Cell Culture Processes in Monoclonal Antibody Production

Li, Feng; Shen, Amy; Amanullah, Ashraf

doi:10.1002/9780470571224.pse506

Cited by 63 publications

(87 citation statements)

References 92 publications

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“…Such loss of production between initial and end-of-production cells might compromise regulatory approval and, in the worst-case scenario, could result in rejection of a particular cell line after months of wasted development effort (Barnes et al 2003). In addition to cell line stability, growth and metabolite characteristics affecting process robustness and scalability also need to be assessed (Li et al 2010). Despite the mAb tendency to lose productivity over a time, the limit in the number of passages that a given cell can be subjected to without impinging on its stability is singular to each cell line (Lee et al 1991).…”

Section: Introductionmentioning

confidence: 99%

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Effects of passage number on growth and productivity of hybridoma secreting MRSA anti-PBP2a monoclonal antibodies

Corrêa

Senna²,

Sousa³

2015

Cytotechnology

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Monoclonal antibodies (mAb) are high added value glycoproteins recommended for immunotherapy, diagnosis, and also for the treatment of bacterial infections resistant to multiple drugs such as Methicillin Resistant Staphylococcus aureus (MRSA). In addition to environmental conditions related to cell cultures, the intrinsic characteristics of hybridoma cells, like the secretion stability of monoclonal antibodies by the cells through successive subcultures, are relevant for the characterization of cell lines related to the productivity of mAb. The rate of mAb production differs significantly between different cell lines and different passage numbers, and it is an important variable in characterization of cell lines. In order to find a more robust, fastergrowing, and higher-productivity cell line of hybridoma, cultivations in 24-well plates were performed in different subculture periods, or cell passages (P), of hybridoma cells producing MRSA anti-PBP2a monoclonal antibodies ]. The objective of this study was to study the effects of cell growth and production of MRSA-antiPBP2a mAb secreted by murine hybridoma cells grown in different passages as well as determine the which passages the hybridomas can be cultivated without harming their growth and productivity. So, cell growth profiles of hybridomas secreting MRSA-antiPBP2a (mAb) and the production of MRSA-antiPBP2a mAb in different subculture periods or cell passages (P) were studied. Cell growth tests, monoclonal antibody productivity, and metabolite characteristics revealed substantial differences in those cells kept between P10 and P50. Similarities in the secretion of monoclonal antibody, growth, and metabolic profiles, were noted in the MRSA-antiPBP2a mAb producing hybridoma cells kept between P10 and P20. Also, glucose consumption (g/L) and lactate production (g/L) in the latter cell cultures were monitored daily through biochemical analyzer. As of P30, it was observed a 4.4 times reduction in productivity, a 13 % reduction in metabolic yield, and a significant change in cell growth. Secretion of MRSA-antiPBP2a mAb should be obtained through the culture of hybridomas up to P20 in order to keep its stability.

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Section: Introductionmentioning

confidence: 99%

“…Considering cost-effectiveness, it is important to have a cell line secreting proteins or antibodies of interest for development of diagnostics kits (Barnes et al 2003;Schmid et al 1990;Xin and Cutler 2006;Beckmann et al 2012;Kim et al 2011;Li et al 2010;Lee et al 1991). …”

Section: Introductionmentioning

confidence: 99%

Effects of passage number on growth and productivity of hybridoma secreting MRSA anti-PBP2a monoclonal antibodies

Corrêa

Senna²,

Sousa³

2015

Cytotechnology

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“…When antibodies began to enter the development pipelines, the biotech manufacturing changed over to fed-batch mainly due to productivity reasons. Antibody therapies may require large doses over a long period of time 33 . In that context, many companies have built large-scale facilities of working volumes ≥ 10,000 L. In the mid-2000, product titers of 5 g/L at the end of the production have become the industry standard 8 .…”

Section: Cell Culture Process Optimizationmentioning

confidence: 99%

“…In that context, many companies have built large-scale facilities of working volumes ≥ 10,000 L. In the mid-2000, product titers of 5 g/L at the end of the production have become the industry standard 8 . Nowadays, biotechnology companies are reporting productivities as high as 10-13 g/L in a fed-batch culture of 2-3 weeks 33,34 .…”

Section: Cell Culture Process Optimizationmentioning

confidence: 99%

“…These also called high-molecular-weight species (HMW) have to be limited to avoid immunogenic reactions in the injected patients. It is also important to keep in mind that the productivity of recombinant cell culture processes has substantially increased from 50 mg/L in batch to titers of 10 to 13 g/L nowadays in fed-batch culture of 2 to 3 weeks 33,34 . Moreover, the literature describes how cell culture conditions can be identified to control protein aggregation in CHO cell cultures 54 .…”

Section: Introductionmentioning

confidence: 99%

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Tailoring recombinant protein quality by rational media design

Brühlmann

Jordan

Hemberger³

et al. 2015

Biotechnology Progress

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Clinical efficacy and safety of recombinant proteins are closely associated with their structural characteristics. The major quality attributes comprise glycosylation, charge variants (oxidation, deamidation, and C‐ & N‐terminal modifications), aggregates, low‐molecular‐weight species (LMW), and misincorporation of amino acids in the protein backbone. Cell culture media design has a great potential to modulate these quality attributes due to the vital role of medium in mammalian cell culture. The purpose of this review is to provide an overview of the way both classical cell culture medium components and novel supplements affect the quality attributes of recombinant therapeutic proteins expressed in mammalian hosts, allowing rational and high‐throughput optimization of mammalian cell culture media. A selection of specific and/or potent inhibitors and activators of oligosaccharide processing as well as components affecting multiple quality attributes are presented. Extensive research efforts in this field show the feasibility of quality engineering through media design, allowing to significantly modulate the protein function. © 2015 American Institute of Chemical Engineers Biotechnol. Prog., 31:615–629, 2015

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Avian embryos and related cell lines: A convenient platform for recombinant proteins and vaccine production

Farzaneh

Hassani

Mozdziak³

et al. 2017

Biotechnology Journal

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Chick embryos are a significant historical research model in basic and applied sciences. The embryonated eggs have been used for virus inoculation in order to vaccine production for nearly a century. Recently, avian eggs and cell lines derived from embryonated eggs have found wide application in biotechnology. This review will discuss about the unique characteristics of avian eggs in terms of safety, large scale and economical production of recombinant proteins. This system also provides the human-like glycosylation on target proteins and therefore can be considered as a suitable host for biomanufacturing of humanized monoclonal antibodies and therapeutic proteins. Avian derived cell lines are an alternative for rapid vaccine manufacturing during a pandemic. Based on the latest knowledge in cell and animal transgenesis, the currently available germ cell-mediated gene transfer system provides a more efficient strategy in gene targeting and creation of transgenic birds that lead to advancements in industrial, biotechnology, and biological research applications. This review covers the recent development of avian fertilized eggs and related cell lines in a variety of human biopharmaceuticals and viral vaccine manufacturing.

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Cell Culture Processes in Monoclonal Antibody Production

Cited by 63 publications

References 92 publications

Effects of passage number on growth and productivity of hybridoma secreting MRSA anti-PBP2a monoclonal antibodies

Effects of passage number on growth and productivity of hybridoma secreting MRSA anti-PBP2a monoclonal antibodies

Tailoring recombinant protein quality by rational media design

Avian embryos and related cell lines: A convenient platform for recombinant proteins and vaccine production

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