Published: 28 Juni 2026(Updated: 29 Juni 2026)
11 min
11 min read
Kulwant Kandra0

Cell culture in the bioreactor: A practical guide to process development from shake flask to scale-up

Cell cultureLife science research

Moving a mammalian cell culture process from shake flask to bioreactor is more than a scale-up exercise. Each transition introduces new challenges in oxygen transfer, pH control, CO₂ management, mixing, and data reproducibility. This practical guide explores the key stages of cell culture process development, explains why process transfer often fails, and shows how integrated bioreactor control and data management help create scalable, reproducible processes from screening through scale-up.

The hidden challenges of cell culture process development

If your shake-flask-to-bioreactor transfer failed the first time, you are not alone. Even when the biology behaves as expected, experienced cell culture labs encounter the same recurring challenges: unexplained drops in viability, inconsistent pH control, CO₂ accumulation that quietly erodes product quality, and process data that does not reproduce at the next vessel or the next site. 

The cells may behave as expected, but what you learn in a shake flask does not necessarily predict how those same cells will behave in a stirred bioreactor. Likewise, what works at bench scale does not always transfer cleanly to pilot scale. Each transition introduces a new set of variables. This guide explains why that happens and what changes when the bioreactor, control software, and process record are treated as a single system.

The cell culture pathway in one view

Most mammalian cell culture process development moves through four stages. Each stage uses different hardware, but the data and control logic should move with the process rather than being recreated at every step.

StageWorking volumeTypical purposeINFORS HT systems
Screening and inoculum expansion~50 mL – 5 L (shake flask)
Cell line evaluation, close section, and biomass build-upMultitron
Minitron
Celltron
Entry-level process development0.3 – 4 L
First instrumented runs and single-vessel PDMinifors 2

Beyond entry-level bench-top development, the workflow expands into parallel process development, advanced PD, and scale-up. These stages require purpose-built systems with control and data infrastructure that can move seamlessly with the process.

eve® serves as the bioprocess software platform across INFORS HT's bench-top bioreactors, providing consistent controller logic from screening through entry-level process development.

The shake flask: capable, but not the full picture

Shake flasks remain the right starting point for cell line evaluation, clone selection, and initial media optimization. At this stage, the ability to run many parallel conditions and sample them manually often delivers the best balance between throughput and cost. The Multitron incubator shaker is designed to make this stage as controlled and reproducible as possible, providing precise temperature, CO₂, and humidity management across the full stack, from screening flasks through larger working volumes. Minitron extends this capability to smaller setups for entry-level labs, while Celltron, INFORS HT's shaker system for CO₂ incubators, provides the same controlled environment within a laboratory's existing incubator infrastructure.

Start with a controlled environment for cell culture screening and expansion

Many labs complete substantial portions of their workflow in shake flasks, including early process screening and production activities where parallelism and cost outweigh the limitations of offline sampling. For deeper process development, including feeding strategy development, parameter optimization, and cascade tuning, the bioreactor provides a much more detailed understanding of process behavior. Cell density can be measured quickly with a cell analyzer, but pH, dissolved oxygen, CO₂ accumulation, and metabolite trajectories are not continuously visible in a shake flask. They are sampled periodically, and what happens between measurements remains unknown.

Once a process moves beyond initial screening and into feeding strategy development, parameter optimization, or transfer activities, the lack of continuous process data quickly becomes a bottleneck. The transition to a bioreactor is not simply a scale-up step. It represents a move from limited process visibility to a fully instrumented environment, significantly increasing the amount of information gained from every run.


Three parameters that get worse before they get better

When mammalian cells (CHO, HEK, Vero, and others) enter a stirred bioreactor for the first time, three parameters tend to behave unexpectedly.

Batch, fed-batch, or perfusion: choosing the right process mode

Once the physical environment is under control, the question shifts to feeding strategy. This is where the bioreactor earns its place in a cell culture process development workflow.

ModeWhat it doesTypical applicationTrade-off
BatchSingle nutrient charge; culture runs until exhaustedEarly screening, simple protein expressionLimited cell density and productivity
Fed-batchSubstrate added continuously or at intervalsWorkhorse mode for therapeutic protein productionRequires more complex feeding strategy and control
PerfusionFresh medium continuously added; spent medium removed while cells are retainedHigh-density culture, continuous biomanufacturingCell retention method, longer runs, and more demanding setup

Fed-batch remains the dominant cultivation strategy in mammalian cell culture and is used for most therapeutic protein production. As a result, it accounts for much of today's bench-top process development activity. Perfusion has become an established cultivation strategy and continues to gain momentum. It is widely used for high-cell-density processes, reducing manufacturing footprints, and supporting continuous biomanufacturing approaches.

At bench scale, the practical challenges of perfusion often involve selecting the right cell retention method, configuring pumps, maintaining aseptic operation during extended runs, and integrating continuous feeding strategies. Across all three modes, the same principle applies: process development becomes more valuable when more conditions can be tested in parallel, with more instrumentation and more complete data capture.

This is where bioreactor selection begins to matter

The Minifors 2 is INFORS HT's bench-top bioreactor for entry-level cell culture process development. It combines sensor instrumentation, gas control, and feeding capability in a single-vessel format that helps laboratories move from shake flasks into a controlled and instrumented environment.

With eve® integration, every run is captured as a complete process record, including both process data and controller configuration. For labs ready to perform cell culture DoE studies, media optimization, or feeding strategy comparisons, the next stages require purpose-built parallel systems designed specifically for mammalian cell culture.

Reproducibility is a system property, not a protocol property

This is where many cell culture process development conversations become difficult. Labs document protocols. They define setpoints. They train operators. Yet variability still appears:

  • Between operators
  • Between runs
  • Between laboratories
  • Between sites

In most cases, the root cause is not the setpoint itself. It is everything surrounding the setpoint, including cascade configuration, PID tuning, sensor calibration, and hardware assignment. Two operators can run the same protocol on the same bioreactor and achieve different outcomes if their controller configurations differ, their sensor calibrations are inconsistent, or their gas-control strategies are configured differently. None of those details are fully captured in a paper protocol. All of them affect the data. What needs to be managed, versioned, audited, and transferred is the complete controller configuration together with the process record. That is what makes a process development result reproducible across operators, runs, and sites.

Bringing control logic and data together

eve® is the bioprocess software platform that captures the complete process record, including setpoints, cascades, sensor data, controller configurations, and alarms, alongside biological data across every bioreactor in a lab. The same software platform operates across INFORS HT's bench-top bioreactor portfolio, allowing control strategies to move with the process. Up to 80 bioreactors can be managed on a single platform, while eve® Premium adds 21 CFR Part 11 compliance for regulated environments.

Beyond data capture, the platform helps reduce operator variability. When controller configurations are versioned and applied automatically, one of the most common sources of run-to-run variability, human error during cascade or sensor setup, is significantly reduced. Increased automation reduces the number of manual interventions required, which in turn decreases opportunities for operators to unintentionally deviate from the same protocol.

Reproducibility is not achieved through a single feature. It is the result of cultivation hardware, control logic, and data systems working together as an integrated platform. In cell culture process development, where small configuration differences can have a significant impact on outcomes, that level of integration often determines whether a process scales successfully or requires rework at each transition.


What the full development path looks like in practice

A typical cell culture process development pathway in a biopharma, CDMO, or advanced therapy lab follows three key stages. Each stage builds on the data, control strategy, and process understanding developed in the previous one.

Stage 1: Screening and inoculum expansion

Where every cell culture process starts: the shake flask

Shake flasks in a CO₂-controlled incubator shaker, focused on cell line evaluation, clone selection, and growth kinetics. Multitron supports this stage with hygienic humidity control and precise bi-directional CO₂ control. Minitron extends this capability into smaller setups, and Celltron brings shake flask cultivation into a lab's existing CO₂ incubator infrastructure.

Stage 2: First process characterisation

Into the bioreactor: where process understanding begins

Minifors 2 is the bench-top bioreactor where a cell culture process makes its first move from shake flask into a controlled, instrumented environment. Critical Process Parameters are first identified here, cascade logic is established, and the data discipline that carries the process through later stages begins. eve® integration captures the full process record from this point onwards — not just setpoints, but the complete controller configuration.

Stage 3: Parallel Process Development, Scale-up & Tech Transfer

Beyond entry-level: where the cell culture workflow continues

The cell culture workflow continues into parallel multi-vessel work, larger working volumes, and pilot scale. Each of these stages requires purpose-built systems with cell-culture-specific vessel geometry, control logic tuned for mammalian work, and a data infrastructure that travels seamlessly with the process from one stage to the next.

Where to go next

If you are working through a specific stage of the pathway above, these resources provide a useful next step.

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Ready to move your cell culture process forward?

If you are evaluating the next step in your cell culture workflow, an INFORS HT specialist can help assess your application and identify the most appropriate development pathway.

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