Untitled

Hendrick, V.; Winnepenninckx, P.; Abdelkafi, C; Vandeputte, Olivier M.; Cherlet, Marc; Marique, Thierry; Renemann, G.; Loa, A.; Kretzmer, G.; Wérenne, John

doi:10.1023/a:1014088919546

Cited by 110 publications

(35 citation statements)

References 26 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…An increase of the antibody production has been mostly described during the G0 or G1 phase for hybridoma or CHO cells ( Kim, & Lee, 2016;Suzuki & Ollis, 1989). In contrast to our study, temperature shifts or butyrate treatment were used to arrest the cell cycle in the G1 phase and therefore enrich G0 cells with assumed higher productivity in the stationary phase, in which most of the product is formed (Du et al, 2015;Hendrick et al, 2001;Münzer et al, 2015;Wippermann et al, 2017). Since no net mitotic growth and no progress of the cells throughout the cell cycle takes place in the stationary phase, this phase was not considered in this study, which focuses on the influence of cell cycle and growthassociated autocrine factors.…”

Section: Discussionmentioning

confidence: 81%

Model‐based identification of cell‐cycle‐dependent metabolism and putative autocrine effects in antibody producing CHO cell culture

Möller

Korte

Pörtner

et al. 2018

Biotech & Bioengineering

View full text Add to dashboard Cite

The understanding of cell-cycle-dependent population heterogeneities in mammalian cell culture and their influence on production rates is still limited. Furthermore, metabolic regulations arising from self-expressed signaling factors (autocrine/autoinhibitory factors) have been postulated in the past, but no determination of such effects have been made so far for fast-growing production Chinese hamster ovary (CHO) cells in chemically defined media. In this study, a novel approach combining near-physiological treatment of cells (including synchronization), population resolved mechanistic modeling and statistical analysis was developed to identify population inhomogeneities. Cell-cycle-dependent population dynamics and metabolic regulations due to a putative autocrine factor were examined and their impact on the metabolic rates and antibody production of near-physiologically synchronized CHO DP-12 cell cultures was determined. To achieve this, a population resolved model was extended to describe putative autocrine-dependentt and cell-cycle-related metabolic rates for glucose, glutamine, lactate, ammonia, and antibody production. The model parameters were estimated based on data of two repeated batch cultivations (three batches each), with main substrates in excess and potentially inhibiting waste products (lactate and ammonium) controlled within narrow ranges. Significant changes, due to a putative autocrine factor, were identified for lactate and ammonia formation and antibody production. The cell growth and the uptake of glucose and glutamine were only partially affected by the putative autocrine under the given conditions. The results indicate the presence of a self-expressed autocrine factor and its strong impact on the metabolism of CHO DP-12 cells. Furthermore, glucose and glutamine uptake, as well as the formation of ammonium and antibody were found to be significantly cell-cycle-dependent. The combined approach has a strong potential to improve the understanding of the interplay of population heterogeneities and signal factors in mammalian cell culture.

show abstract

Section: Discussionmentioning

confidence: 81%

Model‐based identification of cell‐cycle‐dependent metabolism and putative autocrine effects in antibody producing CHO cell culture

Möller

Korte

Pörtner

et al. 2018

Biotech & Bioengineering

View full text Add to dashboard Cite

show abstract

“…Toward this end, an adherent CHO‐K1‐derived cell line that secretes recombinant human

β

‐glucuronidase was adapted for growth in serum‐free chemically defined medium , and a cell bank was established. As butyrate has been previously shown to increase protein production in CHO cells in a number of bioproduction models , we evaluated its utility to increase production of human

β

‐glucuronidase.…”

Section: Resultsmentioning

confidence: 99%

Evaluation of butyrate‐induced production of a mannose‐6‐phosphorylated therapeutic enzyme using parallel bioreactors

Madhavarao

Agarabi

Wong

et al. 2014

Biotech and App Biochem

View full text Add to dashboard Cite

Bioreactor process changes can have a profound effect on the yield and quality of biotechnology products. Mannose-6-phosphate (M6P) glycan content and the enzymatic catalytic kinetic parameters are critical quality attributes (CQAs) of many therapeutic enzymes used to treat lysosomal storage diseases (LSDs). Here, we have evaluated the effect of adding butyrate to bioreactor production cultures of human recombinant β-glucuronidase produced from CHO-K1 cells, with an emphasis on CQAs. The β-glucuronidase produced in parallel bioreactors was quantified by capillary electrophoresis, the catalytic kinetic parameters were measured using steady-state analysis, and mannose-6-phosphorylation status was assessed using an M6P-specific single-chain antibody fragment. Using this approach, we found that butyrate treatment increased β-glucuronidase production up to approximately threefold without significantly affecting the catalytic properties of the enzyme. However, M6P content in β-glucuronidase was inversely correlated with the increased enzyme production induced by butyrate treatment. This assessment demonstrated that although butyrate dramatically increased β-glucuronidase production in bioreactors, it adversely impacted the mannose-6-phosphorylation of this LSD therapeutic enzyme. This strategy may have utility in evaluating manufacturing process changes to improve therapeutic enzyme yields and CQAs.

show abstract

“…Mild hypothermia has been reported to increase the specific productivity of a number of recombinant proteins (Furukawa and Ohsuye 1998;Kaufmann et al 1999;Hendrick et al 2001;Ducommun et al 2002;Yoon et al 2003;Fox et al 2004). In our studies, the specific productivity of SEAP at 33°C was higher than the productivity before the temperature shift or the productivity of the singletemperature culture, regardless of culture condition (i.e., suspension or microcarrier).…”

Section: Discussionmentioning

confidence: 99%

The effects of microcarrier culture on recombinant CHO cells under biphasic hypothermic culture conditions

2009

View full text Add to dashboard Cite

A Chinese hamster ovary (CHO) cell line, producing recombinant secreted human placental alkaline phosphatase (SEAP) was investigated under three different culture conditions (suspension cells, cells attached to Cytodex 3 and Cytopore 1 microcarriers) in a biphasic culture mode using a temperature shift to mild hypothermic conditions (33 degrees C) in a fed-batch bioreactor. The cell viability in both the suspension and the Cytodex 3 cultures was maintained for significantly longer periods under hypothermic conditions than in the single-temperature cultures, leading to higher integrated viable cell densities. For all culture conditions, the specific productivity of SEAP increased after the temperature reduction; the specific productivities of the microcarrier cultures increased approximately threefold while the specific productivity of the suspension culture increased nearly eightfold. The glucose and glutamine consumption rates and lactate and ammonia production rates were significantly lowered after the temperature reduction, as were the yields of lactate from glucose. However, the yield of ammonia from glutamine increased in response to the temperature shift.

show abstract

Untitled

Cited by 110 publications

References 26 publications

Model‐based identification of cell‐cycle‐dependent metabolism and putative autocrine effects in antibody producing CHO cell culture

Model‐based identification of cell‐cycle‐dependent metabolism and putative autocrine effects in antibody producing CHO cell culture

Evaluation of butyrate‐induced production of a mannose‐6‐phosphorylated therapeutic enzyme using parallel bioreactors

The effects of microcarrier culture on recombinant CHO cells under biphasic hypothermic culture conditions

Contact Info

Product

Resources

About