Major advantages of perfusion are high cell numbers and high total production in a relatively small size bioreactor. Moreover, perfusion is optimal when the product of interest is unstable or if the product yield is low. On the other hand, disadvantages are for example technical challenges originating from non-robust cell separation devices as well as sterility concerns from the more complex set-up needed.

In the present work, the use of a WAVE Bioreactor™ system 20/50 in perfusion mode with10 L disposable Cellbag™ bioreactors customized with two dip tubes in combination with disposable hollow fiber filters as external cell separating devices were investigated. A comparison between Alternating Tangential Flow (ATF) and Tangential Flow Filtration (TFF) was performed using a recombinant CHO cell line producing a monoclonal antibody (mAb) as a model system.

A research cell line DHFR^- CHO producing mAb was used. During expansion cultures in shake flasks, MTX selection pressure was performed but omitted in bioreactor. A WAVE Cellbag™ (10 L) containing two dip tubes (GE Healthcare) at 4L working volume was connected either to an ATF-2 device (Refine Technology, USA) or to a ReadyToProcess™ filter (TFF) via a Watson Marlow 620S pump. In both systems, the hollow fiber filters (HF), RTPCFP-2-E-4X2MS, GE Healthcare, Sweden, had 0.2 μm pore size, 1 mm lumen and 850 cm² filter area. The pressure rising flow (ATF), the exhaust flow (ATF) and the recirculation flow rate (TFF) were 0.7 or 1 L/min. The set-points of DO, pH and temperature were 35 %, 7 and 37°C respectively. The agitation rate was varied between 20-26 rpm, 6-7° and 20-27 rpm, 6-8° for ATF and TFF respectively. O₂ addition was performed in the headspace (20-100%) and the DO control was operated by varying the agitation.

The cells were cultivated in serum-free, animal-component free IS CHO CD XP medium (Irvine Scientific, USA) with hydrolysate, supplemented with 3 % of IS-CHO Feed-CD XP (Irvine Scientific, USA) and with 4 mM glutamine with a cell specific perfusion rate of 0.05 Reactor Volume/(day x 10⁶ cells/mL). Supplementations of glucose or glutamine were performed according to cell need. The pH was controlled by adding 0.5 M Na₂CO₃ or pulsing CO₂ into the headspace. The cell density, viability, pH, pCO₂, concentrations of glucose, lactate, glutamine and ammonia were measured by Bioprofile FLEX (Nova Biomedical). Antifoam C (Sigma Aldrich, US) was added up to 50 ppm concentration in the bioreactor either by boost addition or by continuous pumping. The mAb concentration was measured by protein A HPLC.

A very high cell density of 100 x 10⁶ cells/mL was stably maintained in growing phase and at high viability by performing cell bleeds in a perfused WAVE Bioreactor™ using TFF or ATF cell separations. With the settings used here, the maximal cell density was limited to 214 x 10⁶ cells/mL using TTF and 132 x 10⁶ cells/mL using ATF. Using TFF, the cell density could not be further increased due to the limitations of membrane capacity (for the encountered high viscosity), oxygenation and CO₂ level, and using ATF due to pressure limitation to push highly viscous fluid and use of non-pressurisable disposable bioreactor. Thus, the TFF system allowed reaching higher cell densities. To our knowledge, it is the first time that a CHO cell density of more than 200 x 10⁶ cells/mL was achieved in a wave-agitated bioreactor.

Higher retentions of mAb were observed using the TFF system than using the ATF system. In perfusion, the major effect of this retention was loss of mAb in the cell bleeds. Consequently, ATF system was more favourable for production at stable cell density maintained by cell bleeds.

The use of a disposable bioreactor equipped with a disposable separation device offers a solution alleviating technical and sterility challenges occurring in perfusion processes.