused on developing a defined medium.…”

Section: Introductionmentioning

confidence: 99%

A serum-free medium suitable for maintaining cell morphology and liver-specific function in induced human hepatocytes

Liang

et al. 2019

Cytotechnology

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hiHep is a new type of hepatocyte-like cell that is predicted to be a potential unlimited source of hepatocytes for a bioartificial liver. However, hiHep cannot currently be used in clinical settings because serum must be added during the culture process. Thus, a defined medium is required. Because serum is complex, an efficient statistical approach based on the Plackett-Burman design was used. In this manner, an original medium and several significant cell growth factors were identified. These factors include insulin, V H , and V E , and the original medium was optimized based on these significant factors. Additionally, hiHep liver-specific functions and metabolism in the optimized serum-free medium were measured. Results showed that hiHep functions, such as glycogen storage, albumin secretion, and urea production, were well maintained in our optimized serum-free medium. In summary, we created a chemically defined, serumfree medium in which cell growth, proliferation, metabolism, and function were well maintained. This medium has the potential to support the clinical use of hiHep.

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“…and proteins (bovine serum albumin, transferrin, etc.) [ 6 – 9 ]. Therefore, current medium development has been focusing on the chemically defined media.…”

Section: Introductionmentioning

confidence: 99%

Use of real-time cellular analysis and Plackett-Burman design to develop the serum-free media for PC-3 prostate cancer cells

et al. 2017

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In this study, we developed a rapid strategy to screen a serum-free medium for culturing the anchorage-dependent PC-3 prostate cancer cells, which was going to be prepared in large scale to generate GM-CSF/TNFα-surface-modified whole cell prostate cancer vaccine. Automated real-time cellular analysis as a rapid and non-invasive technology was used to monitor the growth of PC-3 cells in 16-well plates. At the same time, Plackett-Burman design was employed to identify the most influential formulation by integrating relevant information statistically. The effects of the 16 selected factors were evaluated during exponential cell growth and three medium constituents (EGF, FGF and linoleic acid) were identified to have significant effects on the cell growth. Subsequently, the response surface methodology with central composite design was applied to determine the interactions among the three factors so that these factors were optimized to improve cell growth. Finally, the prediction of the best combination was made under the maximal response to optimize cell growth by Design-Expert software 7.0. A total of 20 experiments were conducted to construct a quadratic model and a second-order polynomial equation. With the optimized combination validated by the stability test of serial passaging PC-3 cells, the serum-free medium had similar cell density and cell viability to the original serum medium. In summary, this high-throughput scheme minimized the screening time and may thus provide a new platform to efficiently develop the serum-free media for adherent cells.

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Influence of protein and carbohydrate contents of soy protein hydrolysates on cell density and IgG production in animal cell cultures

Cited by 11 publications

References 38 publications

Protein Hydrolysates from Flaxseed Oil Cake as a Media Supplement in CHO Cell Culture

Protein Hydrolysates from Flaxseed Oil Cake as a Media Supplement in CHO Cell Culture

A serum-free medium suitable for maintaining cell morphology and liver-specific function in induced human hepatocytes

Use of real-time cellular analysis and Plackett-Burman design to develop the serum-free media for PC-3 prostate cancer cells

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