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Applied and Environmental Microbiology, September 2001, p. 4346-4348, Vol. 67, No. 9
0099-2240/01/$04.00+0 DOI: 10.1128/AEM.67.9.4346-4348.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
Generation of a Novel Saccharomyces cerevisiae Strain
That Exhibits Strong Maltose Utilization and Hyperosmotic Resistance
Using Nonrecombinant Techniques
Vincent J.
Higgins,1,2,*
Philip
J. L.
Bell,2,3
Ian W.
Dawes,1,2 and
Paul
V.
Attfield2,3
School of Biochemistry and Molecular
Genetics1 and Cooperative Research
Centre for Food Industry Innovation,2 University
of New South Wales, Sydney, New South Wales 2052, and
Department of Biological Sciences, Macquarie University,
Sydney, New South Wales 2109,3 Australia
Received 30 March 2001/Accepted 19 June 2001
 |
ABSTRACT |
A yeast strain capable of leavening both unsugared and sweet bread
dough efficiently would reduce the necessity of carrying out the
expensive procedure of producing multiple baker's yeast strains. But
issues involving the use of genetically modified foods have
rendered the use of recombinant techniques for developing yeast
strains controversial. Therefore, we used strong selection and
screening systems in conjunction with traditional mass mating techniques to develop a strain of Saccharomyces cerevisiae
that efficiently leavens both types of dough.
| |
TEXT |
Two categories of baker's yeast
(Saccharomyces cerevisiae) are used in the modern baking
industry. There are yeast strains optimized for use in dough containing
no added sugar (unsugared dough) and yeasts that are specialized for
use in sweet dough to which sugar has been added at up to 30% (wt/wt)
of flour (2, 6). A yeast strain for use in a broad range
of bread doughs would need to combine efficient maltose metabolism,
which is relevant to fermentative activity in unsugared dough (7,
8, 15), with strong hyperosmotic adaptation, which is relevant
to sweetened dough that is capable of exerting hyperosmotic stress
close to the limit of growth for S. cerevisiae (2,
14). We therefore sought to generate yeast strains with these
combined characteristics.
As a preliminary to strain generation, we developed selective and
high-throughput screening tests for strong maltose utilization and
strong hyperosmotic adaptation traits. Previous work has shown that
strains with strong maltose phenotypes and efficient unsugared dough
leavening also have high maltose permease and maltase protein activities when grown in medium containing galactose (8,
9). To determine whether cycling between growth on galactose and
growth on maltose would enrich for growth of efficient
maltose-utilizing strains, cells of strain L38 (a slow inducer of its
maltose-utilizing activities) and strain NL67 (with high noninduced
levels of maltose permease and 
-glucosidase) were inoculated at a
ratio of approximately 5:1 into yeast extract-peptone-galactose
medium (8) and incubated for 3 h at 30°C. Aliquots
of this culture (10 ml) were transferred to 100 ml of yeast
extract-peptone-maltose medium (8) and incubated for
another 3 h. This process was repeated three times, with the last
incubation taking place overnight in yeast extract-peptone-maltose medium. Cells were subjected to this cycle over the course of 5 days,
with aliquots of culture plated out to single colonies onto yeast
extract-peptone-dextrose agar plates (8) each day. The
maltose utilization phenotype of each colony was determined using an
acidification power test (10) to identify the presence of
either NL67 or L38 cells. The initial mixed population consisted of
<20% cells with rapid maltose utilization. After the first cycle of
enrichment, more than 30% of the cells exhibited NL67-like maltose utilization characteristics. The ratio of efficient
maltose-utilizing cells increased over the five cycles
of enrichment, so that by the fifth cycle virtually all the cells
were of the NL67 type.
Osmotolerant strains produce more gas in the osmotically challenging
high-sugar synthetic dough medium (HSSD) (2). Therefore, these strains would be expected to grow better in a high-sugar environment. To determine whether this was the case, we monitored the
growth rates of the osmotolerant industrial strain L38 and of the
strong maltose-utilizing industrial strains NL25 and NL67 after
inoculation of equal numbers of cells into HSSD. After 72 h of
incubation in HSSD, strain L38 showed strong growth, with an optical
density of >5 compared to 0.2 for NL25. NL67 showed some growth, which
correlates with its known moderate gassing ability in sweet dough
compared to that of NL25 (2). These data indicate that
growth in HSSD is a potentially useful protocol to select for
osmotolerant strains.
The strains selected for use in the mass mating program were commercial
strains used for sweet-dough (L38, L39, L52, L53, L83, L92, and L96)
and unsugared-dough (NL25, NL30, and NL67) leavening. All strains were
shown to efficiently produce CO2 in their respective dough
types (2). Haploid yeasts derived from these strains were
mass mated essentially as outlined by Lindegren and Lindegren
(11). The resultant mass mating mixture using the
osmotolerant strains was subjected to high osmotic growth pressure in
HSSD, where fast-growing types were enriched and selected. To further
increase the genetic variability and osmotic strength of the
population, the enriched population was sporulated and mass mated a
second time, and the resulting hybrids were treated again to the same
hyperosmotic selection. A mass mating mixture using strains NL25, NL30,
and NL67 was also produced and subjected to cycling between growth in
galactose and growth in maltose medium. Sporulation and enrichment were
repeated, with the production of a population of hybrids enriched for
strong maltose-utilizing strains resulting. Finally, sporulated
haploids were produced from hybrids enriched for osmotolerance or
strong maltose utilization. The pools of osmotolerant and
strong-maltose-utilizing haploids were mixed and mass mated. Resultant
hybrids were then enriched for strong maltose utilization. This
enriched population was then enriched for osmotolerant hybrids by
growth in HSSD. This protocol was repeated twice, and hybrid strains
were plated onto yeast extract-peptone-dextrose agar plates for further testing.
The enriched mass-mated population was screened, using the
acidification power test (10), for isolates with strong
maltose-utilizing characteristics. Hybrids that acidified medium
containing maltose more quickly than strain L38 were then subjected to
an osmotolerance screening test, which identified hybrids that produced
more gas bubbles in HSSD during 1 h at 30°C than the NL67
control. Of 2,000 isolates randomly selected from the population, 196 were determined to be regarded close to the positive controls in both
osmotolerance and strong maltose utilization.
To further investigate the phenotype of the 196 isolates, their gassing
abilities in HSSD and low-sugar synthetic dough were tested using a
multifermentation screening system (5). This test has been
shown to correlate accurately with gas production in real bread dough
(2). One isolate produced as much CO2 in low-sugar synthetic dough and HSSD as did the control strains NL67 and
L38, respectively, and was designated strain NL98. The NL98 phenotype
was determined to be stable over 10 generations, and its hybrid status
was confirmed by PCR fingerprinting using yeast multiplex PCR
primers (Bresatech, Sydney, Australia) (3).
The ability of NL98 to leaven unsugared bread dough and
18%-sugar bread dough (12, 13) was compared to that
of strains used in industrial practice. This comparison showed
that industrial strains could be divided into two major groups, one
that had high unsugared-dough activity but low 18%-sugar
dough activity and the other with the opposite activities. Strain
NL98 stood out from these groups, having the highest unsugared-dough
activity as well as good sweet dough activity (Fig.
1).
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FIG. 1.
Comparison of NL98 gassing activities in unsugared and
sweet (18%-sucrose-added) bread doughs with those of
commercially used baker's yeast strains.
|
|
The nonlagging phenotype in unsugared dough has been shown to be a
result of noninduced maltose permease and maltase activities (8,
15). Like the other nonlagging strains, NL98 had high noninduced
levels of maltose permease and maltase activities (Table 1). Mutations in the maltose regulatory
protein which lead to high noninduced maltose permease and maltase
activities are numerous and are located throughout the protein
(4, 9). Hence, programs that relied on mutagenesis of
osmotolerant strains to produce a broad-sugar-range yeast strain would
have been limited in success, due to the difficulties in producing the
number of mutations needed within a defined region to give high
noninduced maltose permease and maltase activities.
View this table:
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|
TABLE 1.
Maltase and maltose permease activities of baker's yeast
strains grown to mid-log phase in maltose, galactose, ethanol, and
glucose
|
|
In an attempt to understand the reasons for the good performance of
NL98 in sweet dough, its invertase levels were measured and found to be
about fourfold higher than those of other osmotolerant strains (Table
2). This result was surprising, since
previously available evidence indicated that the ability of S. cerevisiae to ferment sweet dough is inversely related to the
activity of invertase (6, 16). The amount of glycerol
produced and retained intracellularly has also been reported to
correlate with the abilities of a yeast strain to ferment sweet dough
(1, 12, 14). Measurement of the glycerol parameters showed
that strain NL98 synthesized and retained the polyol at higher levels
in HSSD than either the osmosensitive strains or the osmotolerant
strains (Table 2).
Attempts to develop a true broad-sugar-range yeast strain using
recombinant DNA technology have had limited success (8, 17), and these strains have not been used commercially due to the sensitive nature of the use of genetically modified organisms in
the food industry. Bell et al. (2) suggested that an
important factor in the lack of combined high-sugar- and
low-sugar-dough phenotypes in a single yeast strain might be related to
the duplication of the telomere-associated MAL and invertase
(SUC) loci in yeast strains. The use of a mating strategy
that provides for high genetic variability and strong selection systems
appears to have circumvented this duplication and to have enabled
isolation of a yeast strain that retains high invertase activity yet
displays osmotolerance qualities by means of a very high capacity to
produce and retain glycerol.
| |
FOOTNOTES |
*
Corresponding author. Mailing address: School of
Biochemistry and Molecular Genetics, University of New South Wales,
Sydney, New South Wales 2052, Australia. Phone: 61 2 9385 1832. Fax: 61 2 9385 1050. E-mail: v.higgins{at}unsw.edu.au.
| |
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Applied and Environmental Microbiology, September 2001, p. 4346-4348, Vol. 67, No. 9
0099-2240/01/$04.00+0 DOI: 10.1128/AEM.67.9.4346-4348.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
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