The Importance of a Comparative Characterization of Saccharomyces Cerevisiae and Saccharomyces Pastorianus Strains for Brewing

The volume and market share loss for classical beer types such as pils beer and wheat beer has been declining for several years, but the overall beer market remains almost unchanged as a result of the increasing interest in beer specialties Due to high biodiversity, the diversity of the strains, and the different flavor profiles, reliable and practical information regarding the characteristics of individual brewing strains is required to help brewers to find the right strain for their brewing purposes. This paper presents a comparison of 10 commercially available Technical University of Munich (TUM) brewing yeast strains. The strains were screened for genetic and phenotypic characteristics. After confirming the genetic distinctiveness by using species-specific real-time polymerase chain reaction (RT-PCR) systems and a strain typing method based on PCR-capillary electrophoresis of the partial intergenic spacer 2 (IGS2) fragment (IGS2-314 PCR-capillary electrophoresis), the strains were tested regarding phenotypic characteristics under controlled and identical fermentation conditions in small-scale brewing trials. Besides the fermentation performance, flocculation behavior, sugar metabolism and other phenotypic characteristics, the main focus was on the flavor and aroma profile of each investigated TUM yeast strain.


Introduction
The Bavarian purity law of 1516 only permits barley, hops and water to be used to produce beer [1].In 1993, the purity law was further clarified by the German "vorläufiges Biergesetz" (German preliminary beer law) and expanded in accordance with public perception that beer can only be produced using malt, hops and water.Even 477 years after the Bavarian purity law, there is still a lack of attention devoted to yeast as a raw brewing ingredient.Nowadays there is an increasing focus on yeast.MEIER-DÖRNBERG describes yeast as the flavor engine of the brewing industry [2,3].Yeast metabolism during the fermentation and ripening process gives rise to approximately 80% of all aroma-active compounds in beer, thereby determining its aroma profile [4].There are more than 300 different volatile and non-volatile fermentation by-products, which vary in their concentration from strain to strain.According to WHITE and ZAINASHEFF, brewer's yeast alone is able to produce about 500 different flavor and aroma compounds [5].Yeast strains are as diverse as the resulting flavors, and the choice of yeast strain is therefore directly linked to the individual and special flavors created when developing new beer types and styles.
To date, approximately 1,500 yeast species have been reported [6].The most important yeast species for fermentation technology belong to the Saccharomyces genus and are taxonomically grouped in the Saccharomyces sensu stricto complex [7,8].The Saccharomyces sensu stricto complex consists of Saccharomyces cerevisiae-the yeast used to produce top-fermented beers (often referred to as "ale"), wine, distillers' mash, sake and many other alcoholic beverages, Saccharomyces bayanus-used in wine, cider, cidre and apple wine production, and Saccharomyces pastorianus-the starter culture for bottom-fermented beer (lager) and apple wine production, as well as additional species (S. cariocanus, S. jurei, S. kudriavzevii, S. mikatae, S. paradoxus, S. arboricolus and S. eubayanus) which are not used industrially [7,[9][10][11][12][13].LIBKIND et al. published that the bottom-fermenting strains of the species Saccharomyces pastorianus used in the lager beer production are genetic hybrids of Saccharomyces cerevisiae and the Patagonian wild yeast Saccharomyces eubayanus [12].DUNN and SHERLOCK claimed that there were at least two hybridization events and that all Saccharomyces pastorianus lager strains consist of at least two types [14].The S. pastorianus strains they studied were divided into the groups Saaz and Frohberg.Some industrial strains exhibiting strong fermentation performance belong to the Frohberg group.PERES-TRAVEZ et al. investigated that S. bayanus strains are also hybrids, whereas the parental species are of an European linage of S. eubayanus-like strains and S. bayanus var.uvarum (S. uvarum) [15].Rapid species identification within the Saccharomyces sensu stricto group plays a key role in verifying the purity of a species in a beer starter culture, and for detecting cross contamination.Some special beer styles also use non-Saccharomyces yeast species as starter cultures.Schizosaccharomyces pombe is found in some traditional African beers, and Dekkera bruxellensis in Belgian beers and in German Berliner Weiße.Saccharomycodes ludwigii is used to produce low-alcohol and non-alcoholic beer styles, while in the production of top-fermented wheat beer, Torulaspora delbrueckii can be used as a supplemental yeast strain to create a distinctive fruity aroma [16][17][18].Spontaneous beer fermentation may utilize other non-Saccharomyces species such as Debaryomyces spp., Meyerozyma guilliermondii, Pichia membranifaciens, Candida friedrichii, Naumovia castellii, Dekkera anomala, and Priceomyces spp. in lambic beer [19], and Cryptococcus keutzingii, Rhodotorula mucilaginosa, Candida krusei, Pichia fermentans, and Pichia opuntiae in American coolship ale [20].
A brewing yeast strain should be taxonomically classified at the species and strain level using molecular biological methods.It should also be characterized in terms of its propagation and fermentation performance as well as its aroma profile.The Frisinga-TUM 34/70 ® strain is one of the most abundant lager yeast strains in the brewing industry, and is the reference lager strain when comparing the fermentation performance and final pure beer flavor of other lager strains.The genome of Frisinga-TUM 34/70 ® was also the first of the bottom-fermenting strains to be sequenced and published [21].A study conducted by MÜLLER-AUFFERMANN used the characteristics of TUM 34/70 as a reference to develop a method to rapidly compare the performance of lager yeast strains [22].MEIER-DÖRNBERG further optimized small-scale fermentation vessels used to conduct these trials, as well as the fermentation to make it possible to directly compare the investigated yeast strains [23].These kinds of trials are very useful for breweries wishing to either replace their yeast strain or to introduce a second one to develop specialty beers with specific properties or to modify or improve existing beer styles.
The market share for such beer specialties is steadily increasing.The craft beer movement and the continuing interest in the variety of flavors mean that regional brewers in particular are benefiting from their willingness to experiment with a variety of different yeast strains.While the volume and market share loss of classical beer types such as pils beer and wheat beer has been declining for several years in Germany, the overall beer market remains practically the same [24].The greater diversity of yeast that can be applied in brewing, along with an improved understanding of yeasts' evolutionary history and biology, is expected have a significant and direct impact on the brewing industry, with potential for improved brewing efficiency, product diversity and, above all, customer satisfaction [25].A lot of specialty beers with distinctive flavors are appearing on the market, especially for beers fermented with top-fermenting Saccharomyces cerevisiae strains.These strains produce intense flavors, and they are the focus of many craft-and microbreweries.They include Bavarian wheat beer, ales and Belgian specialty beers.The broad biodiversity and availability of different strains of Saccharomyces cerevisiae offer brewers a wealth of possibilities to create beers with unique attributes and flavor profiles.Descriptions of these top-fermenting specialty yeast strains are therefore of considerable importance when selecting suitable strains in the development of special products.The Bavarian wheat beer strain Saccharomyces cerevisiae LeoBavaricus-TUM 68 ® is a perfect example of a successful specialist yeast strain.It is phenolic-off-flavor (POF)-positive.Depending on the production process, Bavarian wheat beers can exhibit very strong fruity, clove like, estery flavors or a more neutral, yeasty, top-fermented character with a decent fruity note, or they can fall somewhere in between the two.The finished beer aroma is determined in part by the strain and how it is handled as well as by the process parameters.SCHNEIDERBANGER recently described the impact of the different wheat beer yeast strains on fermentation performance, and their respective aroma profiles [26].SCHNEIDERBANGER et al. found that the Bavarian wheat beer strain LunaBavaria-TUM 127 ® used to ferment the first batch does not ferment maltotriose.This produces a different mouthfeel and aroma to wheat beer strains without this maltotriose gap [27].Very different sensory impressions can be achieved by using other top-fermenting yeasts, as MEIER-DÖRNBERG recently showed.By investigating five different ale yeast isolates under the same fermentation and substrate conditions, entirely different and often surprising flavors could be identified in the finished beers.One yeast strain created citrus and fruity beer notes, whereas a second produced more floral flavors [23].Describing both existing and new brewing yeast strains will help us understand their characteristics, and will pave the way for innovative brewers around the world to experiment and create novel products for the beer market.There is a more or less infinite potential for increasing biodiversity among brewing yeast strains.

Materials and Methods
The following methods were performed according to [23].

Yeast Isolates and Strains
A total of ten culture yeast strains were obtained in agar slants from the Yeast Center of the Research Center Weihenstephan for Brewing and Food Quality (BLQ) of the Technical University of Munich (TUM).These ten culture yeast strains included two bottom-fermenting Saccharomyces pastorianus and eight top-fermenting Saccharomyces cerevisiae brewing yeast strains commonly used to produce beer styles dependent on the industrial applications listed in the following Table 1.

Genetic Identification and Strain Determination
To confirm the genetic distinctiveness of each obtained TUM brewing yeast strain, a real-time polymerase chain reaction (RT-PCR) and a strain typing method based on a PCR-capillary electrophoresis of partial intergenic spacer 2 (IGS2) fragment (IGS2-314 PCR-capillary electrophoresis) were used according to HUTZLER [28,29].The RT-PCR was used in each case to identify the species the strain belonged to, and IGS2-314 PCR-capillary electrophoresis was used to confirm that the investigated yeast cultures of the same species represent different strains.

Phenolic Off-Flavor Test
TUM yeast culture strains were taken from wort agar slopes and spread on a yeasts and mold agar plate (YM-agar) containing one of the following precursors: ferulic acid, cinnamic acid and coumaric acid.After three days of incubation at 24 • C, the three single agar plates per yeast isolate were evaluated by sniffing to detect any of the following aromas: ferulic acid becomes 4-vinylguajacol (4-VG, clove-like), cinnamic acid becomes 4-vinylstyrene (4-VS, styrofoam-like) and coumaric acid becomes 4-vinylphenol (4-VP, medicinal-like).
For the YM-agar plates a YM-media was prepared by adding distilled water to 3.0 g malt extract, 3.0 g yeast extract, 5.0 g peptone, 11.0 g glucose monohydrate, and 20.0 g agar to 1000 mL, and autoclaved.After autoclaving, an aliquot of the following stock solutions was added to the YM-media at 45-50 • C under sterile conditions.For the stock solution of coumaric acid, 100 mg of the instant were dissolved in 10 mL of 96% (v/v) ethanol.The stock solution of ferulic and cinnamic acid was made by dissolving 1 g in 20 mL of 96% (v/v) ethanol.10 mL coumaric acid, 2 mL ferulic acid or 2 mL cinnamic acid stock solution was added for 1000 mL YM-media.

Wort
The wort characteristics used for propagation and the brewing trials are shown in Table 4.The wort was based on hopped barley malt concentrate (N53940; Döhler GmbH, Darmstadt, Germany).To achieve an original gravity of 12.4 • P, wort concentrate was diluted with distilled water and boiled for 5 min to guarantee sterile conditions.The same wort batch preparation was used for the propagation and brewing trials to ensure constant wort composition.Free alpha-amino nitrogen was quantified using the MEBAK II.2.8.4.1 method.Sugar composition was determined using the HPLC MEBAK II.3.2.2.1.2method.In order to propagate yeasts, yeast strains were inoculated from agar slants (yeast pure culture) into 60 mL of sterile wort medium in an 100 mL Erlenmeyer flask and incubated for 72 h at ambient temperature (20 • C) and pressure, then agitated at 80 rpm using a WiseShake 207 orbital shaker (Witeg Labortechnik GmbH, Wertheim, Germany).After incubation, yeasts were transferred to 4 kg of sterile wort medium and further propagated at the same conditions for an additional 72 hours.After allowing six hours for sedimentation, the supernatant was decanted and 2 kg of sterile wort medium at pitching temperature (20 • C) was added to the yeast sediment in each container.The yeast concentration was determined in terms of cells/g using a Thoma cell counting chamber with a chamber depth of 0.1 mm and an area of 0.00025 m 3 per square (Brand GmbH&Co.KG, Wertheim, Germany).

Fermentation
Laboratory-scale brewing trials were performed using stainless steel vessels with dimensions of 10 cm diameter x 33 cm height (2.5 liters) with 20% headspace and clamped down lids, according to MEIER-DÖRNBERG [23].The vessels were placed in a tempered cooling chamber (2023 Minicoldlab, LKB-Produkter AB, Bromma, Sweden) to guarantee a constant fermentation temperature.To imitate industrial brewery conditions during fermentation, a head pressure of 0.5 bar was applied to simulate a liquid height of 10 m (median hydrostatic pressure).Brewing trials were evaluated by pitching 8.5 L wort per yeast strain.Each batch was then divided into four fermentation vessels.By having four vessels, samples could be taken daily from one of the four vessels to estimate the specific gravity, cells in suspension and pH, while the other three vessels remained undisturbed.Yeast strains were added at an inoculation rate of 15 million cells/g of homogeneous mixed wort medium for the top-fermenting Saccharomyces cerevisiae yeast strains (LeoBavaricus-TUM 68 ® , LunaBavaria-TUM 127 ® , Colonia-TUM 177 ® , Vetus-TUM 184 ® , Mel-TUM 211 ® , Monacus-TUM 381 ® , Tropicus-TUM 506 ® , and Harmonia-TUM 511 ® ) and an inoculation rate of 30 million cells/g of homogeneous mixed wort medium for bottom-fermenting Saccharomyces pastorianus yeast strains (Frisinga-TUM 34/70 ® and Securitas-TUM 193 ® ).The wort was not oxygenated.Primary fermentation was maintained at 20 • C for the top-fermenting and 15 • C for the bottom fermenting TUM yeast strains.Fermentation was considered complete once the specific gravity remained constant for two consecutive days.An additional five days for maturation was given following primary fermentation at the same fermentation temperature, and seven days for lagering at 0 • C. The beers were then removed from the fermentation vessels, homogenized, and collected in sterile bottles.The specific gravity and pH of the samples were determined from the filtered fermentation samples using a DMA 35N (Anton-Paar GmbH, Graz, Austria) for specific gravity and a pH3210 (WZW, Wissenschaftlich-Technische Werkstätten GmbH, Weilheim, Germany) for pH measurement.The samples were filtered using Whatman ® folded filter paper with a diameter of 320 mm (GE Healthcare Europe GmbH, Freiburg, Germany).

Determining the Cell Count (Cells in Suspension and Total Cell Count)
Cell counts for pitched yeast, cells in suspension until lagering, and total cell count after lagering were determined using a Thoma cell counting chamber with a chamber depth of 0.1 mm and an area of 0.00025 m 3 per square (Brand GmbH&Co.KG, Wertheim, Germany).Cells in suspension were analyzed every 24 h up to the start of lagering.To ensure cell count accuracy during fermentation and maturation, 20 mL of green beer was removed from the middle of the fermentation vessel by using a 10 mL volumetric pipette mounted on a stand.Prior to sampling, the head pressure in the vessel was released very slowly so that the cells in suspension were not affected by a pressure surge.The total cell count was determined after the lagering phase.Beers were removed from the fermentation vessels, and the decanted yeast masses were collected by suspending the yeast cells in a total of 50 g distilled water.The yeast cells were washed by centrifugation twice with 50 g distilled H 2 O (5 min at 3000 rpm) and resuspended with distilled water up to a total of 100 g.Afterwards, distilled water was added to 1 g of the homogenous yeast suspension to make up to 100 mL.Total cell counts were determined in cells/g using the Thoma cell counting chamber.

Sensory Evaluation
Three single sensory tests were conducted which included: expected beer type test, DLG-scheme for beer (Deutsche Landwirtschafts-Gesellschaft) and a descriptive sensory evaluation.All beer samples were tasted and evaluated by a sensory panel of seven DLG-certified tasters with long-standing experience in the sensory analysis of beer at the Weihenstephan Research Center for Brewing and Food Quality.Accredited sensory evaluations were performed according to DIN EN 17025.Sensory evaluations were performed in individual walled tasting stations under controlled environmental conditions.Samples were provided in triplicate sets for all beers in dark glasses, each with a three digit code.All samples were served at 12 • C to guarantee optimal conditions to investigate the predominant flavor diversity.At first the panelists associated the beer samples with their expected beer type (e.g., ale, wheat-, Kölsch-, Alt-, stout, Berliner Weisse, porter-, lager-; Bock-; Märzen-, Rauch-, Schwarz-, Dunkles-, malt beer) followed by an examination of the beer samples according to the DLG-scheme.Secondly, a descriptive sensory evaluation was conducted during which trained panelists described specific flavors.Seven main categories were described (e.g., sweet, tropical fruity, fruity (other fruits), citrus, spicy, floral and other flavors).Every category was evaluated from 0, meaning not noticeable, to 5, extremely noticeable.

Real-Time PCR Assays and IGS2-314 PCR-Capillary Electrophoresis
RT-PCR results confirmed the species identity of the investigated TUM yeast strains of the TUM Yeast Center.In addition, the results of the DNA fingerprinting showed unique banding patterns, also confirming that each yeast represents a genetically different strain (Figure 1).Table 5 shows that the tested RT-PCR systems and the obtained results for all strains.All yeast strains were positive for the Sc-GRC3 and Sce loci.The RT-PCR systems Sc-GRC3 and Sce have positive signals when S. cerevisiae DNA is measured or the DNA of hybrid strains that contain these DNA loci.The top-fermenting yeast strains LeoBavaricus-TUM 68 ® , LunaBavaria-TUM 127 ® , Colonia-TUM 177 ® , Vetus-TUM 184 ® , Mel-TUM 211 ® , Monacus-TUM 381 ® , Tropicus-TUM 506 ® and Harmonia-TUM 511 ® were also positive for the TF-COXII locus, suggesting that they belong to the S. cerevisiae strains.The bottom-fermenting yeast strains Frisinga-TUM 34/70 ® and Securitas-TUM 193 ® were also positive for loci that correlate with the PCR systems Sbp, BF-LRE1 and BF-300, which detect S. bayanus/S.pastorianus strains.In addition, all investigated TUM yeast strains were negative for the RT-PCR system Sdia which detects S. cerevisiae var.diastaticus strains.

Sugar Utilization
As Table 6 shows, not all of the strains were able to metabolize all major wort sugars (e.g., glucose, fructose, sucrose, maltose, maltotriose).Maltotriose could not be utilized by all strains.The top-fermenting yeast strain LunaBavaria-TUM 127 ® could not ferment maltotriose (1.05%), while the culture yeast strains Mel-TUM 211 ® , Tropicus-TUM 506 ® and Vetus-TUM 184 ® only fermented a small amount of maltotriose (26.66%, 59.28% and 60.92%).Variations in the maltotriose utilization for all other strains were above 83%.The results suggested that the utilization degree as well as the ability to utilize maltotriose is strain dependent.

Amino Acid Utilization
The mean amino acid uptake in the finished beers after lagering using the investigated S. pastorianus and S. cerevisiae yeast strains is shown in Supplementary Material Tables S1 and S2.The commonly accepted amino acid uptake classification is indicated with shading according to JONES and PIERCE [22,23,35,36].
As shown in Tables S1 and S2, the total amino acid utilization followed no defined process and was different for each of the investigated TUM yeast strains.As MEIER-DÖRNBERG previously described using five tested S. cerevisiae ale yeast strains, the exact course of absorption and the sequence varies, even if specific amino acids were preferred by the yeast [23].However, in contrast to the tested top-fermenting S. cerevisiae ale yeast strains, the bottom-fermenting S. pastorianus strains metabolized the single amino acids in a similar order.This might depend on the same industrial application (lager and export beer production) for which both strains were commonly used.Fermentation conditions are similar between lager and export beer production, and the Frisinga-TUM 34/70 ® and Securitas-TUM 193 ® strains may adapt to the same circumstances and react with similar cell metabolisms, even if they are genetically different and show unique sensory profiles.Figures 2 and 3 show the free amino nitrogen (FAN) and the total amino acid (AS) utilization of each yeast strain in comparison with the corresponding residual contents.The utilization rate of FAN and AS was correlated for the same yeast strain, but different across strains.The mean amino acid uptake in the finished beers after lagering using the investigated S. pastorianus and S. cerevisiae yeast strains is shown in Supplementary Material Tables S1 and S2.The commonly accepted amino acid uptake classification is indicated with shading according to JONES and PIERCE [23,24,35,36].
As shown in Tables S1 and S2, the total amino acid utilization followed no defined process and was different for each of the investigated TUM yeast strains.As MEIER-DÖRNBERG previously described using five tested S. cerevisiae ale yeast strains, the exact course of absorption and the sequence varies, even if specific amino acids were preferred by the yeast [24].However, in contrast to the tested top-fermenting S. cerevisiae ale yeast strains, the bottom-fermenting S. pastorianus strains metabolized the single amino acids in a similar order.This might depend on the same industrial application (lager and export beer production) for which both strains were commonly used.Fermentation conditions are similar between lager and export beer production, and the Frisinga-TUM 34/70 ® and Securitas-TUM 193 ® strains may adapt to the same circumstances and react with similar cell metabolisms, even if they are genetically different and show unique sensory profiles.Figures 2 and 3 show the free amino nitrogen (FAN) and the total amino acid (AS) utilization of each yeast strain in comparison with the corresponding residual contents.The utilization rate of FAN and AS was correlated for the same yeast strain, but different across strains.

Fermentation Kinetics
Figure 4 shows the drop in specific gravity during fermentation by the investigated yeast strains.As shown in Figure 4, LeoBavaricus-TUM 68 ® has the quickest drop in specific gravity, followed by Colonia-TUM 177 ® .Both strains reached their final gravity after 96 hours of fermentation.Monacus-TUM 381 ® needed 72 hours more to reach the final gravity of 1.8 °P after 168 hours.Mel-TUM 211 ® fermented the wort slower than the other strains but did so continuously until it reached the lowest apparent attenuation of all investigated yeast strains at 66.13% after 216 hours of fermentation.
Table 7 shows the apparent attenuation compared with the fermentation time required by the isolated strains.The different fermentation rates and degrees of apparent attenuation are due to their ability to ferment maltose and maltotriose (see Table 6).LeoBavaricus-TUM 68 ® and Monacus-TUM 381 ® reached the attenuation limit of the wort used at an apparent attenuation of 86.17%.The attenuation limit was previously tested according to MEBAK Bd.II and was achieved by using the top-fermenting Saccharomyces cerevisiae brewing yeast strain LeoBavaricus-TUM 68 ® and the same wort used in this trial.The low apparent attenuation of 76.2% by LunaBavaria-TUM 127 ® was due to the unique strain property of not fermenting one of the major wort sugars, namely maltotriose.The low drop in specific gravity over 144 h was not due to the maltotriose gap in the strain specific sugar metabolism, because maltotriose was taken up by the yeast cell as the last wort sugar, and was therefore not necessary for sufficient cell growth.

Fermentation Kinetics
Figure 4 shows the drop in specific gravity during fermentation by the investigated yeast strains.As shown in Figure 4, LeoBavaricus-TUM 68 ® has the quickest drop in specific gravity, followed by Colonia-TUM 177 ® .Both strains reached their final gravity after 96 hours of fermentation.Monacus-TUM 381 ® needed 72 hours more to reach the final gravity of 1.8 • P after 168 hours.Mel-TUM 211 ® fermented the wort slower than the other strains but did so continuously until it reached the lowest apparent attenuation of all investigated yeast strains at 66.13% after 216 hours of fermentation.
Table 7 shows the apparent attenuation compared with the fermentation time required by the isolated strains.The different fermentation rates and degrees of apparent attenuation are due to their ability to ferment maltose and maltotriose (see Table 6).LeoBavaricus-TUM 68 ® and Monacus-TUM 381 ® reached the attenuation limit of the wort used at an apparent attenuation of 86.17%.The attenuation limit was previously tested according to MEBAK Bd.II and was achieved by using the top-fermenting Saccharomyces cerevisiae brewing yeast strain LeoBavaricus-TUM 68 ® and the same wort used in this trial.The low apparent attenuation of 76.2% by LunaBavaria-TUM 127 ® was due to the unique strain property of not fermenting one of the major wort sugars, namely maltotriose.The low drop in specific gravity over 144 h was not due to the maltotriose gap in the strain specific sugar metabolism, because maltotriose was taken up by the yeast cell as the last wort sugar, and was therefore not necessary for sufficient cell growth.The flocculation behavior of a yeast strain is an important selection criterion to ensure reliable product quality in industrial brewing processes.Besides the genetic background of the yeast strain (e.g., variation in FLO genes), the flocculation behavior is affected by the physiological environment (e.g., the pH and availability of metal ions and nutrients of the wort), by the physical environment (e.g., soluble oxygen, hydrodynamic conditions and low agitation), and the fermentation temperature, as well as a sufficient concentration of yeast cells in suspension [37][38][39].In this research,  The flocculation behavior of a yeast strain is an important selection criterion to ensure reliable product quality in industrial brewing processes.Besides the genetic background of the yeast strain (e.g., variation in FLO genes), the flocculation behavior is affected by the physiological environment (e.g., the pH and availability of metal ions and nutrients of the wort), by the physical environment (e.g., soluble oxygen, hydrodynamic conditions and low agitation), and the fermentation temperature, as well as a sufficient concentration of yeast cells in suspension [37][38][39].In this research, all environmental and fermentation conditions were kept constant, in order to investigate and classify the investigated strains according to their specific flocculation behavior in flocculent and non-flocculent ("powdery") yeast strains (see Table 8).According to ANNEMÜLLER, a flocculent yeast strain accumulates to flocs and settles at the bottom of the fermentation vessel when the nutrients present in brewers wort are largely consumed [40].

Apparent attenuation (AA %) of the final beer
As Figure 5 shows, in contrast to the eight top-fermenting TUM yeast strains, the bottom-fermenting yeast strains Frisinga-TUM 34/70 ® and Securitas-TUM 193 ® flocculated very rapidly in the first three days of the main fermentation and reached a concentration of cells in suspension below the pitching rate.By reaching their apparent attenuation both strains shows cell concentrations below two million yeast cells/mL (e.g., 1.8 and 1.6 million cells/mL), and could therefore be classified according to their flocculation behavior as flocculent yeast strains (see Table 8).With the exception of the LunaBavaria-TUM 127 ® and Vetus-TUM 184 ® yeast strains, the top-fermenting TUM yeast strains LeoBavaricus-TUM 68 ® , Colonia-TUM 177 ® , Mel-TUM 211 ® , Monacus-TUM 381 ® , Tropicus-TUM 506 ® and Harmonia-TUM 511 ® were largely dispersed and remained in a suspension that is close to the pitching concentration, even once they have reached their apparent attenuation.According to BÜHLINGEN et al., the strains exhibited a non-flocculent ("powdery") behavior [41].In contrast, LunaBavaria-TUM 127 ® and Vetus-TUM 184 ® showed similar flocculation behavior to the bottom-fermenting yeast strains and flocculated below four million cells/mL (e.g., 3.5 and 0.5 million cells/mL) by reaching their apparent attenuations.LeoBavaricus-TUM 68 ® also showed noticeable flocculation behavior, but also had the greatest increase in the number of cells, so that, similarly to Colonia-TUM 177 ® , the concentration of cells in suspension at the time of apparent attenuation was still above the pitching concentration.The flocculation behavior of both strains was therefore classified as powdery, but showed rapid flocculation, with a final concentration of cells in suspension below one million cells/mL at the end of maturation.With the exception of Mel-TUM 211 ® and Tropicus-TUM 506 ® , the "powdery" yeast strains fermented beer faster than the "flocculent" yeast strains, but both resulted in similar final attenuations.all environmental and fermentation conditions were kept constant, in order to investigate and classify the investigated strains according to their specific flocculation behavior in flocculent and nonflocculent ("powdery") yeast strains (see Table 8).According to ANNEMÜLLER, a flocculent yeast strain accumulates to flocs and settles at the bottom of the fermentation vessel when the nutrients present in brewers wort are largely consumed [40].
As Figure 5 shows, in contrast to the eight top-fermenting TUM yeast strains, the bottomfermenting yeast strains Frisinga-TUM 34/70 ® and Securitas-TUM 193 ® flocculated very rapidly in the first three days of the main fermentation and reached a concentration of cells in suspension below the pitching rate.By reaching their apparent attenuation both strains shows cell concentrations below two million yeast cells/mL (e.g., 1.8 and 1.6 million cells/mL), and could therefore be classified according to their flocculation behavior as flocculent yeast strains (see Table 8).With the exception of the LunaBavaria-TUM 127 ® and Vetus-TUM 184 ® yeast strains, the top-fermenting TUM yeast strains LeoBavaricus-TUM 68 ® , Colonia-TUM 177 ® , Mel-TUM 211 ® , Monacus-TUM 381 ® , Tropicus-TUM 506 ® and Harmonia-TUM 511 ® were largely dispersed and remained in a suspension that is close to the pitching concentration, even once they have reached their apparent attenuation.According to BÜHLINGEN et al., the strains exhibited a non-flocculent ("powdery") behavior [41].In contrast, LunaBavaria-TUM 127 ® and Vetus-TUM 184 ® showed similar flocculation behavior to the bottom-fermenting yeast strains and flocculated below four million cells/mL (e.g., 3.5 and 0.5 million cells/mL) by reaching their apparent attenuations.LeoBavaricus-TUM 68 ® also showed noticeable flocculation behavior, but also had the greatest increase in the number of cells, so that, similarly to Colonia-TUM 177 ® , the concentration of cells in suspension at the time of apparent attenuation was still above the pitching concentration.The flocculation behavior of both strains was therefore classified as powdery, but showed rapid flocculation, with a final concentration of cells in suspension below one million cells/mL at the end of maturation.With the exception of Mel-TUM 211 ® and Tropicus-TUM 506 ® , the "powdery" yeast strains fermented beer faster than the "flocculent" yeast strains, but both resulted in similar final attenuations.

Change in pH Value
Table 9 shows the drop in pH during the first 96 hours of primary fermentation, the pH value after the maturation phase, and the average pH value of the final beer.As shown in Table 9, the drop in pH and the time taken to reach the minimum pH value for primary fermentation is different for all the investigated yeast strains.
Securitas-TUM 193 ® , Monacus-TUM 381 ® and Mel-TUM 211 ® reached their minimum and final beer pH value after 48 hours.Frisinga-TUM 34/70 ® showed a similar change in pH value to the ale yeast strains Mel-TUM 211 ® , Tropicus-TUM 506 ® and Harmonia-TUM 511 ® , which was already shown by MEIER-DÖRNBERG [23].These four strains reached their minimum pH value for primary fermentation after 48 hours, and recorded a pH value increase of 0.1 after the maturation and lagering phase.LeoBavaricus-TUM 68 ® , LunaBavaria-TUM 127 ® , Colonia-TUM 177 ® and Vetus-TUM 184 ® needed 96 hours to reach their minimum pH value for primary fermentation.Colonia-TUM 177 ® recorded a pH value increase of 0.1 as measured in triplicate in the final beer, while an increase of 0.2 could be registered in the produced beers with LeoBavaricus-TUM 68 ® and LunaBavaria-TUM 127 ® .According to ANNEMÜLLER and MANGER, an increase in the pH value of more than 0.1 could indicate cell autolysis, and might be due to the excretion of yeast metabolites and the uptake and metabolization of pyruvate [42].Frisinga-TUM 34/70 ® , LeoBavaricus-TUM 68 ® , and Harmonia-TUM 511 ® exhibited the strongest capacity for acidification (∆pH 0.8) compared with the other yeast strains.Mel-TUM 211 ® and Tropicus-TUM 506 ® exhibited the weakest capacity for acidification (∆pH 0.5), which might be due to cell autolysis caused by low fermentation performance (see Section 3.2.3).

Phenolic Off-Flavor
Table 10 shows the results of the POF-tests evaluated by sniffing.As shown in Table 10, not all of the investigated yeast strains were capable of building phenolic flavors.The panelists could only detect aroma active components formed by the top-fermenting yeast strains LeoBavaricus-TUM 68 ® and LunaBavaria-TUM 127 ® , commonly used for wheat beer production, and Harmonia-TUM 511 ® (ale beer production) and for Monacus-TUM 381 ® (trappist beer production).For these yeasts, all three corresponding POF-flavors were detected by sniffing.
Figure 6 shows the concentrations of 4-vinylguajacol measured in the finished beers after lagering.According to the evaluation by sniffing, LeoBavaricus-TUM 68 ® , LunaBavaria-TUM 127 ® , Monacus-TUM 381 ® , and Harmonia-TUM 511 ® were POF-positive, with detected concentrations of 4-vinylguajacol above the individual threshold for 4-vinylguajacol of 0.3 mg/L [46].Table 10 shows the results of the POF-tests evaluated by sniffing.As shown in Table 10, not all of the investigated yeast strains were capable of building phenolic flavors.The panelists could only detect aroma active components formed by the top-fermenting yeast strains LeoBavaricus-TUM 68 ® and LunaBavaria-TUM 127 ® , commonly used for wheat beer production, and Harmonia-TUM 511 ® (ale beer production) and for Monacus-TUM 381 ® (trappist beer production).For these yeasts, all three corresponding POF-flavors were detected by sniffing.

Fermentation by-Products
There was a variation in the production of fermentation by-products for all of the yeast strains (Tables 11 and 12).The beers produced with LeoBavaricus-TUM 68 ® , Luna Bavaria-TUM 127 ® , Monacus-TUM 381 ® and Harmonia -TUM 511 ® had the highest levels of isoamyl acetate and 4-vinylguajacol, with concentrations above 2.9 mg/L for isoamyl acetate (Harmonia-TUM 511 ® ) and above 1.2 mg/L for 4-vinylguajacol.The concentration of these esters specific to the production of wheat beers were within the average reference values for regular wheat beers (2-8 mg/L isoamyl acetate and 1-4 mg/L of 4-vinylguajacol) according to Back [47].LeoBavaricus-TUM 68 ® had the highest concentration of higher alcohols (212.07 ± 13.15 mg/L), and the highest level of esters was detected in the beer produced by Harmonia-TUM 511 ® , with a concentration of 57.33 ± 0.65 mg/L.Acetaldehyde, 2.3-pentanedione and diacetyl are associated with unmatured beer, and can result in an unpleasant flavor if the concentrations are above their individual thresholds.The concentration of acetaldehyde is below their individual thresholds of 25 mg/L for all strains.Frisinga-TUM 34/70 ® , LunaBavaria-TUM 127 ® and Colonia-TUM 177 ® showed concentrations of diacetyl above the individual threshold of 0.15 mg/L [46].The production as well as the degradation of diacetyl is strain dependent, and were influenced by fermentation conditions and the yeast management (pitching rate, vitality and viability).

Sulfur Dioxide
Table 13 shows the SO 2 concentration of the finished beers produced by the investigated TUM yeast strains.As shown in the table, all of the investigated yeast strains form sulfur dioxide (SO 2 ) during fermentation.The concentration produced varies from strain to strain and differs by up to a about 9 mg/L SO 2 in the finished beers.This can be confirmed by SWIEGERS and ANNEMÜLLER, who reported that differences between 2 and 10 mg/L SO 2 can be detected in the finished beer under identical fermentation conditions [40,48].In conclusion and also according to the results obtained by MEIER-DÖRNBERG in 2017, the SO 2 formation is mainly influenced by the used yeast strain and is strain dependent [23].As Table 13 shows, Securitas-TUM 193 ® produced the highest quantity of SO 2 at a total amount of 9.47 ± 0.68 on average.According to BACK, each additional mg/L SO 2 below 5 mg/L prolongs the flavor stability of beer by about one month (Back Technologisches Seminar Weihenstephan 2015).Therefore TUM yeast strain Securitas-TUM 193 ® could be very suitable for producing lager beers with a long-term flavor stability.The lowest concentration was produced by yeast strain Monacus-TUM 381 ® and Harmonia-TUM 511 ® at a concentration of 0.5 mg/L.The second lowest concentration in the finished beer of 1.63 ± 0.51 mg/L SO 2 was produced by the top-fermenting wheat beer yeast strain LunaBavaria-TUM 127 ® .Sensory analysis of the beers was conducted after maturation and lagering.All of the beers produced had no prevailing off-flavors and were rated with a four or a five in every category of the DLG scheme for beer (data not shown).In terms of the descriptive sensory evaluation, the following Figures 7-11 show the aroma profile of each investigated TUM yeast strain.The overall flavor impression is shown in orange, and the most distinct individual flavor attributes are shown in blue.The individual flavor attributes represent the most noted and highest rated flavors by all panelists within the seven main aroma categories.The average values of the single flavor attributes are summarized in main categories and represent the overall flavor impression.As shown in the figures, LeoBavaricus-TUM 68 ® and LunaBavaria-TUM 127 ® had a very distinct clove-like aroma.In addition to Monacus-TUM 381 ® and Harmonia-TUM 511 ® , all four Saccharomyces cerevisiae yeast strains were POF positive, with analytically detected concentrations above the individual threshold of 4-vinylguajacol.A clove-like aroma is the main aroma compound in German wheat beers, and probably the reason for why over 90% of the tasters associated the produced and tasted beers with wheat beer.In contrast to LeoBavaricus-TUM 68 ® , LunaBavaria-TUM 127 ® and Monacus-TUM 381 ® , the clove-like flavor was not recognized by the panelists for Harmonia-TUM 511 ® (flavor intensity of 0.14, e.g., Figure 11), even if this strain produced the highest concentration of 4-VG at 3.33 mg/L.
According to MEIER-DÖRNBERG [23], this may be caused and suppressed by synergistic effects and due to the well-balanced flavor profile with citrus and fruity flavors, which were perceived as being slightly more distinct.In conclusion, 28.5% of the panelists could not clearly assign this beer to a wheat nor to an ale style.MEIER-DÖRNBERG suggested that this strain was particularly suitable for brewing a beer with the fruitiness of an ale style brewed beer, underlined by the slightly spicy and yeasty flavors of a wheat beer and proposed calling it "Bavarian Ale".The brewing yeast Mel-TUM 211 ® and Tropicus-TUM 506 ® were an ale beer style, and the beers produced were very fruity.Tropicus-TUM 506 ® has fruity flavors, especially within the tropical fruit category.Vetus-TUM 184 ® also produces fruity and sweet flavors as well as a flavor reminiscent of wine, which was described as dry, and could be responsible for the drier beer flavor expected in beers of the alt type.Colonia-TUM 177 ® seemed to be suitable for more than one beer type.The panelists assigned the beer produced using Colonia-TUM 177 ® to a kölsch and an alt style (27.27% kölsch and alt).The produced beer had a sweet and yeasty flavor with aromas slightly reminiscent of citrus fruits, such as grapefruit.The bottom-fermenting yeast strain Frisinga-TUM 34/70 ® had a well-balanced aroma profile with a tendency towards floral and fruity flavor impressions.The produced beers were clearly described as being lager beers.In comparison, the beers produced using Securitas-TUM 193 ® were also assigned to fruity beer types such as ale and kölsch (28.57%Lager, 14.28% Ale and 14.28% kölsch).This could be confirmed by the specific aroma profile.Securitas-TUM 193 ® was characterized by plenty of fruity flavors, particularly reminiscent of berries, with additional fresh yeasty and sulfuric flavors, typically for lager beers, and a sweet body.
Fermentation 2017, 3, 41 18 of 25 like flavor was not recognized by the panelists for Harmonia-TUM 511 ® (flavor intensity of 0.14, e.g., Figure 11), even if this strain produced the highest concentration of 4-VG at 3.33 mg/L.According to MEIER-DÖRNBERG [24], this may be caused and suppressed by synergistic effects and due to the well-balanced flavor profile with citrus and fruity flavors, which were perceived as being slightly more distinct.In conclusion, 28.5% of the panelists could not clearly assign this beer to a wheat nor to an ale style.MEIER-DÖRNBERG suggested that this strain was particularly suitable for brewing a beer with the fruitiness of an ale style brewed beer, underlined by the slightly spicy and yeasty flavors of a wheat beer and proposed calling it "Bavarian Ale".The brewing yeast Mel-TUM 211 ® and Tropicus-TUM 506 ® were an ale beer style, and the beers produced were very fruity.Tropicus-TUM 506 ® has fruity flavors, especially within the tropical fruit category.Vetus-TUM 184 ® also produces fruity and sweet flavors as well as a flavor reminiscent of wine, which was described as dry, and could be responsible for the drier beer flavor expected in beers of the alt type.Colonia-TUM 177 ® seemed to be suitable for more than one beer type.The panelists assigned the beer produced using Colonia-TUM 177 ® to a kölsch and an alt style (27.27% kölsch and alt).The produced beer had a sweet and yeasty flavor with aromas slightly reminiscent of citrus fruits, such as grapefruit.The bottom-fermenting yeast strain Frisinga-TUM 34/70 ® had a well-balanced aroma profile with a tendency towards floral and fruity flavor impressions.The produced beers were clearly described as being lager beers.In comparison, the beers produced using Securitas-TUM 193 ® were also assigned to fruity beer types such as ale and kölsch (28.57%Lager, 14.28% Ale and 14.28% kölsch).This could be confirmed by the specific aroma profile.Securitas-TUM 193 ® was characterized by plenty of fruity flavors, particularly reminiscent of berries, with additional fresh yeasty and sulfuric flavors, typically for lager beers, and a sweet body.

Conclusions
All 10 investigated TUM brewing yeast strains showed different phenotypic characteristics and flavor profiles.The most interesting differences are presented in the following Table 14 and highlighted in red, yellow, or green according to their performance and brewing characteristics.Based on the results of the genetic analysis, the species identity as well as the genetic distinctness of the investigated TUM yeast strains of the TUM Yeast Center could be confirmed.Except Frisinga-TUM 34/70 ® and Securitas-TUM 193 ® , which belong to the Saccharomyces pastorianus species, all other TUM yeast strains belonged to Saccharomyces cerevisiae.All 10 TUM yeast strains showed different fermentation rates and degrees of apparent attenuation and can be explained by their different ability to ferment maltotriose.The top-fermenting yeast strain Mel-TUM 211 ® only fermented a low level of maltotriose (26.66% ± 0.26%), while the LunaBavaria-TUM 127 ® yeast strain could not ferment maltotriose at all (01.05% ± 2.89%).In the case of non-fermentation of maltotriose, LunaBavaria-TUM 127 ® beers reached their apparent attenuation faster than Mel-TUM 211 ® , and needed less time for fermentation.Except for the strains Mel-TUM 211 ® and Tropicus-TUM 506 ® , the pH of the final beer

Conclusions
All 10 investigated TUM brewing yeast strains showed different phenotypic characteristics and flavor profiles.The most interesting differences are presented in the following Table 14 and highlighted in red, yellow, or green according to their performance and brewing characteristics.Based on the results of the genetic analysis, the species identity as well as the genetic distinctness of the investigated TUM yeast strains of the TUM Yeast Center could be confirmed.Except Frisinga-TUM 34/70 ® and Securitas-TUM 193 ® , which belong to the Saccharomyces pastorianus species, all other TUM yeast strains belonged to Saccharomyces cerevisiae.All 10 TUM yeast strains showed different fermentation rates and degrees of apparent attenuation and can be explained by their different ability to ferment maltotriose.The top-fermenting yeast strain Mel-TUM 211 ® only fermented a low level of maltotriose (26.66% ± 0.26%), while the LunaBavaria-TUM 127 ® yeast strain could not ferment maltotriose at all (01.05% ± 2.89%).In the case of non-fermentation of maltotriose, LunaBavaria-TUM 127 ® beers reached their apparent attenuation faster than Mel-TUM 211 ® , and needed less time for fermentation.Except for the strains Mel-TUM 211 ® and Tropicus-TUM 506 ® , the pH of the final beer

Conclusions
All 10 investigated TUM brewing yeast strains showed different phenotypic characteristics and flavor profiles.The most interesting differences are presented in the following Table 14 and highlighted in red, yellow, or green according to their performance and brewing characteristics.Based on the results of the genetic analysis, the species identity as well as the genetic distinctness of the investigated TUM yeast strains of the TUM Yeast Center could be confirmed.Except Frisinga-TUM 34/70 ® and Securitas-TUM 193 ® , which belong to the Saccharomyces pastorianus species, all other TUM yeast strains belonged to Saccharomyces cerevisiae.All 10 TUM yeast strains showed different fermentation rates and degrees of apparent attenuation and can be explained by their different ability to ferment maltotriose.The top-fermenting yeast strain Mel-TUM 211 ® only fermented a low level of maltotriose (26.66% ± 0.26%), while the LunaBavaria-TUM 127 ® yeast strain could not ferment maltotriose at all (01.05% ± 2.89%).In the case of non-fermentation of maltotriose, LunaBavaria-TUM 127 ® beers reached their apparent attenuation faster than Mel-TUM 211 ® , and needed less time for fermentation.Except for the strains Mel-TUM 211 ® and Tropicus-TUM 506 ® , the pH of the final beer was within the range of 4.4 to 4.6 [49].Mel-TUM 211 ® and Tropicus-TUM 506 ® exhibited the weakest capacity for acidification (∆pH 0.5) of all the investigated strains, which might be due to cell autolysis caused by the low fermentation performance.The total amino acid utilization was also different for each investigated TUM yeast strain, and no conclusion can be drawn as to cell growth.The cell concentration was measured during the main fermentation phase and maturation phase to classify the investigated strains according to their specific flocculation behavior.Not every top-fermenting yeast strain shows powdery behavior.LunaBavaria-TUM 127 ® and Vetus-TUM 184 ® showed a flocculent behavior similar to the bottom-fermenting yeast strains Frisinga-TUM 34/70 ® and Securitas-TUM 193 ® .As expected, some of the yeast strains most commonly used in industry Frisinga-TUM 34/70 ® and LeoBavaricus-TUM 68 ® showed the best phenotypic characteristics, thereby standing out from the other investigated yeast strains.However, every brewer's ultimate goal is the final desirable taste of the produced beer.In this respect, the main focus in this study was on the individual and main flavor impression of the final beers.Only the top-fermenting yeast strains LeoBavaricus-TUM 68 ® , LunaBavaria-TUM 127 ® , Harmonia-TUM 511 ® , and Monacus-TUM 381 ® were capable of building phenolic off-flavors, which was confirmed by the concentrations of 4-vinylguajacol in the finished beers, which were above the individual threshold.Except for the Monacus-TUM 381 ® strain, all panelists recognized the clove like flavor and therefore referred to these beers as wheat style beers.The production of fermentation by-products, as well as the resulting flavor composition in the finished beers was strain-dependent and followed no defined order.The formation of sulfur dioxide (SO 2 ) during fermentation could be detected in all strains, but concentrations differed from 0.50 ± 0.00 mg/L for Monacus-TUM 381 ® and Harmonia-TUM 511 ® , to a considerably higher level on average of 9.47 ± 0.68 mg/L for Securitas-TUM 193 ® .The bottom-fermenting yeast strain Securitas-TUM 193 ® could therefore be very suitable for the production of lager beers with high flavor stability.This characterization model for yeast strains allows brewers around the world access to a simplified and targeted selection of brewing yeast strains suitable for their specific purposes.By analyzing and comparing different yeast strains, breweries can be given customized advice when selecting a yeast strain suitable for their brewing process or type of beer, irrespective of whether they want to replace their existing yeast strain to improve the aroma profile of existing beer styles, develop new beer styles, or optimize the fermentation process by selecting a strain with the corresponding fermentation characteristics.Knowledge about the different yeast strain characteristics can, in particular, promote the competitiveness of small and medium-sized breweries and, if necessary, secure their existence by being part of the steadily increasing market for beer specialties [24].

Table 10 .
Phenolic off-flavor (POF) test results for the investigated yeast strains.

Figure 7 .
Figure 7.Comparison of the flavors grouped according to the main categories and the respective main aroma attributes for the bottom-fermenting Saccharomyces pastorianus yeast strains Frisinga-TUM 34/70 ® and Securitas-TUM 193 ® .

Figure 7 .
Figure 7.Comparison of the flavors grouped according to the main categories and the respective main aroma attributes for the bottom-fermenting Saccharomyces pastorianus yeast strains Frisinga-TUM 34/70 ® and Securitas-TUM 193 ® .

Figure 8 .
Figure 8.Comparison of the flavors grouped according to the main categories and the respective main aroma attributes for the top-fermenting Saccharomyces cerevisiae yeast strains LeoBavaricus-TUM 68 ® and LunaBavaria-TUM 127 ® .

Figure 9 .
Figure 9.Comparison of the flavors grouped according to the main categories and the respective main aroma attributes for top-fermenting Saccharomyces cerevisiae yeast strains Colonia-TUM 177 ® and Vetus-TUM 184 ® .

Figure 8 .
Figure 8.Comparison of the flavors grouped according to the main categories and the respective main aroma attributes for the top-fermenting Saccharomyces cerevisiae yeast strains LeoBavaricus-TUM 68 ® and LunaBavaria-TUM 127 ® .

Figure 8 .
Figure 8.Comparison of the flavors grouped according to the main categories and the respective main aroma attributes for the top-fermenting Saccharomyces cerevisiae yeast strains LeoBavaricus-TUM 68 ® and LunaBavaria-TUM 127 ® .

Figure 9 .
Figure 9.Comparison of the flavors grouped according to the main categories and the respective main aroma attributes for top-fermenting Saccharomyces cerevisiae yeast strains Colonia-TUM 177 ® and Vetus-TUM 184 ® .

Figure 9 .
Figure 9.Comparison of the flavors grouped according to the main categories and the respective main aroma attributes for top-fermenting Saccharomyces cerevisiae yeast strains Colonia-TUM 177 ® and Vetus-TUM 184 ® .

Figure 10 .
Figure 10.Comparison of the flavors grouped according to the main categories and the respective main aroma attributes for top-fermenting Saccharomyces cerevisiae yeast strains Mel-TUM 211 ® and Monacus-TUM 381 ® .

Figure 11 .
Figure 11.Comparison of the flavors grouped according to the main categories and the respective main aroma attributes for top-fermenting Saccharomyces cerevisiae yeast strains Tropicus-TUM 506 ® and Harmonia-TUM 511 ® .

Figure 10 . 25 Figure 10 .
Figure 10.Comparison of the flavors grouped according to the main categories and the respective main aroma attributes for top-fermenting Saccharomyces cerevisiae yeast strains Mel-TUM 211 ® and Monacus-TUM 381 ® .

Figure 11 .
Figure 11.Comparison of the flavors grouped according to the main categories and the respective main aroma attributes for top-fermenting Saccharomyces cerevisiae yeast strains Tropicus-TUM 506 ® and Harmonia-TUM 511 ® .

Figure 11 .
Figure 11.Comparison of the flavors grouped according to the main categories and the respective main aroma attributes for top-fermenting Saccharomyces cerevisiae yeast strains Tropicus-TUM 506 ® and Harmonia-TUM 511 ® .

Table 1 .
Technical University of Munich (TUM) culture yeast strains for industrial brewing.
• C/10 min; 40 cycles of 95 • C/10 s, 60 • C/55 s; 20 • C. IAC135 was developed by RIEDL at the Research Center Weihenstephan for Brewing and Food Quality of the Technical University Munich and is listed in Table

Table 3 .
Primer, probe and target DNA sequences of the internal amplification control system (IAC135) used for real-time PCR systems.

Table 4 .
Starting wort composition used for propagation and brewing trials (12.4 • P wort).

Table 5 .
Qualitative results of the real-time PCR systems used for the investigated yeast strains and the reference strains to differentiate Saccharomyces sensu stricto species.

Table 6 .
Mean percentage of total wort sugar utilization in beer, measured in triplicate after lagering; confidence level 95%.

Table 6 .
Mean percentage of total wort sugar utilization in beer, measured in triplicate after lagering; confidence level 95%.