212. Compositional and ultrastructural characterization of the SMA strain of Saccharomyces pastorianus
Greg Potter (1), Suzanne M. Budge (1), Alex Speers (2), Chantel Swart (3),
Hendrik Swart (3), Pieter Van Wyk (3); (1) Dalhousie University,
Halifax, NS, Canada; (2) The International Center for Brewing and
Distilling, Edinburgh, U.K.; (3) University of the Free State,
Bloemfontein, South Africa
Yeast, Fermentation, and Microbiology
Poster
Carbon dioxide (CO2) is a well-established and industrially important by-product of fermentative growth in Saccharomyces cerevisiae and Saccharomyces pastorianus, yet the specific mechanism and site of CO2 generation within the cell has not been elucidated. In this study we have analyzed the SMA strain of Saccharomyces pastorianus
using another application of nano-scanning Auger microscopy (NanoSAM),
where specific cells can be targeted by argon-etching to expose the
interior and then subsequently viewed with a high-resolution scanning
electron microscope (SEM). These high-resolution images of the interior
of argon-etched fermenting SMA yeast cells uncovered a maze of
coalescing CO2 bubbles that increased in complexity and
number with fermentation duration. Similar cell preparations were also
visualized using transmission electron microscopy (TEM), and smaller
networks of CO2 bubbles were identified that provide
information on the formation and origin of intracellular bubbles. An
unusual group of oxygenated fatty acids, 3-hydroxy (OH) oxylipins, are
presumed to play a potential role in flocculation during fermentation,
so the effect of gas bubble formation and, thus, fermentation on 3-OH
oxylipin production was also of interest. To investigate this,
fermentatively and non-fermentatively grown SMA cells were examined
using time-of-flight secondary ion mass spectrometry (TOF-SIMS) and the
negative atomic ions C–, NH–, O–, OH–, P–, and S– and negative molecular ions 160– (3-hydroxy 8:0) and 188–
(3-hydroxy 10:0) were monitored. Distinctly different cellular
compositions were found in the fermenting and non-fermenting cells. In
particular, both 3-OH 8:0 and 3-OH 10:0 were constitutively produced in
respiring cells, while there was a delayed onset of 3-OH 8:0 production
in fermenting cells. Thus, the novel application of these
nanotechnological techniques has revealed a correlation between
metabolic state (fermentation vs. respiration), bubble production and
3-OH oxylipin profile. Further investigations using the biological
applications of these material science techniques in conjunction with
more conventional lipid analyses will uncover the role of 3-OH oxylipins
in flocculation and the origin of these hydroxylated fatty acids in
fermentation yeasts.
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