SIMULATED MOVING BED (SMB) - A POWERFUL TOOL FOR CONTINUOUS PURIFICATION OF XYLITOL
Applications | | KNAUERInstrumentation
Continuous purification of biochemicals is a critical challenge in industrial biotechnology. Xylitol, a sugar alcohol with applications in food and pharmaceutical industries, is typically produced by microbial fermentation. Achieving high purity and yield in downstream processing determines overall process efficiency, cost and environmental impact. Simulated moving bed chromatography (SMBC) offers a continuous separation approach that can outperform traditional batch methods in throughput, solvent consumption and resin utilization.
The study aimed to develop and demonstrate an SMBC method for purifying xylitol from a fermentation mash derived from a Candida yeast conversion of xylose. Key goals included achieving near‐complete purity and recovery, optimizing operational parameters for continuous operation and comparing performance to conventional batch chromatography.
A fed‐batch fermentation mash containing xylose, arabinose, glycerol, mannitol and xylitol was clarified and diluted. Initial batch HPLC tests on polymeric Eurokat Ca columns confirmed feasibility in isocratic mode. Separation experiments at 40 °C, 50 °C and 60 °C identified 50 °C as optimal. Retention and porosity data were collected to configure the SMBC system via PurityChrom MCC software. The continuous setup used an open-loop design with a waste outlet to remove unretained components.
Temperature screening showed best resolution between xylitol and mannitol at 50 °C. Overload tests with a 1:2 diluted mash achieved near‐baseline separation. The process was divided into raffinate (non-xylitol) and extract (xylitol) fractions. After six operational cycles, extract samples contained xylitol at 100 % purity with no detectable contamination, and raffinate and waste fractions showed no xylitol carryover. The continuous SMBC process delivered 1.8 g/h of pure xylitol with full recovery, representing a seven-fold higher yield compared to batch chromatography.
SMBC enabled continuous high‐purity xylitol production with reduced solvent and resin usage. The improved throughput and yield lower downstream processing costs and footprint. The robustness of the method allows processing feeds with up to four times higher xylitol concentration without loss of performance. Industries can apply this approach to scale large-volume xylitol purification or adapt it to other sugar alcohol separations.
Further scale-up could involve parallel SMB trains and higher-capacity columns to match industrial fermentation volumes. Integration with inline monitoring and control can enhance automation and process reproducibility. Exploring novel stationary phases or hybrid continuous-chromatography techniques may broaden applicability to complex fermentation broths and other value-added bioproducts.
The developed SMBC method provides a robust, efficient and scalable solution for continuous xylitol purification from fermentation mash. It achieves complete purity and recovery while significantly outperforming batch chromatography in throughput and resource usage. This approach can be readily transferred to industrial settings and extended to other sugar-derived bioproducts.
HPLC, Consumables, LC columns
IndustriesFood & Agriculture
ManufacturerKNAUER
Summary
Simulated Moving Bed Chromatography for Continuous Xylitol Purification
Importance of the Topic
Continuous purification of biochemicals is a critical challenge in industrial biotechnology. Xylitol, a sugar alcohol with applications in food and pharmaceutical industries, is typically produced by microbial fermentation. Achieving high purity and yield in downstream processing determines overall process efficiency, cost and environmental impact. Simulated moving bed chromatography (SMBC) offers a continuous separation approach that can outperform traditional batch methods in throughput, solvent consumption and resin utilization.
Objectives and Study Overview
The study aimed to develop and demonstrate an SMBC method for purifying xylitol from a fermentation mash derived from a Candida yeast conversion of xylose. Key goals included achieving near‐complete purity and recovery, optimizing operational parameters for continuous operation and comparing performance to conventional batch chromatography.
Methodology and Instrumentation
A fed‐batch fermentation mash containing xylose, arabinose, glycerol, mannitol and xylitol was clarified and diluted. Initial batch HPLC tests on polymeric Eurokat Ca columns confirmed feasibility in isocratic mode. Separation experiments at 40 °C, 50 °C and 60 °C identified 50 °C as optimal. Retention and porosity data were collected to configure the SMBC system via PurityChrom MCC software. The continuous setup used an open-loop design with a waste outlet to remove unretained components.
Used Instrumentation
- AZURA Lab SMB system with four Assistants ASM 2.1L and seven 8-position valves
- Four AZURA P 4.1S pumps (10/50 mL/min)
- CORI-Flow M13 flow meters
- SMB oven for temperature control
- Eight Eurokat Ca preparative columns (150 × 20 mm, 25–56 µm)
- Analytical system: Eurokat Ca columns (300 × 8 mm, 10 µm) and dedicated sugar analysis module
Results and Discussion
Temperature screening showed best resolution between xylitol and mannitol at 50 °C. Overload tests with a 1:2 diluted mash achieved near‐baseline separation. The process was divided into raffinate (non-xylitol) and extract (xylitol) fractions. After six operational cycles, extract samples contained xylitol at 100 % purity with no detectable contamination, and raffinate and waste fractions showed no xylitol carryover. The continuous SMBC process delivered 1.8 g/h of pure xylitol with full recovery, representing a seven-fold higher yield compared to batch chromatography.
Benefits and Practical Applications
SMBC enabled continuous high‐purity xylitol production with reduced solvent and resin usage. The improved throughput and yield lower downstream processing costs and footprint. The robustness of the method allows processing feeds with up to four times higher xylitol concentration without loss of performance. Industries can apply this approach to scale large-volume xylitol purification or adapt it to other sugar alcohol separations.
Future Trends and Opportunities
Further scale-up could involve parallel SMB trains and higher-capacity columns to match industrial fermentation volumes. Integration with inline monitoring and control can enhance automation and process reproducibility. Exploring novel stationary phases or hybrid continuous-chromatography techniques may broaden applicability to complex fermentation broths and other value-added bioproducts.
Conclusion
The developed SMBC method provides a robust, efficient and scalable solution for continuous xylitol purification from fermentation mash. It achieves complete purity and recovery while significantly outperforming batch chromatography in throughput and resource usage. This approach can be readily transferred to industrial settings and extended to other sugar-derived bioproducts.
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