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Quantitative monitoring of yeast fermentation using Raman spectroscopy
Authors:Jens A. Iversen  Rolf W. Berg  Birgitte K. Ahring
Affiliation:1. Section for Sustainable Biotechnology, Aalborg University, A. C. Meyers V?nge 15, 2450, Copenhagen, SV, Denmark
3. Center for Bioproducts and Bioenergy, Washington State University Tri-Cities, 2710 Crimson Way, Richland, WA, 99354, USA
2. Department of Chemistry, Technical University of Denmark, Bygning 207, 2800, Lyngby, Denmark
Abstract:
Compared to traditional IR methods, Raman spectroscopy has the advantage of only minimal interference from water when measuring aqueous samples, which makes this method potentially useful for in situ monitoring of important industrial bioprocesses. This study demonstrates real-time monitoring of a Saccharomyces cerevisiae fermentation process using a Raman spectroscopy instrument equipped with a robust sapphire ball probe. A method was developed to correct the Raman signal for the attenuation caused by light scattering cell particulate, hence enabling quantification of reaction components and possibly measurement of yeast cell concentrations. Extinction of Raman intensities to more than 50 % during fermentation was normalized with approximated extinction expressions using Raman signal of water around 1,627 cm?1 as internal standard to correct for the effect of scattering. Complicated standard multi-variant chemometric techniques, such as PLS, were avoided in the quantification model, as an attempt to keep the monitoring method as simple as possible and still get satisfactory estimations. Instead, estimations were made with a two-step approach, where initial scattering correction of attenuated signals was followed by linear regression. In situ quantification measurements of the fermentation resulted in root mean square errors of prediction (RMSEP) of 2.357, 1.611, and 0.633 g/L for glucose, ethanol, and yeast concentrations, respectively.
Keywords:
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