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1.
The potential of cashew apple bagasse as a source of sugars for ethanol production by Kluyveromyces marxianus CE025 was evaluated in this work. This strain was preliminarily cultivated in a synthetic medium containing glucose and xylose
and was able to produce ethanol and xylitol at pH 4.5. Next, cashew apple bagasse hydrolysate (CABH) was prepared by a diluted
sulfuric acid pretreatment and used as fermentation media. This hydrolysate is rich in glucose, xylose, and arabinose and
contains traces of formic acid and acetic acid. In batch fermentations of CABH at pH 4.5, the strain produced only ethanol.
The effects of temperature on the kinetic parameters of ethanol fermentation by K. marxianus CE025 using CABH were also evaluated. Maximum specific growth rate (μmax), overall yields of ethanol based on glucose consumption
YP \mathord | / |
\vphantom P S1 S1 \textGY_{{P \mathord{\left/ {\vphantom {P {S_1 }}} \right. \kern-\nulldelimiterspace} {S_1 }}}^{\text{G}} and based on glucose + xylose consumption (Y
P/S
), overall yield of ethanol based on biomass (Y
P/X
), and ethanol productivity (P
E) were determined as a function of temperature. Best results of ethanol production were achieved at 30°C, which is also quite
close to the optimum temperature for the formation of biomass. The process yielded 12.36 ± 0.06 g l−1 of ethanol with a volumetric production rate of 0.257 ± 0.002 g l−1 h−1 and an ethanol yield of 0.417 ± 0.003 g g−1 glucose. 相似文献
2.
Candida shehatae NCL-3501 utilized glucose and xylose efficiently in batch cultures. The specific rate of ethanol production was higher with mixtures of glucose and xylose (0.64–0.83 g g –1 cells d –1) compared to that with individual sugars (0.38–0.58 g g –1 cells d –1). Although the optimum temperature for growth was 30°C, this strain grew and produced appreciable levels of ethanol at 45°C. A stable ethanol yield (0.40–0.43 g g –1 substrate utilized) was obtained between 10 g L –1 and 80 g L –1 of initial xylose concentration. Conversion efficiency was further improved by immobilization of the cells in calcium alginate beads. Free or immobilized cells of C. shehatae NCL-3501 efficiently utilized sugars present in rice straw hemicellulose hydrolysate, prepared by two different methods, within 48 h. Ethanol yields of 0.45 g g –1 and 0.5 g g –1 from autohydrolysate, and 0.37 g g –1 from acid hydrolysate were produced by free and immobilized cells, respectively. 相似文献
3.
Summary Ethanol was produced from xylose by converting the sugar to xylulose, using commercial xylose isomerases, and simultaneously converting the xylulose to ethanol by anaerobic fermentation using different yeast strains. The process was optimized with the yeast strain Schizosaccharomyces pombe (Y-164). The data show that the simultaneous fermentation and isomerization of 6% xylose can produce final ethanol concentrations of 2.1% w/v within 2 days at temperatures as high as 39°C.Nomenclature SFIX
simultaneous fermentation and isomerization of xylose
-
V
p
volumetric production (g ethanol·l -1 per hour)
-
Q
p
specific rate (g ethanol·g -1 cells per hour)
-
Y
s
yield from substrate consumed (g ethanol, g -1 xylose)
- ET
ethanol concentration (% wt/vol)
- XT
xylitol concentration (% wt/vol)
- Glu
glucose
- Xyl
xylose
- --m
maximum
- --f
final 相似文献
4.
Previously, a Saccharomyces cerevisiae strain was engineered for xylose assimilation by the constitutive overexpression of the Orpinomyces xylose isomerase, the S. cerevisiae xylulokinase, and the Pichia stipitis SUT1 sugar transporter genes. The recombinant strain exhibited growth on xylose, under aerobic conditions, with a specific growth
rate of 0.025 h −1, while ethanol production from xylose was achieved anaerobically. In the present study, the developed recombinant yeast was
adapted for enhanced growth on xylose by serial transfer in xylose-containing minimal medium under aerobic conditions. After
repeated batch cultivations, a strain was isolated which grew with a specific growth rate of 0.133 h −1. The adapted strain could ferment 20 g l −1 of xylose to ethanol with a yield of 0.37 g g −1 and production rate of 0.026 g l −1 h −1. Raising the fermentation temperature from 30°C to 35°C resulted in a substantial increase in the ethanol yield (0.43 g g −1) and production rate (0.07 g l −1 h −1) as well as a significant reduction in the xylitol yield. By the addition of a sugar complexing agent, such as sodium tetraborate,
significant improvement in ethanol production and reduction in xylitol accumulation was achieved. Furthermore, ethanol production
from xylose and a mixture of glucose and xylose was also demonstrated in complex medium containing yeast extract, peptone,
and borate with a considerably high yield of 0.48 g g −1. 相似文献
5.
Summary The yeast-like organism Aureobasidium pullulans efficiently converted abetd-xylose to cell mass ( Y
X/S=0.45 g·g –1) with negligible production of polyols ( Y
P/S=0.003 g·g –1) under aerobic conditions. A. pullulans grown semiaerobically exhibited different fermentation capacities in seven basal (vitaminless) medium and medium containing a mixture of seven vitamins. It was found that under semiaerobic conditions a mixture of vitamins significantly enhanced production of ethanol from abetd-xylose, resulting in a 15-fold higher yield coefficient of ethanol ( Y
E/S=0.22 g·g –1) as compared to that achieved in vitaminless medium. This increase in ethanol production was accomplished at the expense of cell mass. A. pullulans produced extremely low amounts of polyols throughout all aerobic and semiaerobic experiments. A. pullulans displayed strictly NADPH-linked xylose reductase and NAD +-linked xylitol dehydrogenase activities. 相似文献
6.
Summary The ability of Candida guillermondii to produce xylitol from xylose and to ferment individual non xylose hemicellulosic derived sugars was investigated in microaerobic conditions. Xylose was converted into xylitol with a yield of 0,63 g/g and ethanol was produced in negligible amounts. The strain did not convert glucose, mannose and galactose into their corresponding polyols but only into ethanol and cell mass. By contrast, fermentation of arabinose lead to the formation of arabitol. On D-xylose medium, Candida guillermondii exhibited high yield and rate of xylitol production when the initial sugar concentration exceeded 110 g/l. A final xylitol concentration of 221 g/l was obtained from 300 g/l D-xylose with a yield of 82,6% of theoretical and an average specific rate of 0,19 g/g.h.Nomenclature Q p
average volumetric productivity of xylitol (g xylitol/l per hour)
- q p
average specific productivity of xylitol (g xylitol/g of cells per hour)
- So
initial xylose concentration (g/l)
- tf
incubation time (hours)
- Y P/S
xylitol yield (g of xylitol produced/g of xylose utilized)
- Y E/S
ethanol yield (g of ethanol produced/g of substrate utilized)
- Y X/S
cells yield (g of cells/g of substrate utilized)
-
specific growth rate coefficient (h –1)
- max
maximum specific growth rate coefficient (h –1) 相似文献
7.
We have studied the ethanolic fermentation of D-xylose with Pachysolen tannophilus in batch cultures. We propose a model to predict variations in D-xylose consumed, and biomass and ethanol produced, in which we include parameters for the specific growth rate, for the consumption of D-xylose and production of ethanol either related or not to growth.The ideal initial pH for ethanol production turned out to be 4.5. At this pH value the net specific growth rate was 0.26 h –1, biomass yield was 0.16 g.g –1, the cell-maintenance coefficient was 0.073 g.g –1.h –1, the parameter for ethanol production non-related to growth was 0.064 g.g –1,h –1 and the maximum ethanol yield was 0.32 g.g –1.List of Symbols
A
c
Carbon atomic weight
-
a
d1/h
Specific cell-maintenance rate defined in Eq. (8)
-
c
Mass fraction of carbon in the biomass
-
E g/l
Ethanol concentration
-
f
x
Correction factor defined in Eq. (13)
-
f
x
Correction factor defined in Eq. (13)
-
f
xi
Correction factor defined in Eq. (14)
-
k
d1/h
Death constant
-
M
E
Ethanol molecular weight
-
M
s
Xylose molecular weight
-
M
xi
Xylitol molecular weight
-
m g xylose/g biomass
Maintenance coefficient for substrate
-
m
dg xylose/g biomass
Maintenance coefficient when k
d
-
q
Eg ethanol/g biomass.
Specific ethanol production rate
-
s g/l
Residual xylose concentration
-
s
0 g/l
Initial xylose concentration
-
t h
Time
-
x g/l
Biomass concentration
-
x
0 g/l
Initial biomass concentration
-
Y
E/sg ethanol/g xylose
Instantaneous ethanol yield
-
¯Y
E/sg ethanol/g xylose
Mean ethanol yield
-
Y
E
s/T
g ethanol/g xylose
Theoretical ethanol yield
-
Y
E
s/*
g ethanol/g xylose
Corrected instantaneous ethanol yield
-
¯Y
E
s/*
g ethanol/g xylose
Corrected mean ethanol yield
-
Y
x/sg biomass/g xylose
Biomass yield
-
¯Y
xi/sg xylitol/g xylose
Mean xylitol yield
Greek Letters
g ethanol/g biomass
Growth-associated product formation parameter
-
g ethanol/g biomass.h
Non-growth-associated product formation parameter
-
dg ethanol/g biomass.h
Non-growth-associated product formation parameter when k
d0
-
h
Variable defined in Eq. (6) or Eq. (7)
-
1/h
Specific growth rate
-
m1/h
Maximum specific growth rate 相似文献
8.
Summary As components of combined fermentation of both glucose and xylose to ethanol by separated or coculture processes, the effects of initial sugar concentrations on the fermentative performances of Pichia stipitis Y7124, Candida shehatae ATCC 22984, Saccharomyces cerevisiae CBS1200 and Zymomonas mobilis ATCC10988 were investigated. From the characteristics of sugar and produced ethanol tolerances the most suitable microorganisms for the achievement of glucose and xylose fermentations have been selected with respect to different fermentation schemes.Nomenclature Tf
fermentation time (hours)
- Ef
ethanol concentration (g/l)
- Y P/S
ethanol yield (g of ethanol produced/g of sugar used)
- qp
average specific productivity of ethanol (g ethanol/g of cells per hour)
- max
maximum specific growth rate (h –1) 相似文献
9.
Glucose repressed xylose utilization in Candida tropicalis pre-grown on xylose until glucose reached approximately 0–5 g l –1. In fermentations consisting of xylose (93 g l –1) and glucose (47 g l –1), xylitol was produced with a yield of 0.65 g g –1 and a specific rate of 0.09 g g –1 h –1, and high concentrations of ethanol were also produced (25 g l –1). If the initial glucose was decreased to 8 g l –1, the xylitol yield (0.79 g g –1) and specific rate (0.24 g g –1 h –1) increased with little ethanol formation (<5 g l –1). To minimize glucose repression, batch fermentations were performed using an aerobic, glucose growth phase followed by xylitol production. Xylitol was produced under O 2 limited and anaerobic conditions, but the specific production rate was higher under O 2 limited conditions (0.1–0.4 vs. 0.03 g g –1 h –1). On-line analysis of the respiratory quotient defined the time of xylose reductase induction. 相似文献
10.
A family of 10 competing, unstructured models has been developed to model cell growth, substrate consumption, and product formation of the pyruvate producing strain Escherichia coli YYC202 ldhA::Kan strain used in fed-batch processes. The strain is completely blocked in its ability to convert pyruvate into acetyl-CoA or acetate (using glucose as the carbon source) resulting in an acetate auxotrophy during growth in glucose minimal medium. Parameter estimation was carried out using data from fed-batch fermentation performed at constant glucose feed rates of
qVG=10 mL h –1. Acetate was fed according to the previously developed feeding strategy. While the model identification was realized by least-square fit, the model discrimination was based on the model selection criterion (MSC). The validation of model parameters was performed applying data from two different fed-batch experiments with glucose feed rate
qVG=20 and 30 mL h –1, respectively. Consequently, the most suitable model was identified that reflected the pyruvate and biomass curves adequately by considering a pyruvate inhibited growth (Jerusalimsky approach) and pyruvate inhibited product formation (described by modified Luedeking–Piret/Levenspiel term).List of symbols c A
acetate concentration (g L –1)
- c A,0
acetate concentration in the feed (g L –1)
- c G
glucose concentration (g L –1)
- c G,0
glucose concentration in the feed (g L –1)
- c P
pyruvate concentration (g L –1)
- c P,max
critical pyruvate concentration above which reaction cannot proceed (g L –1)
- c X
biomass concentration (g L –1)
- K I
inhibition constant for pyruvate production (g L –1)
- K IA
inhibition constant for biomass growth on acetate (g L –1)
- K P
saturation constant for pyruvate production (g L –1)
- K P
inhibition constant of Jerusalimsky (g L –1)
- K SA
Monod growth constant for acetate (g L –1)
- K SG
Monod growth constant for glucose (g L –1)
- m A
maintenance coefficient for growth on acetate (g g –1 h –1)
- m G
maintenance coefficient for growth on glucose (g g –1 h –1)
- n
constant of extended Monod kinetics (Levenspiel) (–)
- q V
volumetric flow rate (L h –1)
- q VA
volumetric flow rate of acetate (L h –1)
- q VG
volumetric flow rate of glucose (L h –1)
- r A
specific rate of acetate consumption (g g –1 h –1)
- r G
specific rate of glucose consumption (g g –1 h –1)
- r P
specific rate of pyruvate production (g g –1 h –1)
- r P,max
maximum specific rate of pyruvate production (g g –1 h –1)
- t
time (h)
- V
reaction (broth) volume (L)
- Y P/G
yield coefficient pyruvate from glucose (g g –1)
- Y X/A
yield coefficient biomass from acetate (g g –1)
- Y X/A,max
maximum yield coefficient biomass from acetate (g g –1)
- Y X/G
yield coefficient biomass from glucose (g g –1)
- Y X/G,max
maximum yield coefficient biomass from glucose (g g –1)
-
growth associated product formation coefficient (g g –1)
-
non-growth associated product formation coefficient (g g –1 h –1)
-
specific growth rate (h –1)
- max
maximum specific growth rate (h –1) 相似文献
11.
Summary Optimal growth conditions for Zymomonas mobilis have been established using continuous cultivation methods. Optimal substrate utilization efficiency occurs with 2.5 g l –1 yeast extract, 2.0 g l –1 ammonium sulfate and 6.0 g l –1 magnesium sulfate in the media. Catabolic activity is at its maximum with glucose uptake rates of 16–18 g l –1 h –1 and ethanol production rates of 8–9 g l –1 h –1, Q g values of 22–26 and Q p values between 11 and 13, which results in 40 g l –1 h –1 ethanol yields using a 100 g l –1 substrate feed. Any increase in these parameters goes on cost of substrate utilization efficiency. Calcium pantothenate can not substitute yeast extract.Abbreviations G
Glucose (%)
- Pant
Calcium pantothenate (mg l –1)
- D
Dilution rate (h –1)
- NH 4
Ammonium sulfate (%)
- M g
Magnesium sulfate (%)
- S 1
Residual glucose in the fermenter (g l –1)
- S 0
Glucose feed (g l –1)
- Eth
Ethanol concentration (g l –1)
- GUR
Glucose uptake rate (g l –1 h –1)
- Q g
Specific glucose uptake rate (g g –1 h –1)
- Q p
Specific ethanol production rate (g g –1 h –1)
- EPR
Ethanol production rate (g l –1 h –1)
- Y g
Yield coefficient for glucose (g g –1)
- Y p
Conversion efficiency (%)
- C
Biomass concentration (g l –1)
Present address: (Until June 1982) Institut für Mikrobiologie, TH Darmstadt, 6100 Darmstdt, Federal Republic of Germany 相似文献
12.
Black cumin (Nigella sativa L.) is considered as a noteworthy herbal medicine. However, no study has been conducted on the physiological adaptive mechanism of it to salinity stress, especially under in vitro condition. To this aim, the callus cultures of ten different genotypes of N. sativa were applied to evaluate the changes occurring in biochemical traits under salinity stress. The calluses were exposed to the in vitro salt stress using different sodium chloride concentrations (0, 84, and 250 mM). A reduction occurred in the content of K+ and callus growth by enhancing the NaCl concentration. However, most of the content of Na+ (4 mgg− 1 DW), malondialdehyde (1.38 μmolg− 1 FW), total phenolic content (1.18 mg GAEg−1 FW), thymol (25.26 mgg− 1 DW), total flavonoids content (0.06 mg QEg− 1 FW), total flavonols (TFL) content (0.023 mg QEg− 1 FW), total anthocyanins (Ant) (0.05 μmol g− 1 FW) and DPPH activity (58.17%) was observed at 250 mM of NaCl. In fact, two secondary metabolites including TFL and Ant can be considered as the major contributors to the potential antioxidant activity of N. sativa at the callus level. The elicitation through NaCl opens new avenues for the selection of best dosages of NaCl for the enhancement of commercially important secondary metabolites, in superior genotypes (Nig1 and Nig2) of N. sativa at cellular level. 相似文献
13.
The influence of ethanol on the degradation kinetics of linear alkyl benzene sulfonate (LAS) and organic matter was investigated using batch experiments with different initial LAS concentrations (8.3 mg L−1 to 66.9 mg L−1) and biomass immobilized on sand. Data were fitted with a substrate inhibition model. Concentrations of 2.4 mg LAS L−1 and 18.9 mg LAS L−1 (without and with ethanol) provided the maximum LAS utilization rate by the biomass (Sbm). For LAS degradation, ethanol addition favored a lower decrease in the specific substrate utilization rate (robs), even at the LAS concentration usually reported as inhibitory (> 14.4 mg L−1). For organic matter degradation, robs was higher with ethanol. Higher biomass differentiation was observed at higher LAS concentrations. With ethanol, microbial selection occurred at LAS concentrations near Sbm. At higher LAS concentrations, the dominance and diversity values did not change significantly with ethanol, whereas without ethanol, their behaviors were irregular. 相似文献
14.
Substrates that contain hexose as well as pentose sugars can form an interesting substrate for the production of ethanol. Pichia stipitis and a respiratory-deficient mutant of Saccharomyces diastaticus were used to convert such a substrate into ethanol under continuous culture conditions. With a sugar mixture (glucose 70%/xylose 30%) at 50 g/l, the xylose was entirely consumed when the dilution rate (D) did not exceed 0.006 h –1 whereas the glucose was entirely consumed whatever the D. The study of influence of initial substrate concentration (S 0) was performed at D = 0.015 h –1. Under these conditions the substrate was entirely consumed when its initial concentration did not exceed 20 g/l. With S 0 = 80 g/l the residual xylose concentration reached 20.5 g/l. At low D or at low S 0, P. stipitis was the dominant species in the fermentor. Increasing the D or S 0 resulted in the wash-out of P. stipitis mainly because of its low ethanol tolerance.
Correspondence to: J. P. Delgenes 相似文献
15.
Saccharomyces’ physiology and fermentation-related properties vary broadly among industrial strains used to ferment glucose. How genetic
background affects xylose metabolism in recombinant Saccharomyces strains has not been adequately explored. In this study, six industrial strains of varied genetic background were engineered
to ferment xylose by stable integration of the xylose reductase, xylitol dehydrogenase, and xylulokinase genes. Aerobic growth
rates on xylose were 0.04–0.17 h −1. Fermentation of xylose and glucose/xylose mixtures also showed a wide range of performance between strains. During xylose
fermentation, xylose consumption rates were 0.17–0.31 g/l/h, with ethanol yields 0.18–0.27 g/g. Yields of ethanol and the
metabolite xylitol were positively correlated, indicating that all of the strains had downstream limitations to xylose metabolism.
The better-performing engineered and parental strains were compared for conversion of alkaline pretreated switchgrass to ethanol.
The engineered strains produced 13–17% more ethanol than the parental control strains because of their ability to ferment
xylose. 相似文献
16.
During second‐generation bioethanol production from lignocellulosic biomass, the desired traits for fermenting microorganisms, such as Saccharomyces cerevisiae, are high xylose utilization and high robustness to inhibitors in lignocellulosic hydrolysates. However, as observed previously, these two traits easily showed the antagonism, one rising and the other falling, in the C6/C5 co‐fermenting S. cerevisiae strain. In this study, LF1 obtained in our previous study is an engineered budding yeast strain with a superior co‐fermentation capacity of glucose and xylose, and was then mutated by atmospheric and room temperature plasma (ARTP) mutagenesis to improve its robustness. The ARTP‐treated cells were grown in 50% (v/v) leachate from lignocellulose pretreatment with high inhibitors content for adaptive evolution. After 30 days, the generated mutant LF1‐6 showed significantly enhanced tolerance, with a six‐fold increase in cell density in the above leachate. Unfortunately, its xylose utilization dropped markedly, indicating the recurrence of the negative correlation between xylose utilization and robustness. To alleviate this antagonism, LF1‐6 cells were iteratively mutated with ARTP mutagenesis and then anaerobically grown using xylose as the sole carbon source, and xylose utilization was restored in the resulting strain 6M‐15. 6M‐15 also exhibited increased co‐fermentation performance of xylose and glucose with the highest ethanol productivity reported to date (0.525 g g ?1 h ?1) in high‐level mixed sugars (80 g L ?1 glucose and 40 g L ?1 xylose) with no inhibitors. Meanwhile, its fermentation time was shortened by 8 h compared to that of LF1. During the fermentation of non‐detoxified lignocellulosic hydrolysate with high inhibitor concentrations at pH ~3.5, 6M‐15 can efficiently convert glucose and xylose with an ethanol yield of 0.43 g g ?1. 6M‐15 is also regarded as a potential chassis cell for further design of a customized strain suitable for production of second‐generation bioethanol or other high value‐added products from lignocellulosic biomass. 相似文献
17.
Summary These studies examined several process variables important in scaling up the fermentation of xylose by Candida shehatae. Inoculum age and cell density were particularly influential. Young (24-h) inocula fermented xylose to ethanol two to three times as fast as older (48- or 72-h) inocula. With all three inocula ages, the initial fermentation rates were essentially linear with cell density, up to 4 g dry wt cells L -1. Above that cell density, the ethanol production rate appeared to be oxygen limited, particularly with 24-h old cells. Aeration also played a role in xylose utilization. The fermentation proceeded under both aerobic and anaerobic conditions, but xylose was not completely utilized anaerobically. With aeration, 25% more ethanol was formed in about one third the time than without aeration. Ethanol yields were similar under the two conditions. Cell growth on xylose was observed in the absence of oxygen. Cells went through essentially one doubling in 24 h. Based on the sugar consumed, a Y
ATP of 9.9 was obtained. Slow continuous feeding of glucose significantly increased the xylose utilization rate.Maintained in cooperation with the University of Wisconsin, Madison, Wisconsin, USA 相似文献
18.
Lignocellulosic biomass is considered nowadays to be an economically attractive carbohydrate feedstock for large-scale fermentation of bulk chemicals such as lactic acid. The filamentous fungus Rhizopus oryzae is able to grow in mineral medium with glucose as sole carbon source and to produce optically pure l(+)-lactic acid. Less is known about the conversion by R. oryzae of pentose sugars such as xylose, which is abundantly present in lignocellulosic hydrolysates. This paper describes the conversion of xylose in synthetic media into lactic acid by ten R. oryzae strains resulting in yields between 0.41 and 0.71 g g −1. By-products were fungal biomass, xylitol, glycerol, ethanol and carbon dioxide. The growth of R. oryzae CBS 112.07 in media with initial xylose concentrations above 40 g l −1 showed inhibition of substrate consumption and lactic acid production rates. In case of mixed substrates, diauxic growth was observed where consumption of glucose and xylose occurred subsequently. Sugar consumption rate and lactic acid production rate were significantly higher during glucose consumption phase compared to xylose consumption phase. Available xylose (10.3 g l −1) and glucose (19.2 g l −1) present in a mild-temperature alkaline treated wheat straw hydrolysate was converted subsequently by R. oryzae with rates of 2.2 g glucose l −1 h −1 and 0.5 g xylose l −1 h −1. This resulted mainly into the product lactic acid (6.8 g l −1) and ethanol (5.7 g l −1). 相似文献
19.
Summary During xylose fermentation by Candida
shehatae ATCC 22984 with batch cell recycling, the volumetric ethanol fermentation rate increased two-fold, and the xylitol production rate increased three-fold as the cell density increased to ten-fold. In continuous fermentation with membrane-assisted cell recycle, the fermentation rates increased almost linearly with increasing agitation rates up to 300 rpm. The maximum continuous ethanol production rates obtained with 90 and 200 g L –1 xylose were respectively 2.4 and 4.4 g L –1h –1. The cell density was 65–70 g (dry wt) L –1. Ethanol yields ranged from 0.26 to 0.41 g g –1. 相似文献
20.
The importance of non-Saccharomyces yeast species in fermentation processes is widely acknowledged. Within this group, Pichia kudriavzevii ITV-S42 yeast strain shows particularly desirable characteristics for ethanol production. Despite this fact, a thorough study of the metabolic and kinetic characteristics of this strain is currently unavailable. The aim of this work is to study the nutritional requirements of Pichia kudriavzevii ITV-S42 strain and the effect of different carbon sources on the growth and ethanol production. Results showed that glucose and fructose were both assimilated and fermented, achieving biomass and ethanol yields of 0.37 and 0.32 gg−1, respectively. Glycerol was assimilated but not fermented; achieving a biomass yield of 0.88 gg−1. Xylose and sucrose were not metabolized by the yeast strain. Finally, the use of a culture medium enriched with salts and yeast extract favored glucose consumption both for growth and ethanol production, improving ethanol tolerance reported for this genre (35 g L−1) to 90 g L−1 maximum ethanol concentration (over 100%). Furthermore Pichia kudriavzevii ITV-S42 maintained its fermentative capacity up to 200 g L−1 initial glucose, demonstrating that this yeast is osmotolerant. 相似文献
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