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Network-based contextualisation of LC-MS/MS proteomics dataGeiger, Armin Guntram 12 1900 (has links)
Thesis (MSc)--Stellenbosch University, 2014. / ENGLISH ABSTRACT: This thesis explores the use of networks as a means to visualise, interpret and
mine MS-based proteomics data.
A network-based approach was applied to a quantitative, cross-species LCMS/
MS dataset derived from two yeast species, namely Saccharomyces cere-
visiae strain VIN13 and Saccharomyces paradoxus strain RO88.
In order to identify and quantify proteins from the mass spectra, a workflow
consisting of both custom-built and existing programs was assembled. Networks
which place the identifed proteins in several biological contexts were
then constructed. The contexts included sequence similarity to other proteins,
ontological descriptions, proteins-protein interactions, metabolic pathways and
cellular location.
The contextual, network-based representations of the proteins proved effective
for identifying trends and patterns in the data that may otherwise have
been obscured. Moreover, by bringing the experimentally derived data together
with multiple, extant biological resources, the networks represented the
data in a manner that better represents the interconnected biological system
from which the samples were derived. Both existing and new hypotheses based
on proteins relating to the yeast cell wall and proteins of putative oenological
potential were investigated. These proteins were investigated in light of
their differential expression between the two yeast species. Examples of proteins
that were investigated included cell wall proteins such as GGP1 and SCW4. Proteins with putative oenological potential included haze protection
factor proteins such as HPF2. Furthermore, differences in capacity for maloethanolic
fermentation between the two strains were also investigated in light
of the protein data. The network-based representations also allowed new hypotheses
to be formed around proteins that were identified in the dataset, but
were of unknown function. / AFRIKAANSE OPSOMMING: Hierdie studie verken die gebruik van netwerke om proteonomiese data te visualiseer,
te interpreteer en te ontgin.
'n Netwerkgebaseerde benadering is gevolg ter ontleding van 'n kwantitatiewe
LC-MS/MS datastel wat afkomstig was van twee gis-spesies nl, Saccharomyces
cerevisiae ras VIN1 en Saccharomyces paradoxus ras RO88.
Die massaspektra is met bestaande en selfgeskrewe rekenaarprogramme verwerk
om 'n werkvloei saam te stel ter identifisering en kwantifisering van die
betrokke proteïene. Hierdie proteïene is dan aan bestaande biologiese databasisse
gekoppel om die proteïene in biologiese konteks te plaas. Die gekontekstualiseerde
is dan gebruik om biologiese netwerke van die data te bou. Die
kontekste beskou onder meer lokalisering van selaktiwiteite, ontologiese beskrywings,
ooreenkomste in aminosuur-volgordes en interaksies met bekende
proteïene asook assosiasie en verbintenisse met metaboliese paaie.
Hierdie kontekstuele, netwerk-gebaseerde voorstelling van die betrokke prote-
ïene het effektief duidelike data-tendense en patrone opgelewer wat andersins
nie opmerkbaar sou wees nie. Daarby het die kombinering van eksperimentele
data en bestaande biologiese bronne 'n beter perspektief aan die data-analise
verleen. Beide bestaande en nuwe hipoteses tov gis-selwandproteïene en prote
ïene met moontlike wynkundige potensiaal is ondersoek in die lig van hul
differensiële uitdrukking in die twee gis-spesies. Voorbeelde wat ondersoek is sluit in selwandproteïene soos GGP1 en SCW4 asook waasbeskermingsfaktorproteïen HPF2. Verskille tov kapasiteit mbt malo-etanoliese gisting is ook
gevind. Die netwerk-gebaseerde voorstellings het ook aanleiding gegee tot die
formulering van nuwe hipoteses mbt datastel-proteïene waarvan die funksies
tans onbekend is.
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| 62 |
Molecular typing of wine yeasts : evaluation of typing techniques and establishment of a databaseHoff, Justin Wallace 03 1900 (has links)
Thesis (MSc)--Stellenbosch University, 2012. / ENGLISH ABSTRACT: The yeast species, Saccharomyces cerevisiae and S. bayanus are well known for the key role
they play during alcoholic fermentation in both wine and beer industries. These yeasts are
available in pure active dried form and can be used to produce different wine styles and to
manage quality. There are more than 200 commercial wine yeast strains on the market and
include naturally isolated strains and hybrids. With all these commercial yeasts available, strain
authenticity is very important to the manufacturer of active dried wine yeasts (ADWY) because it
can prevent commercial losses and maintain market credibility. It is as important to the
winemaker as it may impact wine quality. Various traditional and molecular techniques have
been successfully applied to perform quality control of wine yeast strains.
The aims of this study were to evaluate electrophoretic karyotyping (CHEF) and PCRbased
methods to distinguish between Saccharomyces wine yeast strains and to establish a
database containing molecular profiles of commercial strains. CHEF karyotyping was chosen
because it is generally used in the wine industry to distinguish between wine yeast strains, but
can be time-consuming. Alternatively, PCR-based methods are considered to be reliable and
fast. These PCR methods included the evaluation of interdelta regions, multiplex-PCR of miniand
microsatellites, MET2 gene RFLP analysis and the use of several species-specific primers.
In this study, 62 commercial wine yeast strains, were randomly selected from various
manufacturers of ADWY, and two reference strains, S. bayanus CBS 380 and S. cerevisiae
CBS 1171, were evaluated. CHEF karyotyping could successfully differentiate between all 64
yeast strains. The two primer sets used for interdelta amplifications, delta1-2 and delta12-21,
yielded 59 and 62 profiles, respectively. Yeast strains considered to be similar or identical
according to interdelta amplification results, were resolved with CHEF karyotyping. CHEF
karyotyping was proven to be more accurate than interdelta amplifications in distinguishing
between commercial wine yeast strains. However, the results of interdelta amplifications were
very useful and less time-consuming. The multiplex-PCR of mini- and microsatellite primers only
succeeded in identifying a specific band within 55 of the 64 yeast strains including the S.
cerevisiae reference strain, a possible indication of species specificity. However, oenological
designation using MET2 gene RFLP analysis and species-specific primers indicated that all the
commercial strains in this study had a S. cerevisiae ancestry. Restriction analysis of the MET2
gene with EcoRI also successfully identified AWRI Fusion and Zymaflore X5 as hybrid yeast
strains. A wine yeast database was created and contains three libraries, i.e. CHEF karyotypes,
delta1-2 and delta12-21 electrophoretic profiles. The database was proven to be functional and
showed great accuracy in grouping and identifying test strains. The database has many
possible applications, but there is still some optimisation and refinement needed. / AFRIKAANSE OPSOMMING: Die Saccharomyces sensu stricto kompleks, is bekend vir die belangrike rol wat hierdie giste
speel tydens alkoholiese fermentasie in biede wyn en bier industrieë. Dit is om hierdie rede dat
kelders rein aktief gedroogte wyngis gebruik vir die produksie van spesifieke wynstyle, asook
kwaliteit. Daar is meer as 200 kommersiële wyngiste op die mark beskikbaar en dit sluit
natuurlike isolate en hibriede in. Daarom is gisras verifikasie baie belangrik vir die vervaardiger
van aktief gedroogde wyngiste asook die wynmaker om finansiële verliese te voorkom en mark
vertrouenswaardigheid te handhaaf. Verskeie tradisionele en molekulêre metodes word
suksesvol toegepas vir gehalte beheer van die gisrasse.
Die doel van hierdie studie was om elektroforetiese kariotipering (CHEF) en PKR
gebaseerde tegnieke se vermoë om tussen Saccharomyces wyngiste te onderskei, te
ondersoek. Ook deel van die doelwitte was om ‘n databasis te skep wat die verskillende
elektroforetiese profiele van die kommersiële gisrasse bevat. Tydens hierdie studie is 62
kommersiële gisrasse van verskeie vervaardigers ewekansig geselekteer. Saccharomyces
bayanus CBS 380 en S. cerevisiae CBS 1171 is as verwysingsrasse gebruik. Elektroforetiese
kariotipering (CHEF) is gekies omdat dit een van die mees algemeenste tegnieke is wat gebruik
word om tussen wyngiste te onderskei, maar dit word as tydrowend en arbeidsintensief beskou.
As ‘n alternatief is daar na PKR gebaseerde tegnieke gekyk. Hierdie tegnieke word as
betroubaar en vinnig beskou. Verskeie PKR gebaseerde tegnieke is ondersoek, naamlik PKR
van interdelta areas, multipleks-PKR van mini- en mikrosatelliete, MET2 geen RFLP analise en
die gebruik van spesie-spesifieke inleiers. Interdelta amplifikasies en mini- en makrosatelliet
inleiers is geselekteer as gevolg van hul vermoë om Saccharomyces wyngiste tot op spesie en
ras vlak te onderskei. Die MET2 geen en spesie-spesifieke inleiers is geselekteer om die
kommersiele wyngis as S. cerevisiae, S. bayanus of as hibriede te klassifiseer.
CHEF kariotipering kon tussen al 64 giste onderskeid tref. Die twee stelle inleiers wat vir
interdelta amplifikasie gebruik was, delta1-2 en delta12-21, het onderskeidelik 59 en 62 profiele
gelewer. Gis rasse wat identiese profiele met die delta inleiers gelewer het, kon egter met CHEF
kariotipering onderskei word. Die resultate het getoon dat CHEF kariotipering beter tussen die
kommersiële wyngiste kon onderskei as die interdelta amplifikasies, maar dat die interdelta
amplifikasies nogsteeds goeie onderskeiding toon en dat dit minder tydrowend is. Die
multipleks-PKR van mini- en mikrosatelliete kon slegs ‘n enkele band in 55 van die 64 giste uit
lig. ‘n Moontlike aanduiding van spesie spesifiekheid. Die oenologiese groepering volgens
MET2 geen analise en spesies-spesifieke inleiers dui aan dat al die kommersiele wyngiste wat
in hierdie studie gebruik is, moontlik van S. cerevisiae afkomstig is. Restriksie analise van die
MET2 geen met EcoRI het ook AWRI Fusion en Zymaflore X5 as hibriede geïdentifiseer. Die
CHEF kariotipes en interdelta elektroforetiese profiele is gebruik om ‘n databasis van die
kommersiële Saccharomyces wyngiste op te stel. Die databasis is funksioneel en het die toets rasse akkuraat geïdentifiseer en korrek gegroepeer. Die databasis moet egter nog verdere
optimisering en verfyning ondergaan.
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| 63 |
Industrial yeast strains engineered for controlled flocculationGovender, Patrick 03 1900 (has links)
Thesis (PhD (Viticulture and Oenology. Wine Biotechnology))--University of Stellenbosch, 2009. / In many industrial fermentation processes, Saccharomyces cerevisiae yeast should ideally meet two partially conflicting demands. During fermentation a high suspended yeast count is of paramount importance to maintain a rapid fermentation rate, whilst efficient flocculation should ideally be initiated only on completion of the primary alcoholic fermentation, so as to enhance product clarification and recovery. Most commercial wine yeast strains are non-flocculent, probably because this trait was counter-selected to avoid fermentation problems. In this study, we assessed molecular strategies to optimise the flocculation behaviour of non-flocculent laboratory and wine yeast strains. For this purpose, the chromosomal copies of three dominant flocculation genes, FLO1, FLO5 and FLO11, of a non-flocculent S. cerevisiae laboratory strain (FY23) and two commercial wine yeast strains (BM45 and VIN13) were placed under the transcriptional control of the stationary phase-inducible promoters of the S. cerevisiae ADH2 or HSP30 genes.
Under standard laboratory media and culture conditions, all six promoter-gene combinations resulted in specific flocculation behaviours in terms of timing and intensity. The data show that the strategy resulted in the expected and stable expression patterns of these genes in both laboratory and industrial wine yeast strains. Most importantly, the data confirm that inducible expression of the native FLO1 and FLO5 open reading frames, albeit to varying degrees, are responsible for a quantifiable cell-cell adhesion phenotype that can be characterized as a Flo1 flocculation phenotype. On the other hand, we found that inducible expression of the native FLO11 ORF under these conditions resulted in flor/biofilm formation and invasive growth phenotypes. However, the specific impact of the expression of individual dominant FLO genes with regard to characteristics such as flocculation efficiency, cell wall hydrophobicity, biofilm formation and substrate adhesion properties showed significant differences between the commercial strains as well as between commercial and laboratory strains. These adhesion phenotype differences may at least in part be attributed to wine yeast FLO gene open reading frames containing significantly smaller intragenic repeat regions than laboratory strains.
The data show that the ADH2 regulatory sequences employed in this study were unsuitable for the purpose of driving FLO gene expression under wine-making conditions. However, HSP30p-based FLO1 and FLO5 wine yeast transformants displayed similar flocculent phenotypes under both synthetic and authentic red wine-making conditions, and the intensities of these phenotypes were closely aligned to those observed under nutrient-rich YEPD conditions. The fermentation activities of
HSP30p-based transgenic yeast strains were indistinguishable from that of their parental host wine yeast strains. The chemical composition of wines obtained using transgenic yeast strains were similar to those produced by parental strains. The BM45-derived HSP30p-FLO5 transformant in particular was capable of generating compacted or ‘caked’ lees fractions, thereby providing a distinct separation of the fermented wine product and lees fractions. Furthermore, in this study we report a novel FLO11 induced flocculation phenotype that seems to exclusively develop under authentic red wine-making conditions. This strong FLO11 flocculation phenotype was not wine yeast strain dependant, possessed both Ca2+-dependant and Ca2+-independent flocculation characteristics and was insensitive to inhibition by both glucose and mannose. A distinct advantage of this unique FLO11 phenotype was highlighted in its ability to dramatically promote faster lees settling rates. Moreover, wines produced by HSP30p-FLO11 wine yeast transformants were significantly less turbid than those produced by their wild type parental strains. The benefit of this attractive property is it facilitates simpler and faster recovery of wines and also promotes greater volume recovery of the wine product.
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| 64 |
Modifying redox potential and its impact on metabolic fluxes in Saccharomyces cerevisiaeJain, Vishist Kumar 03 1900 (has links)
Thesis (PhD (Science) (Viticulture and Oenology. Wine Biotechnology))--University of Stellenbosch, 2010. / ENGLISH ABSTRACT: The production of glycerol by Saccharomyces cerevisiae under anaerobic conditions is
essential for maintaining the intracellular redox balance thereby allowing continuous
energy generation through conversion of sugars into ethanol. In addition, glycerol can
act as an osmolyte and is synthesized to maintain turgor pressure under hyperosmotic
conditions. The production of ethanol from sugars can be a redox-neutral process,
where the NAD+ (nicotinamide adenine dinucleotide) that is consumed during the
glycolytic conversion of glyceraldehyde-3-phosphate to pyruvate is later regenerated by
the reduction of acetaldehyde to ethanol. However, in particular the redirection of
metabolic flux of pyruvate to biomass formation leads to excess NADH formation. The
intracellular redox balance in these conditions is then primarily maintained through
formation of glycerol which is control by two main enzymes, namely Gpd1p and Gpd2p.
Deletion of the genes coding for these two proteins leads to accumulation of NADH and
renders the cells incapable of maintaining their fermentative ability and growth under
anaerobic conditions.
The goal of this study was to investigate the growth, fermentative ability and metabolite
synthesis of various gpd1Δgpd2Δ double mutant (DM) strains in which the redox
balancing potential was partially restored through expression of native or heterologous
genes. Strains were constructed by introducing alternative NADH oxidizing pathways or
manipulating existing pathways to favour the oxidation of excess NADH. More
specifically, the modifications included (i) sorbitol formation; (ii) establishing a pathway
for propane-1,2-diol formation; and (iii) increasing ethanol formation. Apart from
genetically manipulating the gpd1Δgpd2Δ double mutant, the addition of pyruvate
during growth was also investigated. The experiments were carried out under oxygen
limited conditions in a high sugar medium and the fermented product was analyzed for
total sugar consumed, biomass and primary and secondary metabolites formed by the
different strains. The relationships between sugar consumption, growth and metabolite
production by different strains were investigated by comparing the data generated from
the different strains by using multivariate data analysis tools. Analysis of the pathways
involved in the production of primary (acids, ethanol and other metabolites) and
secondary metabolites (aroma compounds) were also carried out in order to establish
flux modification in comparison to the wild type (WT) strain. The results revealed that these manipulations improved the fermentative capacity of the
gpd1Δgpd2Δ double mutant, suggesting a partial recovery of NAD+ regeneration ability,
albeit not to the extent of the WT strain. As expected a significant correlation was found
between sugar consumption and ethanol and biomass formation. Ethanol yields but not
final concentrations were increased by the genetic manipulations. Sorbitol by DM(srlD)
and DM(SOR1) strains and propane-1,2-diol by DM(gldA, GRE3, mgsA) strain were
formed in significant amounts although at lower molar yields than glycerol.
Furthermore, by genetic manipulation the yield of secondary metabolites (isobutanol,
isoamyl alcohol, 2-phenyl ethanol and isobutyric acid) was increased whereas the ethyl
acetate concentration and yield decreased. The results indicate that aroma compound
properties of wine yeasts could be favourably changed by manipulating the glycerol
synthesizing pathway. The addition of pyruvate during the growth of gpd1Δgpd2Δ
double mutant contributes to excess NADH re-oxidation through additional ethanol
formation. / AFRIKAANSE OPSOMMING: Die produksie van gliserol deur Saccharomyces cerevisiae onder anaërobiese
toestande is noodsaaklik vir die onderhouding van die intrasellulêre redoksbalans en
maak dus ononderbroke energie-ontwikkeling tydens die omsetting van suikers in
etanol moontlik. Daarbenewens kan gliserol as ‘n osmoliet optree en word dit
gesintetiseer om turgordruk onder hiperosmotiese toestande te onderhou. Die
produksie van etanol uit suikers kan ‘n redoksneutrale proses wees, waar die NAD+
(nikotinamiedadenien-dinukleotied) wat tydens die glikolitiese omskakeling van
gliseraldehied-3-fosfaat na piruvaat verbruik word, later deur die reduksie van
asetaldehied na etanol regenereer word. Die nasending van die metaboliese vloeiing
van piruvaat na biomassavorming lei egter na ‘n oormaat NADH-vorming. Onder hierdie
toestande word die intrasellulêre redoksbalans dan hoofsaaklik deur die vorming van
gliserol onderhou. Laasgenoemde word veral deur twee ensieme beheer, naamlik
Gpd1p en Gpd2p. Die delesie van die gene wat vir hierdie twee proteïene enkodeer, lei
tot ‘n akkumulasie van NADH en veroorsaak dat die selle nie hulle gistingsvermoë en
groei onder anaërobiese toestande kan onderhou nie.
Die doelwit van hierdie studie was om die groei, gistingsvermoë en metabolietsintese
van verskeie gpd1Δgpd2Δ dubbelmutant (DM) rasse te ondersoek waarin die
redoksbalanseringspotensiaal gedeeltelik herstel is deur die uitdrukking van inheemse
of heteroloë gene. Rasse is gekonstrueer deur alternatiewe NADH-oksiderende weë in
te voer of deur bestaande weë te manipuleer om die oksidasie van oormaat NADH te
bevoordeel. Meer spesifiek het die modifikasies die volgende ingesluit: (i)
sorbitolvorming; (ii) die vestiging van ‘n weg vir propaan-1,2-diol-vorming; en (iii) die
verhoging van etanolvorming. Buiten die genetiese manipulering van die gpd1Δgpd2Δ
dubbelmutant, is die byvoeging van piruvaat tydens groei ook ondersoek. Die
eksperimente is onder suurstofbeperkte toestande in ‘n hoë-suiker medium uitgevoer en
die gegiste produk is ondersoek vir totale suikerverbruik, biomassa en primêre en
sekondêre metaboliete wat deur die verskillende rasse gevorm is. Die verhoudings
tussen suikerverbruik, groei en metabolietproduksie deur die verskillende rasse is
ondersoek deur die data wat deur die verskillende rasse gegeneer is deur middel van
meerveranderlike data-analise te vergelyk. Analise van die weë wat in die produksie
van primêre (sure, etanol en ander metaboliete) en sekondêre metaboliete (aromaverbindings) betrokke is, is ook uitgevoer om die verandering in vloei te bepaal in
vergelyking met die wildetipe (WT) ras.
Die resultate het gewys dat hierdie manipulasies die gistingsvermoë van die
gpd1Δgpd2Δ-dubbelmutant verbeter het, wat ‘n gedeeltelike herstel van NAD+-
regenerasievermoë voorstel, hoewel nie tot dieselfde mate as in die WT-ras nie. Soos
verwag, is ‘n beduidende korrelasie tussen suikerverbruik en etanol- en
biomassavorming gevind. Etanolopbrengs is deur genetiese manipulasies verhoog,
maar nie die finale konsentrasies van etanol nie. Sorbitol is in beduidende hoeveelhede
deur die DM(srlD) en DM(SOR1)-rasse gevorm en propaan-1,2-diol deur die DM(gldA,
GRE3, mgsA) -rasse, hoewel teen laer molare opbrengste as gliserol. Verder is die
opbrengs van sekondêre metaboliete (isobutanol, iso-amielalkohol, 2-fenieletanol en
isobottersuur) deur genetiese manipulasie verhoog, terwyl die etielasetaatkonsentrasie
en -opbreng verlaag is. Die resultate dui aan dat die aromaverbindingseienskappe van
wyngiste voordelig verander kan word deur die gliserolsintetiseringsweg te manipuleer.
Die byvoeging van piruvaat tydens die groei van die gpd1Δgpd2Δ-dubbelmutant dra by
tot uitermate NADH-reoksidasie tydens die bykomende vorming van etanol.
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| 65 |
Transcriptional regulation of the endo-polygalacturonase-encoding gene in Saccharomyces cerevisiaeLouw, Campbell Trout 03 1900 (has links)
Thesis (PhD (Science) (Viticulture and Oenology. Wine Biotechnology))--University of Stellenbosch, 2010. / ENGLISH ABSTRACT: Wine fermentation with a yeast strain able to degrade grape cell polysaccharides can
result in improved processability and an increase in wine quality by improving extraction
of essential compounds from the grapes during the maceration stage. Pectin is the only
important cell wall polysaccharide that can be degraded by wild-type Saccharomyces
cerevisiae strains. Pectin is degraded by a polygalacturonase (PG) encoded by the
PGU1 gene (ORF YJR153W). Only certain S. cerevisiae strains can degrade pectin and
PG activity is thus strain specific. The lack of activity in certain strains has been
attributed to a number of factors: (1) the complete absence of the PGU1 gene, (2) the
PGU1 gene is present but the allele is dysfunctional and (3) the PGU1 gene is present
but not transcribed. The lack in transcription has been shown to be due to the gene
having a dysfunctional promoter or to regulatory differences between strains. Results
published in the literature are contradictory. The primary aim of this investigation was to
clarify the regulation of PG activity in S. cerevisiae and to determine why there are
differences in PG activity between different strains. Regulation of PG activity between
several wine and laboratory strains with varying PG activities was compared by looking
at the sequence of the PGU1 gene and its promoter as well as transcription levels of
this gene and its main transcription factors, TEC1 and STE12. In order to identify
regulatory factors influencing PG activity, the S. cerevisiae genome was screened for
activators and inhibitors of PG activity. Fourteen inhibitors and two activators of PG
activity were identified during this screen. Real-time PCR analysis showed that the PG
activity is regulated by transcription of the PGU1 gene. A linear relationship was
demonstrated between PGU1 and its two transcription factors TEC1 and STE12. Some
of the genes identified as inhibitors of PGU1 transcription are involved in gene silencing
by Telomere Position Effect (TPE) indicating that PGU1 is possibly silenced due to its
subtelomeric location within 25 kb from the right telomere of chromosome X. Moving the
PGU1 gene with its native regulatory machinery to a different position away from its
telomere resulted in an increase in PGU1 transcription and PG activity, demonstrating
the epigenetic influence on PGU1 regulation. Results from this study suggested that the
strain related difference in PGU1 expression occurs at an epigenetic level, with steric
hindrance preventing RNA polymerase access to the PGU1 promoter and thus inhibiting
transcription of this gene in some strains. Understanding regulation of PG activity can potentially lead to the development of more
effective strategies to improve PG degradation by S. cerevisiae. The genetic model
describing regulation of PGU1 transcription was extended by this study and a novel
mechanism of regulation of PG activity was identified.
The secondary aim of this study written as an addendum to this thesis, focussed on
degradation of another grape cell wall polysaccharide xylan by recombinant strains of S.
cerevisiae. These strains were enabled to degrade this polysaccharide through
heterologous expression of novel xylanase encoding genes from various origins.
Xylanase activity of the recombinant strains generated was compared. Overexpressing
the complete gene xynA of Ruminococcus flavefaciens, the functional domain xynAa or
the functional domain xynAc within optimal conditions for these enzymes all conferred
very low xylanase activity to S. cerevisiae, with xynAc resulting in the highest xylanase
activity. Since overexpression of the R. flavefaciens xynA gene yielded very low activity
under optimal conditions activity in wine making conditions would be negligible. The
genes XYN2 and XYN4 from Trichoderma reesei and Aspergillus niger respectively
yielded higher levels of activity. According to these results, only the expression of XYN2
and XYN4 could have a potential effect on wine
An effective strategy for improving pectin degradation can in future potentially be
combined with heterologous expression of a xylanase encoding gene in S. cerevisiae in
order to engineer a wine yeast strain with improved polysaccharase abilities. / AFRIKAANSE OPSOMMING: Gisting van druiwe met polisakkaried-afbrekende gisrasse kan lei tot ‘n verbetering in
wyn prosessering en tot die produksie van hoër kwaliteit wyne deur die ekstraksie van
belangrike wynkomponente uit druifselle te verbeter. Pektien is die hoof komponent van
die druifselwand wat deur wilde tipe Saccharomyces cerevisiae giste afgebreek kan
word en word afgebreek deur ‘n poligalaktoronase (PG) wat deur die PGU1 (YJR153W)
geen gekodeer word. Slegs spesifieke gisrasse kan pektien afbreek en die ensiem
aktiwiteit is dus ras-spesifiek. Die gebrek aan PG aktiwiteit in sekere rasse is al omskryf
as gevolg van die afwesigheid van die geen, die teenwoordigheid van ‘n nie-funksionele
alleel of dat die geen wat teenwoordig is nie uitgedruk word nie. Transkripsie is al
bewys om nie plaas te vind nie a.g.v. die teenwoordigheid van ‘n nie-funksionele
promotor of a.g.v. ‘n verskil in regulering van transkripsie tussen rasse. Sommige
studies wat PG regulering ondersoek het, het teenstrydige resultate verkry. Die
hoofdoel van hierdie studie was om PG regulering te ondersoek en te bepaal waarom
daar verskille in PG aktiwiteit tussen verskillende gisrasse voorkom. Regulering van PG
aktiwiteit is ondersoek tussen wyn en laboratorium gisrasse met wisselende vlakke van
PG aktiwiteit deur die DNS volgorde van die PGU1 geen en sy promotor, so wel as die
DNS volgorde van die geen se hoof transkripsie faktore TEC1 en STE12 te bepaal. Om
reguleerders van PG aktiwiteit te identifiseer is die genoom van die gis S. cerevisiae
ondersoek om faktore te identifiseer wat PG aktiwiteit aktiveer of inhibeer. “Real-time
PCR” het bewys dat PG aktiwiteit gereguleer word deur transkripsie van die PGU1 geen
en dat daar ‘n lineêre verhouding tussen die transkripsie van die PGU1 geen en sy twee
hoof transkripsie faktore TEC1 en STE12 bestaan. Sommige van die gene wat
geïdentifiseer is as inhibeerders van PG aktiwiteit is voorheen bewys om betrokke te
wees by die inhibering van transkripsie deur middel van die telomeer posisie effek, dit
dui daarop dat transkripsie van die PGU1 geen moontlik geïnhibeer word as gevolg van
die geen se subtelomeriese posisie binne 25 kb vanaf die regter telomeer van
chromosoom X. Die PGU1 geen is met sy natuurlike regulerings elemente na ‘n ander
posisie in die genoom, weg van sy naaste telomeer geskuif, die verandering in posisie
van die geen het gelei tot ‘n toename in PG aktiwiteit en transkripsie van die PGU1
geen en het dus bewys regulering word beïnvloed deur ‘n epigenetiese effek. Die
resultate van hierdie studie het daarop gedui dat die verskil in transkripsie van die
PGU1 geen plaasvind op ‘n epigenetiese vlak waartydens die chromatien struktuur toegang van die RNA polimerase tot die PGU1 geen voorkom en dus word transkripsie
van die geen sodoende in sommige rasse voorkom.
Die tweede doelwit van hierdie studie het gefokus op die afbraak van ‘n ander
komponent van die druif selwand, xilaan, deur S. cerevisiae. Hierdie navorsing vorm ‘n
addendum aan die tesis en Xylanase aktiwiteit van verskeie rekombinante rasse is in
hierdie studie vergelyk. Baie lae xylanase aktiwiteit is verleen aan rekombinante giste
wat die volledige xynA geen gekloneer van die bakteriee Ruminococcus flavefaciens,
asook twee aktiewe domeins van die geen, domein xynAa en domein xynAc uitdruk.
Van die voorafgenoemde giste het die uitdrukking van die domein xynAc die
rekombinante gis ras met die hoogste aktiwiteit tot gevolg gehad. Ooruitdrukking van
die gene XYN2 en XYN4 wat gekloneer is van die fungi Trichoderma reesei en
Aspergillus niger onderskeidelik, het beide gisrasse wat oor hoë vlakke van xylanase
aktiwiteit beskik tot gevolg gehad. Hierdie resultate dui dus daarop dat van die gene
ondersoek in die studie, slegs XYN2 en XYN4 potensiaal het om xylanase aktiwiteit van
wyngiste te verbeter.
Deur die regulering van PG aktiwiteit te bestudeer kan meer effektiewe strategieë
potensieel ontwikkel word om PG aktiwiteit in S. cerevisiae te verbeter. Hierdie studie
het die genetiese model wat PG regulering omskryf uitgebrei deur ‘n nuwe meganisme
van regulering van toepassing op PGU1 te identifiseer.
As ons die regulering van die PGU1 goed verstaan kan dit in die toekoms gekombineer
word met ‘n effektiewe strategie om ‘n gis aan te pas om xylaan af te breek, om
sodoende ‘n wyngis geneties te verbeter om beide xylaan en pektien te kan afbreek.
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Characterization and evaluation of glucose oxidase activity in recombinant Saccharomyces cerevisiae strainsMalherbe, Daniel Francois 03 1900 (has links)
Thesis (PhD)--Stellenbosch University, 2010. / ENGLISH ABSTRACT: Popular wine styles prepared from fully-ripened, more mature grapes are characterized
by intense fruitiness and varietal flavors. However, lengthy maturation of
grapes in the vineyard does not only translate into higher flavor intensity but also
into higher sugar levels, which, in turn, leads to wines with higher concentrations of
alcohol. Excessive alcohol levels can compromise wine flavor and render wine unbalanced.
This, along with health issues and anti-social behavior linked to high-risk
alcohol consumption patterns, stricter legislation and increased tax rates associated
with high-alcohol wines, have increased demand for wines with reduced alcohol
concentrations, without loss of the intense fruity aromas. Although low-alcohol
wines can be made using physical post-fermentation processes, such approaches are
often expensive and can impact adversely on wine flavor. As an alternative strategy,
yeast strains are being developed by several research groups to convert some of the
grape sugars into metabolites other than ethanol.
Based on promising results from previous preliminary work, this study focused
on the development of an industrial Saccharomyces cerevisiae wine strain producing
glucose oxidase (GOX; b-D-glucose:oxygen oxidoreductase, EC 1.1.3.4).
GOX oxidizes b-D-glucose to D-glucono-d-lactone and gluconic acid (GA) extracellularly,
thus preventing its entry into glycolysis, thereby diverting a portion of the sugar carbon away from ethanol. The GOX-encoding gene from the foodgrade
fungus, Aspergillus niger was used to construct three cassettes (GOX1, GOX2
and GOX2LOX). In these gene cassettes, the A. niger GOX gene was placed under
the regulation of the S. cerevisiae phosphoglycerate-kinase-1 gene promoter
(PGK1P) and terminator (PGK1T ). To facilitate secretion, in GOX1 the yeast mating
pheromone-factor a secretion signal (MFa1S) was fused to the GOX gene, and
in GOX2 the native A. niger secretion signal of GOX was used. These gene cassettes
were each integrated into the genome of two laboratory yeast strains (BY4742 and
S1278b) and one industrial wine yeast strain (VIN13). An additional integration
cassette, designated GOX2LOX, was constructed to knock out the IME1 gene in S.
cerevisiae. In GOX2LOX, GOX2 was fused to a loxP cassette. VIN13-D1 was obtained
by integrating a single copy of GOX2LOX into the IME1 locus. To generate
an asporogenic, GOX-producing wine yeast, VIN13-D2 was created by sporulation,
micromanipulation and re-diploidisation of VIN13-D1. Comparative analysis indicated
that (i) GOX2 resulted in higher levels of extracellular glucose oxidase activity
than GOX1; and that (ii) the levels of secreted glucose oxidase activity in the wine
yeast transformants were sufficiently high to conduct follow-up small-scale wine
fermentation trials.
The wine yeast transformant, VIN13-D1 was evaluated under red and white experimental
winemaking conditions. Results from this work indicated that glucose
oxidase was produced and secreted by VIN13-D1 that dominated the fermentation
to the end, but also that the enzyme was not highly active under the evaluated winemaking
conditions. Consequently, no significant decrease in ethanol concentrations
was observed in the wine made from VIN13-D1 when compared to that from
VIN13. Wine samples were analyzed by Fourier transform-middle infrared spectrometry
(FT-MIR) to determine the chemical composition and Gas chromatography
with a flame ionization detector (GC-FID) to evaluate the concentrations of
aroma compounds. The levels of gluconic acid were determined by enzymatic assays.
Multivariate data analysis (PCA and PLS1-discrim) was applied to highlight
significant differences between the wines made by VIN13 (wild-type) and VIN13-
D1. Chemometric projections of the score plots for all results allowed insight into
all significant variation up to three principal components (PCA) or PLS components,
which showed very clearly that GA is a key factor in evaluating the effect of
GOX in VIN13-D1 fermentation with regard to VIN13 fermentations. The VIN13-
D1 effect manifestations were best shown on PLS1-discrim score plots that revealed that, of the restricted variable subsets the FT-MIR-compounds and GC-compounds
yielded better results, with the GC-compounds displaying greater discriminability
between cultivars and VIN13 / VIN13-D1. It can be concluded from these results
that the greatest influence of VIN13-D1 produced wines could be observed in the
aroma components, but, because there were also discriminability effects discernable
in the FT-MIR-compounds, thus the flavor components were also affected.
The activity of GOX in grape juice was further investigated in controlled small
scale fermentations performed in a bio-reactor. It was confirmed that GOX is active
under aerobic conditions, inactive under anaerobic conditions, and can be activated
instantly when an anaerobic culture is switched to aerobic conditions (simulated
micro-oxygenation). These fermentations showed that glucose oxidase is active in
grape juice, and that oxygen play a key-role in the enzyme’s activation. Finally, it
was shown with the help of a simplified model, that under ideal conditions, GOX
secreted from VIN13-D1, can be employed to reduce the ethanol by a predefined
concentration for the production of low alcohol wines.
This work gives more insight into how to employ a GOX-producing wine yeast
during winemaking and strongly suggests the use of micro-oxygenation to activate
the enzyme in order to reduce available glucose, thereby diverting a portion of the
sugar carbon away from ethanol production. / AFRIKAANSE OPSOMMING: Gewilde wynstyle word dikwels gemaak van volryp, goed ontwikkelde druiwe,
gekarakteriseer deur intense aromas en smaakkomponente wat direk met spesifike
kultivars geassosieer word. ’n Nadelige gevolg om druiwe te lank aan die wingerdstok
te laat bly hang sodat meer intense geurkomponente kan ontwikkel, is die
toename in suikerinhoud. Hierdie addisionele suiker lei tot wyne met hoër alkoholvlakke.
Te hoë alkoholvlakke kan wyn ongebalanseerd laat voorkom en die
smaak nadelig beïnvloed. Dit, tesame met gesondheidsredes en anti-sosiale gedrag
wat gekoppel kan word aan die inname van te veel alkohol, strenger wetgewing
aangaande dronkbestuur en die toename in belasting op wyne met ’n hoër alkoholinhoud,
het aanleiding gegee tot ’n aanvraag vir wyn met ’n verlaagte alkoholinhoud,
sonder dat aroma- en geurkomponente ingeboet word. Alhoewel daar sekere
fisiese/gemeganiseerde prosesse beskikbaar is om die alkohol in wyn te verwyder of
te verminder, is ’n nadeel dat hierdie prosesse baie duur en arbeidsintensief is, en dat
dit deur sommige wynpuriste as te ingrypend in die ‘natuurlike’ proses van wynmaak
beskou word. Sommige van hierdie alkoholverwyderingsprosesse kan ook die wyn se geur- en aromakomponente nadelig beïnvloed. As alternatief tot hierdie
fisies-chemiese prosesse word wyngiste reg oor die wêreld deur verskillende
navorsingsgroepe ontwikkel sodat van die druifsuikers nie na alkohol omgeskakel
word nie, maar eerder ander metaboliete.
Belowende navorsingsresultate in ’n voorafgaande studie het aanleiding gegee
tot hierdie navorsingsprojek. In hierdie studie word daar klem gelê op die ontwikkeling,
deur middel van genetiese manipulering, van ’n industriële wynras van
Saccharomyces cerevisiae sodat dit in staat sal wees om glukose-oksidase (GOX;
b-D-glukose:suurstof oksidoreduktase, EC 1.1.3.4) te produseer. GOX kan reeds
b-D-glukose in die medium oksideer na glukoonsuur (GA), wat sodoende verhoed
dat dit verder gemetaboliseer word via glukolise, en dit het tot gevolg dat
’n gedeelte van die beskikbare suiker nie omgeskakel word na alkohol nie. Die
strukturele glukose-oksidase-geen (GOX) van die voedsel-gegradiëerde fungus, Aspergillus
niger is gebruik tydens die konstruksie van drie kassette (GOX1, GOX2 en
GOX2LOX). Binne hiedie geenkassette is A. niger se GOX-geen se transkripsieinisiëring
en -terminering onafhanklik deur die fosfogliseraat-kinase-1-promotor
(PGK1P) en termineerder (PGK1T ) bewerkstellig. Om uitskeiding van GOX uit die
gis te bewerkstellig, is daar van die a-spesifieke gisferomoon-a-faktor (MFa1S)
in GOX1 gebruik gemaak, en in GOX2, van A. niger se eie natuurlike sekresiesein.
Hierdie geenkassette is binne-in die genoom van twee labaratoriumgisrasse
van S. cerevisiae (BY4742 en S1278b) asook een industriële wyngisras (VIN13)
geintegreer. ’n Addisionele integreringskasset (die sogenaamde GOX2LOX-kasset)
is gemaak om die IME1-geen van S. cerevisiae te elimineer. Binne die GOX2LOXkasset
is GOX2 aan ’n loxP-kasset gekoppel. Die nuwe wyngis VIN13-D1 is verkry
deur ’n genomiese integrasie van GOX2LOX binne-in die IME1-lokus. Om die niesporulerende
GOX-produserende wyngis VIN13-D2 te verkry, is VIN13-D1 gesporuleer,
onderwerp aan mikromanipulasie en toegelaat om te herdiploidiseer. Ontledings
het aangedui dat (i) GOX2 aanleiding gegee het tot hoër vlakke van ekstrasellulêre
glukose-oksidase aktiwiteit in vergelyking met GOX1; en (ii) dat die
vlakke van uitgeskeide biologies-aktiewe glukose-oksidase vir die wyngisrasse aansienlik
hoër was. Dit het verdere kleinskaalse wynfermentasies geregverdig.
Die getransformeerde wyngis VIN13-D1 is op eksperimentele skaal in die maak
van rooi- en witwyn geëvalueer. Ontledings van hierdie eksperimentele wyne het
daarop gedui dat glukose-oksidase deur die VIN13-D1-gisselle geproduseer en suksesvol
uitgeskei tydens die wynmaakproses is, en dat VIN13-D1 die fermentasie gedomineer het en die alkoholiese gisting voltooi het. Resultate het egter ook aangedui
dat die geproduseerde glukose-oksidase nie baie aktief was onder die wynmaaktoestande
wat in hierdie eksperimentele wynmaakproses gegeld het nie, en gevolglik
was daar nie ’n drastiese verlaging in die alkoholvlakke sigbaar toe VIN13-D1
se wyne met VIN13 se wyne vergelyk is nie. Wynmonsters is deur middel van
Fourier-transformasie-mid-infrarooispektroskopie (FT-MIR) ontleed ten einde die
chemiese samestelling te bepaal, en gaschromatografie-massaspektrometrie (GCMS)
is aangewend om die wynaromakomponente te bepaal. Die vlakke van glukoonsuur
is deur middel van ensiematiese reaksies bepaal. Multiveranderlike data-analise
[hoofkomponentanalise (PCA) en parsiële kleinte kwadrate (PLS1) diskriminantanalise]
is op die data van die verskeie analitiese tegnieke toegepas om onderliggende
veskille tussen die wyne van VIN13 (wilde-tipe) en VIN13-D1 uit te wys. Chemometriese
projeksies het aangetoon dat daar wel beduidende variasies sigbaar was tot en
met drie hoofkomponente en/of PLS-komponente wat duidelik aandui dat glukoonsuur
’n sleutelfaktor was ten opsigte van die uitwerking wat GOX op VIN13-D1-
fermentasies in vergelyking met VIN13-fermentasies. VIN13-D1 effek manifestasies
is die beste waargeneem op grafieke wat PLS1-diskriminantanalise-data bevat.
Verder het PLS1-diskriminantanalise ook aangetoon dat van die ‘groepe’ wat
gebruik was tydens die analise, die FT-MIR-komponente en die GC-komponente
beter resultate gelewer het. Die GC-komponente het hulle verder daartoe geleen
om tussen die verskillende kultivars en VIN13/VIN13-D1-fermentasies te diskrimineer.
Daar kan dus met sekerheid gesê word dat die grootste invloed in VIN13-D1
wyne sigbaar is in die aromakomponent, maar omdat daar wel ook variasies sigbaar
was in die MIR-komponente, dat die smaakkomponente ook beïnvloed was.
Die aktiwiteit van GOX in druiwesap is verder ondersoek deur gebruik te maak
van kleinskaalse fermentasies in bioreaktors. Daar is bevestig dat die VIN13-D1-
geproduseerde GOX biologies-aktief was tydens aerobiese kondisies, onaktief was
tydens anaerobiese kondisies, en onmiddelik geaktiveer kon word wanneer ’n anaerobiese
fermentasie aerobies gemaak word (gesimuleerde mikro-oksigenasie). Hierdie
verskillende fermentasies dui daarop dat glukose-oksidase inderdaat aktief is in
druiwesap, en dat suurstof ’n sleutelfaktor is tydens die aktivering van die ensiem.
Met behulp van ’n vereenvoudigde model kon aangetoon word dat tydens ideale
toestande dit wel moontlik is om die alkoholvlakke te verlaag na ’n voorafbepaalde
konsentrasie vir die bereiding van lae-alkohol wyne.
Hierdie studie verskaf verdere insig hoe om ’n GOX-produserende wyngis gedurende die wynmaakproses vir die verlaging van die alkoholvlakke te benut. Verder
is dit duidelik dat suurstof van kardinale belang is vir die aktivering van die glukoseoksidase-
ensiem en dat ’n tegniek soos mikro-oksigenasie ’n belangrike rol in hierdie
verband tydens die wynmaakproses sou kon speel.
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Fructophilic yeasts to cure stuck fermentations in alcoholic beveragesSutterlin, Klaus A. (Klaus Alfred) 03 1900 (has links)
Thesis (PhDAgric (Viticulture and Oenology. Wine Biotechnology))--University of Stellenbosch, 2010. / ENGLISH ABSTRACT: Stuck alcoholic fermentations are a major enological problem for the international
winemaking industry. Incomplete wine fermentations are frequently characterized by high
residual fructose concentrations and the near-absence of residual glucose, a fact that is due to
the glucophilic character of the wine yeast Saccharomyces cerevisiae. Wines with high contents
of post fermentation sugar are very susceptible for microbial spoilage since residual fructose
and/or glucose can be metabolized by bacteria and yeast to undesired by-products such as
volatile acid and off-flavours, resulting in wine spoilage and considerable economic losses. It
has been reported that stuck fermentations are usually caused by several synergistically acting
inhibition factors, and the glucose to fructose ratio (GFR) is thought to play an important role in
this context. This study is aimed at contributing towards a better understanding of this industrial
problem, and at finding industrially applicable solutions.
In a first part, this study describes the isolation of two appropriate strains of the
fructophilic yeast Zygosaccharomyces bailii from the natural microflora of grapevine, followed by
trials in small scale test fermentations using stuck industrial fermentations as model media.
These experiments were expanded to also investigate large scale industrial fermentations. As a
result, a strategy for the treatment of stuck fermentations was developed and successfully
applied in several wineries with fermentation problems. This methodology represents an entirely
novel and industrially applicable solution to high residual fructose levels.
In a second part, the data contributes to elucidating the molecular nature of the
fructophilic phenotype of Z. bailii by characterizing some of the genes and proteins that may be
responsible for the fructophilic character. In particular, the investigation focused on the first two
steps of hexose metabolism, the transport of sugar into the cell by permeases and sugar
phosphorylation by hexokinases, which combined are thought to be primarily responsible for
sugar preference.
One result of this study was Fructoferm W3©, a dry yeast product which is commercially
available. Fructoferm W3 was awarded with the innovation medal for enological products at
Intervitis/Interfructa, Stuttgart, Germany in 2007. / AFRIKAANSE OPSOMMING: Die voorkoms van steek alkoholiese fermentasies is ‘n ernstige problem in die internasionale
wyn industrie. Onvolledige fermentasies word dikwels gekenmerk deur hoë residuele fruktose
konsentrasies en die veitlike afwesigheid van residuele glukose. Die kenmerke kan meestal
toegeskryf word aan die glukofilliese kakakter van die wyngis Saccharomyces cerevisiae. Wyne
met ‘n hoë suiker inhoud na die afloop van fermentasie is vatbaar vir mikrobiese bederf
aangesien residuele fruktose en/of glukose gemetaboliseer kan word deur bakterië en gis om
ongewenste byprodukte soos vlugtige sure en bygeure te vorm wat kan lei tot wyn bederf en
aansienlike ekonomies verlies. Dit is vasgestel dat steek fermentasies gewoonlik veroorsaak
word deur verskeie sinergisties werkende inhibisie faktore, waartoe die glukose/fruktose
verhouding ‘n noemenswaardiege bydrae lewer. Die mikpunt van hierdie studie was om ‘n
bydrae te lewer tot die begrip van steek fermentasies en die daarstelling van moontlike
industriële oplossings.
Die eerste deel van die werk beskryf die isolasie van twee rasse van die gis
Zygosaccharomyces baillie uit die natuurlike wingerd mikroflora, gevolg deur steekproewe in die
vorm van kelinskaalse fermentasies met steek industriële fermentasies gebruik as model media.
Hierdie ekserimente is vervolgens uitgebrei om grootskaalse industriële steek fermentasies te
bestudeer. Die uitkoms van hierdie werk het gelei tot die ontwikkeling van ‘n strategie vir die
behandeling van steek fermentasies wat susksesvol toegepas is in verskeie wynmakerye. Die
metodiek bring ‘n nuwe en industrieel toepasbare oplossing vir hoë residuele fruktose vlakke.
Die data aangebied in die tweede afdeling dra by tot die verheldering van die molekulêre natuur
van die fruktofilliese fenotipe van Z. baillie deur die tipering van gene en protiëne wat moontlik
verantwoordelik is vir die fruktofilliese karakter van die gis. Die ondersoek het spesifiek op die
eerste twee stappe van heksose metabolisme, naamlik die invoer van suiker in die sel deur
permeases en suiker fosforilering deur heksokinases, gekonsentreer. Die kombinasie van die
twee prosesse is vermoedelik verantwoordelik vir die regulering van suiker voorkeur.
‘n Gevolg van die studie was die ontwikkeling van ‘n droë gisproduk, Fructferm W3©, wat
kommersieel beskikbaar gestel is. Fructoferm W3 is in 2007 toegeken met die innovasie
medalje vir wynkundige produkte by Intervittis/Interfructa in Stuttgart, Duitsland.
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The control of cellular adhesion of Saccharomyces cerevisiae by the FLO gene regulator Mss11pBester, Michael Christiaan 03 1900 (has links)
Thesis (PhD (Science) (Viticulture and Oenology. Wine Biotechnology))--University of Stellenbosch, 2010. / ENGLISH ABSTRACT: The yeast Saccharomyces cerevisiae senses change within its environment and responds
through specific adaptive cellular programmes, in particular by modifying gene expression.
Many adaptive changes affect the physico-chemical properties of the cell wall, and several
mechanisms that specifically affect the expression levels of genes that encode for cell wall
components have been described previously. Cell wall modification directly impacts on general
cell wall properties and cell-cell and cell-surface interactions. Many of these properties have
been directly linked to families of cell wall proteins referred to as adhesins. In particular
members of the Flocculation (FLO) gene family have been shown to play a crucial role in
adhesion phenotypes. Flo11p functions in a variety of phenotypes including agar invasion,
plastic adhesion and the formation of pseudohyphae, “flor” and “mats”, whereas Flo1p appears
to control flocculation. The regulation of FLO11 expression is well documented and is mainly
controlled by the mitogen activated protein kinase (MAPK) and cyclic AMP protein kinase A
(cAMP-PKA) signalling cascades. Genetic analysis shows that Mss11p acts downstream and is
central to these pathways, and furthermore interacts with the cAMP-PKA component Flo8p to
activate transcription. In this study we further explore additional gene targets of Flo8p and
Mss11p, as well as their regulation and their impact on cell wall characteristics and associated
adhesion phenotypes.
Our analysis shows that Mss11p is also required for FLO1 expression, and functions
together with Flo8p to control many Flo-dependent adhesion phenotypes. Genome-wide gene
expression analysis further reveals that altered Mss11p levels leads to the change in the
expression of various cell membrane and cell wall genes, notably AQY2 and members of the
DAN and TIR gene families. Further genetic analysis indicates that adhesion phenotypes
display an almost exclusive dependence on FLO gene expression. We also demonstrate that
these phenotypes require Flo10p and are thus dependent on the specific balance of Flo
proteins in the cell wall. The analysis of signalling deletion mutants show that regulation of
FLO10 shares signalling components with FLO11, but that the two genes are differentially
regulated. Unlike FLO11, FLO10 transcription also does not display an absolute requirement for
Mss11p but rather for the MAPK component Ste12p.
Whole genome expression analysis were also performed on strains with altered levels of
Flo8p which were compared with the above mentioned transcriptome data set. This analysis
shows that Flo8p and Mss11p co-regulate the FLO genes, as well as AQY2 and TIR3, but also
have significant unique gene targets. The combination of transcriptome data with current
information concerning transcription factor (TF) interaction networks reveals the importance of
network interaction between Cin5p, Flo8p, Mga1p and Mss11p. From these data we
constructed a TF interaction model in which Flo8p acts as the predominantly activating TF
component, whereas Mss11p function as a target hub TF, possibly as a mediator- or
polymerase II holo-enzyme component.
Finally we provide a first report on “mat” formation by an industrial wine yeast strain, and
show that by adjusting FLO11 expression in this strain we are able to significantly change this
phenotypic behaviour. / AFRIKAANSE OPSOMMING: Die gis Saccharomyces cerevisiae neem veranderinge in sy omgewing waar en reageer daarop
deur middel van spesifieke sellulêre programme, in die besonder deur geenuitdrukking aan te
pas. Verskeie aanpasbare veranderinge beïnvloed die fisieke, asook chemiese eienskappe van
die selwand, en talle meganismes is al beskryf wat die uitdrukkingsvlakke beïnvloed van gene
wat vir selwandkomponente kodeer. Die modifikasie van die selwand het ’n direkte impak op
selwand-eienskappe, asook die sel-sel- en sel-oppervlak-interaksies. Verskeie van hierdie
eienskappe word direk gekoppel aan die selwandproteïenfamilies, wat ook as adhesie-faktore
bekend staan. Veral lede van die Flokkulasie (FLO) -geenfamilie het ’n noodsaaklike funksie in
adhesie-fenotipes. Flo11p speel ’n rol in verskeie fenotipes, wat insluit die indringende groei van
agar, plastiekaanhegting en die vorming van pseudohifes, “flor“ en “matte“, terwyl Flo1p
flokkulasie beheer. Die regulering van FLO11-uitdrukking is deeglik gedokumenteerd en dit
word hoofsaaklik gereguleer deur die mitogeen-geaktiveerde proteïenkinase (MAPK) en sikliese
AMP-proteïenkinase A (cAMP-PKA) seintransduksiekaskades. Genetiese analises toon dat
Mss11p stroom-af en sentraal tot hierdie kaskades funksioneer, en dit aktiveer transkripsie deur
interaksie met die cAMP-PKA-komponent, Flop8. In hierdie studie word ’n ondersoek gedoen
na addisionele teikengene van Flo8p en Mss11p, en hoe hierdie gene gereguleer word, asook
hul impak op selwandeienskappe en geassosieerde adhesie-fenotipes.
Ons analises toon dat Mss11p ook benodig word vir die ekspressie van FLO1 en dat dit,
tesame met Flo8p, beheer uit oefen oor verskeie Flo-afhanklike fenotipes. Genoomwye
geenekspressie-analises wys verder daarop dat veranderde Mss11p-vlakke lei tot die
aanpassing van die ekspressie van verskeie selmembraan- en selwandgene, naamlik AQY2
asook lede van die DAN- en TIR-geenfamilies. Verdere genetiese analise dui daarop dat
adhesie-fenotipes byna eksklusief afhanklik is van FLO-geenekspressie. Daar is verder getoon
dat hierdie fenotipes ook Flo10p benodig en dus afhanklik is van die spesifieke balans van Floproteïene
in die selwand. Die analise van seintransduksiemutante demonstreer dat FLO10 en
FLO11 seintransduksie-komponente deel, maar dat hierdie gene verskillend gereguleer word.
Anders as FLO11, toon FLO10 nie ’n absolute noodsaaklikheid vir Mss11p nie, maar eerder vir
die MAPK-komponent, Ste12p.
Totale genoomekspressie-analises is ook gedoen op gisrasse met aangepaste vlakke van
Flo8p en dis vergelyk met bogenoemde transkripsiedatastel. Hierdie analise wys dat Flo8p and
Mss11p die FLO-gene, asook AQY2 en TIR3, koreguleer, maar ook beduidende unieke
teikengene het. Die kombinasie van transkripsiedata met huidig beskikbare informasie
betreffende transkripsiefaktor (TF) -interaksienetwerke dui op die relevansie van
netwerkinteraksie tussen Cin5p, Flo8p, Mga1p en Mss11p. Hiervan is daar ’n model opgestel
waarin Flo8p in die meeste gevalle as die aktiverende TF-komponent optree, terwyl Mss11p as
TF-teiken dien, moontlik as ’n mediator- of polimerase II holoënsiemkomponent.
Laatens word daar vir die eerste keer verslag gedoen van ”mat”-vorming deur ’n industriële
wyngisras en toon ons verder dat hierdie fenotipe beduidend verander word deur middel van die
aanpassing van FLO11-uitdrukking.
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The colour and phenolic content of Robertson Red grape cultivars : distribution, correlation with wines and analysesVan der Merwe, Hanneli 03 1900 (has links)
Thesis (PhD)--Stellenbosch University, 2013. / ENGLISH ABSTRACT: South African red wine is often acknowledged world wide as being full bodied and deep in
colour. This is often the result of high temperatures that is experienced during the important
growth stages of grapes especially post véraison. In the Robertson area in South Africa
however, temperatures often exceeds the range for optimal anthocyanin development during
these growth stages. The distinction between grapes being technologically ripe and being ripe
on a phenolic level is also accepted as an important determining factor for the perfect time to
pick grapes. In co-operative wineries such as Robertson Winery (RW) where grapes are
delivered from a large area and different producers, it is difficult to individualise grape blocks
when it comes to ripeness level in terms of sugar or phenolic ripeness. In most circumstances a
generalised set of parameters for deeming grapes ripe or acceptable for delivery is the best
substitute. The levels of these parameters are based on research literature that is available for
the area as well as data collected through years of maintaining the vineyards of that area. The
grape parameters that are currently being used by RW for ripeness and quality are pH, titratable
acidity (TA) and sugar level. In recent years RW in conjunction with the Department of
Viticulture and Oenology, Stellenbosch University, decided to investigate more parameters to
determine the quality of grapes at the time of harvest. Most importantly for the grape growers
this quality is connected to a price point and therefore compensation. Two important quality
parameters of red wine are the red colour and mouth feel of wine. Anthocyanin and tannins are
respectively connected to these two quality attributes and are both widely accepted as quality
indicators. Wine with high anthocyanin and tannin content often originates from grapes with a
high colour and phenolic profile. The existence of a correlation between grape and wine
anthocyanin and tannin content is therefore the basis of attempting to use these parameters in
the grape to predict end wine’s colour and phenolic quantity. Determination of anthocyanin and tannin content of grapes has already become part of some private owned wineries’ standard set
of determinations. However, sample preparations, extractions and consumables needed are all
factors that need to be reduced to make the measurement and therefore the use of these
parameters more viable in a co-operative cellar laboratory, where large volumes of grapes are
received during harvest.
The first objective of this work was to determine the levels of anthocyanin and tannin in red
grapes from different vineyard blocks from the producers of RW from three successive vintages.
This would give insight as to what can be seen as a low and high anthocyanin and tannin
content for grapes received at the cellar. For this purpose, blocks of the most important red
wine cultivars for RW was selected and analysed for these compounds. The ranges and
average levels of anthocyanin and tannin content were determined using measurement
techniques that could be used by any winery. The average mono flavanol and total colour level
of the grapes were found to be lower than those often reported in literature, with total grape flavanols being higher. However, a wide range of values for these compounds were found that
correlated with those found in other studies. The possible reasons for differences in levels of
occurrence of these compounds were discussed and mostly pertain to differences in cultivar,
micro climatic and season.
The second objective was to determine the correlation between levels of colour and phenolic
compounds in grapes and their corresponding wines. Such correlations will form the foundation
for the use of phenolic content to predict the colour and phenolic potential of the wine and
possibly wine quality as well. When the grape and wine colour and phenolic data were
correlated for all seasons and cultivars inclusive it was found that grape and wine colour
showed better correlations than for instance total phenols and tannins. This was especially true
for total colour pigments in red grapes, measured with HPLC, when correlated with certain
spectrophotometric analysis of wine colour. Cultivar and season as well as the synergism
between the two were further investigated for its role in affecting correlations. When these
relationships were further differentiated by season and by cultivar the resulting correlations
varied. This work contributed a great deal of information to support the use of grape colour and
phenolic compounds for the prediction of end wine colour and phenolic composition.
The third objective was to investigate near infrared spectroscopy (FT-NIR) as a viable option to
rapidly measured anthocyanins, tannins and total phenolics in red grapes. If proven
successfully, this could be employed by a large cellar such as RW. FT-NIR has been used with
success on grape extracts and in this instance the focus was to establish a calibration on the
grape homogenate itself. Preliminary results showed that FT-NIR could be applied for the use
of determination of anthocyanin and tannin levels in red grapes originating from RW. The prediction of total phenols was not found to be as accurate, but this could also be due to the
reference method that was used.
This work brought some interesting, practical information not only of importance for RW, but all
wineries that are concerned with improving the basis on which grape quality is determined. The
use of aerial data mapping for indicating areas regarding important grape colour and phenolic
parameters was used in this study and is a very visual way of showing the distribution of certain
ripeness parameters over a large area. Correlations between the grape and wines of such a
large amount of red grape blocks for a specific area have not also been reported in South Africa
before. The use of FT-NIR to determine anthocyanins and tannin concentrations in grape
homogenates is also novel for its use in South African wineries. This work may assist grape
and wine producers as well as analysts on the phenolic and colour profile of grapes and wines
from RW. / AFRIKAANSE OPSOMMING: Suid-Afrikaanse rooiwyn word wêreld-wyd geken aan ‘n dieprooi kleur en vol struktuur. Die
grootste rede vir hierdie verskynsel is hoë temperature wat ervaar word tydens rypwording en
veral na véraison. In die Robertson wynstreek is temperature egter tydens rypwording dikwels
vêr bo dit was as optimaal vir antosianien ontwikkeling beskou word. Die gepaste tyd om
druiwe te pluk word nie net gedryf deur die tegnologiese rypheidsvlak nie, maar ook deur
fenoliese rypheid. In ‘n koöperatiewe kelder omgewing soos Robertson Wynkelder (RW) word
‘n hoë lading druiwe elke dag ontvant vanaf verskillende produsente oor ‘n breë streek. Dit
maak dit moeilik om te bepaal watter druiwe werklik beide tegnologies en fenolies ryp is. Die
beste manier om hiervoor te vergoed is om ‘n standaard te stel vir ‘n reeks voorafbepaalde
parameters. Die vlakke van die gekose parameters is, word bepaal deur navorsinguitsette
sowel as die geskiedkunde data wat ingesamel is vanaf elkeen van die bepaalde blokke. Die
parameters wat tans in gebruik is by RW om oesdatum en kwaliteit by inname te bepaal is pH,
titreerbare suur (TA) en suiker vlak. Die tekortkoming hier is dat kwaliteit van druiwe beswaarlik
met slegs hierdie informasie kan bepaal word, maar dat dit die betaling van die produsent by
aflewering wesenlik kan beïnvloed. Dit het RW genoop om in samewerking met die
Departement van Wingerd en Wynkunde, Universiteit van Stellenbosch nog parameters te
ondersoek wat hierdie rypheid- en kwaliteitsbepaling by inname sou kon versterk. Twee
belangrike faktore wat kwaliteit van rooiwyn bepaal is die kleur en struktuur. Antosianiene en
tanniene is onderskeidelik verantwoordelik vir hierdie kwaliteits eienskappe van wyn. Wyn wat
bestempel word as hoog in kleur en tannien inhoud word dikwels verbind met druiwe wat hoog
is in hierdie faktore. Die moontlike korrelasie tussen die antosianien en tannien inhoud van
druiwe en die wyn wat daarvan berei word is dus die basis waarop die potensiële toepassing
van hierdie parameters berus. Die bepaling van antosianien en tannien vlakke word reeds in sommige laboratoriums gedoen. Die monster voorbereidings tyd, ekstraksies, toerusting en
verbruikbare items nodig om hierdie tipe analieses te doen is egter hoog. Die analiese van
hierdie komponente is meer lewensvatbaar in groot laboratoriums (soos in ‘n koöperatiewe
kelder) waar groter volume druiwe ingeneem word gedurende parstyd.
Die eerste doelwit van hierdie studie was om te bepaal teen watter vlakke antosianiene en
tanniene in druiwe voorkom, spesifiek van die Robertson area. Die het behels ‘n wye
verskeidenheid van blokke, verspreid oor die hele streek wat oor 3 seisoene gemonitor is in
terme van veral kleur en tanniene maar ook ander belangrike parameters. Die idee hier is om
insig te kry rakende watter vlakke bestempel kan word as laag en hoog in terme van
antosianien en tanniene vir die Robertson streek. Daarvoor is slegs die mees aangeplantste
rooi kultivars gebruik. Die verspreiding en gemiddelde vlakke waarteen antosianien en tanniene
voorkom was bepaal deur gebruik te maak van metodes wat as relatief algemeen in laboratoria
gebruik word. Die gemiddelde mono-flavonoïed en totale kleur pigment inhoud van die druiwe was laer as van die vlakke wat in die literatuur beskikbaar is, met totale flavanole wat hoër was.
Die wyer verspreiding van die waardes het egter beter gekorreleer met die waardes soos
beskryf in die literatuur. Die moontlike redes vir die verskillende vlakke word in die studie
bespreek en word waarskynlik bepaal deur verskille in kultivar, mikro-klimaat en seisoen.
Die tweede doelwit was om te bepaal of daar ‘n korrelasie te vinde is tussen die kleur en
tannien inhoud van die druiwe en ooreenstemmende wyne. Sulke tipe korrelasies sal die basis
vorm om antosianien en tannien inhoud van wyn reeds in die druiwe fase te kan voorspel.
Nadat die ingesamelde druif en wyn data as ‘n geheel beskou was, was dit sigbaar dat die
wynkleur parameters beter korrelasies bied as meeste tannien en totale fenole. Dit was veral
waar in die geval van totale kleur pigmente soos gemeet met die HPLC teenoor die wynkleur
parameters gemeet met spektrofotometriese metodes. Verdere ondersoeke in terme van die
impak wat die kultivar en seisoenale kan hê het tot variërende korrelasies gelei.. Hierdie werk
het ‘n groot bydrae gelewer om voorspellings van wyn kleur en fenoliese inhoud reeds met
sukses vanaf die druif te bepaal.
Derdens het die werk fourier transformasie naby infrarooi skandering (FT-NIR) ondersoek as ‘n
lewensvatbare metode vir die bepaling van antosianien, tannien en totale fenoliese inhoud van
druiwe en wyn. FT-NIR word reeds oor ‘n wye reeks wyne en druiwe ekstraksiemonsters
toegepas en die doelwit hier was om druiwe homogenaat as matriks te kalibreer. Voorlopige
resultate het bevind dat antosianien en tannien vlakke in druiwe van RW gemeet kan word met
die FT-NIR, maar dat die kalibrasie vir totale fenole nog verbeter kan word. Hierdie werk het ‘n wye reeks interessante en prakties bruikbare informasie na vore gebring wat
van onskatbare belang is vir RW en ander kelders wat besorgd is oor die verbetering van
algemene druifkwaliteit. Geografiese kaarte wat belangrike druifkleur en fenoliese parameters
aandui is in hierdie studie gebruik en wys hoe data visueel voorgestel kan word om die
geheelindruk van gekose parameters oor ‘n groot area te vergelyk. Korrelasies tussen druiwe
en wyn van so ‘n groot hoeveelheid druiwe blokke is nog nooit voorheen in Suid-Afrika getoon
nie. Dieselfde geld vir die gebruik van FT-NIR vir die meet van kleur en fenoliese parameters in
druiwe homogenate. Hierdie werk kan druiwe- en wynproduseerders sowel as analiste
assisteer in terme van die kleur en fenoliese profiel van druiwe en wyn van RW. / Robertson Winery with Mr Bowen Botha as well as THRIP for funding this project
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Analysis of endo-polygalacturonase activity in a recombinant yeast containing a reconstituted PGU1 geneVan Wyk, Herine 03 1900 (has links)
Thesis (MSc (Wine Biotechnology))--University of Stellenbosch, 2009. / The PGU1 gene encodes an endo-polygalacturonase, an enzyme that degrades pectin. Although the presence and function of this gene is well characterized in Saccharomyces cerevisiae, its regulation is very complex and not yet fully understood. Yeast producing a highly active polygalacturonase (PG) during alcoholic fermentation could potentially improve filtration and turbidity and also enhance extraction of certain aroma compounds. This could replace the addition of expensive commercial enzyme preparations that often contain unwanted enzymes.
The first objective of this study was to evaluate PGU1 expression in recombinant strains of S. cerevisiae that originally lacked the PGU1 gene. A functional PGU1 gene and its promoter were successfully re-introduced into their native position in the genomes of five wine strains. Three of these strains recovered PG activity while two did not transcribe the gene and subsequently lacked activity. The three strains that recovered activity were used in microvinification experiments to determine the effect of PG-producing yeast on the aroma profile of the wine. No significant differences were observed in the volatile compounds production between the recombinants and their respective wild types, but some tendencies arose, especially for the monoterpene geraniol.
The second objective of this study was to analyze the PGU1 gene and promoter from Saccharomyces paradoxus RO88 (a strain that exhibits high PG activity) and to compare it to those of S. cerevisiae S288C in order to identify differences that could potentially be responsible for the difference in their PG activities. Comparison of the gene sequences revealed several amino acid differences, one of which was in the peptide secretion signal. Analyses of the promoters also indicated some potentially important differences. Furthermore, S. cerevisiae strain VIN13, RO88 as well as two interspecies hybrids (all displaying varying PG activities) were compared under winemaking conditions. Clear differences were observed for the production of certain compounds. RO88 and the hybrids produced higher concentrations of certain volatile compounds, although they were not strong fermenters. Two recombinants, each containing a PGU1-overexpressing plasmid (one with the PGU1 gene from S. paradoxus and the other from S. cerevisiae), were also used in vinification to determine the effects of the different PGU1 gene on the aroma profile of the wine. Unfortunately, the plasmids were unstable and lost during the fermentation. Nevertheless, some tendencies were observed that indicated possible higher production of certain compounds by the recombinants compared to their wild types.
This study identified that regulation of the PGU1 gene differs between strains with different genetic backgrounds. Certain differences were observed in the PGU1 gene and promoter
sequences between S. cerevisiae and S. paradoxus that could potentially be the reason for the difference in their PG activities. From an oenological point of view, the presence of PGU1 in the genome of a fermenting strain tends to increase the aromatic potential of wine. These results provide a good platform for further studies on the PGU1 gene.
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