From the three growth rates, the lower rate used (0 1 h−1) seems

From the three growth rates, the lower rate used (0.1 h−1) seems to be preferable, taking into account its reproducibility and the ability of cells to consume the glycerol provided by the feed in the early stages of the fermentation. Comparing these results to those obtained with constant feeds, both allowed the achievement of very similar maximum ODs (between 50 and 60, approximately), and because the feeding solutions for the exponential feeds require much larger quantities of glycerol, constant feeds seem preferable, considering the lower costs

associated in a further scale-up strategy. Similarly to the results obtained for constant feeding experiments, cellular viability results in exponential Navitoclax in vivo feeding showed that the number of dead cells increased throughout the fed-batch phase. Since glycerol concentration ICG-001 price did not seem to have a great influence in cell growth and

viability, it seems that other aspect may be affecting cell growth in late stages of the fermentation. One of the possibilities is the accumulation of toxic byproducts during the process, that has been reported in fed-batch processes [14], [22] and [27]. Another possible factor that might be influencing these results is tryptone concentration, which might be hampering E. coli viability as a limiting substrate. Maximum OD reached in these fermentations was a little lower (about 40), which can

be associated with IPTG induction, since this inducer is known to be toxic and promote metabolic stress [13] and [17]. The comparison of cytometry results from the fermentations at constant feeding with the same feeding rate (1 g/L/h) showed overall lower percentages of permeabilized and dead cells. This may be possibly due to the higher concentration of tryptone present in these fermentations, confirming the above mentioned possible effect of low tryptone concentrations in cell viability. Another reason for these seemingly better results might be related with process duration. In these last assays, the whole process (batch and fed-batch) only took 13 h to develop, against the 17 and 22 h of the processes that used Glycogen branching enzyme the same feeding rate. This shorter period was probably due to the early implementation of the fed-batch technique (7 h of batch fermentation, against 9 and 10 for the other assays). With lower fermentation times, possibly toxic by-products are less likely to accumulate, or they do so at lower levels, and so their effect on cell viability is not so evident. From Fig. 5, we can see that specific hSCOMT activity enhances progressively after induction, with the highest value (442.34 nmol/h/mg) being achieved 6 h after induction, since the promoter had more time to act. In this study, several fermentation conditions were tested to increase SCOMT production in E.

Leave a Reply

Your email address will not be published. Required fields are marked *

*

You may use these HTML tags and attributes: <a href="" title=""> <abbr title=""> <acronym title=""> <b> <blockquote cite=""> <cite> <code> <del datetime=""> <em> <i> <q cite=""> <strike> <strong>