Cell Culture Process Improvement Via Supplementation of Vitamins and Other Supplements
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Abstract
Monoclonal antibodies have become a key class of therapeutic agents on the market and are one of the
pharmaceutical industry's fastest-growing items right now. About eighty Mabs have received permission for
marketing. An ever-growing need exists for the process of developing monoclonal antibodies to be
optimized in a way that maximizes cost effectiveness. To do this, a thorough comprehension of the
metabolic processes found in mammalian cells is required. This will facilitate the effective optimization of
the chemical and physical parameters. The optimization of vitamin and other supplementation for an
efficient process for producing monoclonal antibodies is described in this thesis.
In this work, mammalian cell lines were used to test twelve different supplements and ten different vitamins
in fed batch method. The trials were conducted in shaking flasks with identical basal media maintained at
34°C. Every day, biochemical analysis, osmo, cell count, and sampling were carried out. The shake flasks
were collected and samples were tested for antibody titers using a Cedex biochemical analyzer once the cell
viability dropped to 50%.
Cell growth, cell viability, lactate generation, and antibody buildup in the broth were used to analyze the
results. Only one additional supplement, out of ten distinct vitamins and twelve different supplements,
significantly contributed to the improvements in Titer, VCC, Cell Viability, and reduced lactate buildup,
while the vitamins had no discernible impact. Therefore, in the most recent round of the experiment, this
additional supplement was used in certain flasks along with others that had been concentrated more. The
process was optimized in this way.
