CA1226835A - Biochemical process and composition - Google Patents
Biochemical process and compositionInfo
- Publication number
- CA1226835A CA1226835A CA000468659A CA468659A CA1226835A CA 1226835 A CA1226835 A CA 1226835A CA 000468659 A CA000468659 A CA 000468659A CA 468659 A CA468659 A CA 468659A CA 1226835 A CA1226835 A CA 1226835A
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- Prior art keywords
- enzyme
- activity
- pentosan
- composition
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- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12C—BEER; PREPARATION OF BEER BY FERMENTATION; PREPARATION OF MALT FOR MAKING BEER; PREPARATION OF HOPS FOR MAKING BEER
- C12C7/00—Preparation of wort
- C12C7/04—Preparation or treatment of the mash
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- A—HUMAN NECESSITIES
- A21—BAKING; EDIBLE DOUGHS
- A21D—TREATMENT, e.g. PRESERVATION, OF FLOUR OR DOUGH, e.g. BY ADDITION OF MATERIALS; BAKING; BAKERY PRODUCTS; PRESERVATION THEREOF
- A21D8/00—Methods for preparing or baking dough
- A21D8/02—Methods for preparing dough; Treating dough prior to baking
- A21D8/04—Methods for preparing dough; Treating dough prior to baking treating dough with microorganisms or enzymes
- A21D8/042—Methods for preparing dough; Treating dough prior to baking treating dough with microorganisms or enzymes with enzymes
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- A—HUMAN NECESSITIES
- A23—FOODS OR FOODSTUFFS; TREATMENT THEREOF, NOT COVERED BY OTHER CLASSES
- A23F—COFFEE; TEA; THEIR SUBSTITUTES; MANUFACTURE, PREPARATION, OR INFUSION THEREOF
- A23F5/00—Coffee; Coffee substitutes; Preparations thereof
- A23F5/16—Removing unwanted substances
- A23F5/163—Removing unwanted substances using enzymes or microorganisms
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- A—HUMAN NECESSITIES
- A23—FOODS OR FOODSTUFFS; TREATMENT THEREOF, NOT COVERED BY OTHER CLASSES
- A23L—FOODS, FOODSTUFFS, OR NON-ALCOHOLIC BEVERAGES, NOT COVERED BY SUBCLASSES A21D OR A23B-A23J; THEIR PREPARATION OR TREATMENT, e.g. COOKING, MODIFICATION OF NUTRITIVE QUALITIES, PHYSICAL TREATMENT; PRESERVATION OF FOODS OR FOODSTUFFS, IN GENERAL
- A23L7/00—Cereal-derived products; Malt products; Preparation or treatment thereof
- A23L7/10—Cereal-derived products
- A23L7/104—Fermentation of farinaceous cereal or cereal material; Addition of enzymes or microorganisms
- A23L7/107—Addition or treatment with enzymes not combined with fermentation with microorganisms
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- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12C—BEER; PREPARATION OF BEER BY FERMENTATION; PREPARATION OF MALT FOR MAKING BEER; PREPARATION OF HOPS FOR MAKING BEER
- C12C5/00—Other raw materials for the preparation of beer
- C12C5/004—Enzymes
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- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12C—BEER; PREPARATION OF BEER BY FERMENTATION; PREPARATION OF MALT FOR MAKING BEER; PREPARATION OF HOPS FOR MAKING BEER
- C12C7/00—Preparation of wort
- C12C7/04—Preparation or treatment of the mash
- C12C7/047—Preparation or treatment of the mash part of the mash being unmalted cereal mash
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- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12C—BEER; PREPARATION OF BEER BY FERMENTATION; PREPARATION OF MALT FOR MAKING BEER; PREPARATION OF HOPS FOR MAKING BEER
- C12C9/00—Methods specially adapted for the making of beerwort
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- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12N—MICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
- C12N9/00—Enzymes; Proenzymes; Compositions thereof; Processes for preparing, activating, inhibiting, separating or purifying enzymes
- C12N9/14—Hydrolases (3)
- C12N9/24—Hydrolases (3) acting on glycosyl compounds (3.2)
- C12N9/2402—Hydrolases (3) acting on glycosyl compounds (3.2) hydrolysing O- and S- glycosyl compounds (3.2.1)
- C12N9/2405—Glucanases
- C12N9/2434—Glucanases acting on beta-1,4-glucosidic bonds
- C12N9/244—Endo-1,3(4)-beta-glucanase (3.2.1.6)
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- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12P—FERMENTATION OR ENZYME-USING PROCESSES TO SYNTHESISE A DESIRED CHEMICAL COMPOUND OR COMPOSITION OR TO SEPARATE OPTICAL ISOMERS FROM A RACEMIC MIXTURE
- C12P19/00—Preparation of compounds containing saccharide radicals
- C12P19/14—Preparation of compounds containing saccharide radicals produced by the action of a carbohydrase (EC 3.2.x), e.g. by alpha-amylase, e.g. by cellulase, hemicellulase
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- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12Y—ENZYMES
- C12Y302/00—Hydrolases acting on glycosyl compounds, i.e. glycosylases (3.2)
- C12Y302/01—Glycosidases, i.e. enzymes hydrolysing O- and S-glycosyl compounds (3.2.1)
- C12Y302/01006—Endo-1,3(4)-beta-glucanase (3.2.1.6)
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- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12Y—ENZYMES
- C12Y302/00—Hydrolases acting on glycosyl compounds, i.e. glycosylases (3.2)
- C12Y302/01—Glycosidases, i.e. enzymes hydrolysing O- and S-glycosyl compounds (3.2.1)
- C12Y302/01073—Licheninase (3.2.1.73)
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Abstract
Abstract of the Disclosure "Biochemical Process and Composition"
There is described an enzyme and a composition containing it which has pentosanase activity, particularly at higher temperatures e.g. around 90°C. The enzyme and composition may be prepared by fermentation of Talaromyces emersonii, particularly strain IMI
116815 and means for enriching the fermentation broth with pentosanase activity relative to other enzyme activity which may also be present is also disclosed.
The enzyme and composition containing it have a wide range of possible uses, particularly where thermostability is important, including applications in baking, starch manufacture, mixed silage and animal feed production, and tea and coffee extraction.
There is described an enzyme and a composition containing it which has pentosanase activity, particularly at higher temperatures e.g. around 90°C. The enzyme and composition may be prepared by fermentation of Talaromyces emersonii, particularly strain IMI
116815 and means for enriching the fermentation broth with pentosanase activity relative to other enzyme activity which may also be present is also disclosed.
The enzyme and composition containing it have a wide range of possible uses, particularly where thermostability is important, including applications in baking, starch manufacture, mixed silage and animal feed production, and tea and coffee extraction.
Description
isle BIOCHEMICAL PROCESS END COMPOSITION
This invention relates to a novel process for the biodegradation of pentosans, to an enzyme useful therefore and a process for obtaining a composition containing it.
Pentosans are a class of polymers of one or more naturally-occurring pentoses. They occur in a variety of natural sources, such as cereals, e.g. wheat and oats, plants erg. tea and coffee, seaweed, fruits, vegetables and sorghum, and their presence is undesirable in a number of applications to which the natural source may be put. Thus, for example, pentosans occur in cereal flour, in which they bind water, and they contribute to stiffening or staling of bread after baking. reduction in the pentosan content of the flour reduces the liability to stiffening in this situation. In another example, pentosans occur in coffee and occur in soluble gums co-extracted with the coffee in the manufacture of instant coffee granules or powder. Reducing the pentosan content of such materials enables higher solid levels to be achieved in the extraction with consequent economies in the manufacturing process.
In our British Patent Specification No. 1421127, we describe a method for the production of enzymes which will degrade ~-glucans derived from barley and related B-1,4/~-1,3 glucans. Roy principal enzyme obtained is a 4/3~1,3-glucanase, of particular value in the treatment of barley, although other ~-glucanase, laminarinase, hydroxyethyl cellulose, cellulose and aimless activities are said also to be able to be present. Microorganisms of the species Penicillium emersonii are employed as the enzyme source, and in particular the strain which was deposited with the Commonwealth Mycological Institute, Knew, England under the number IMP 116815.
I! I I
We have now been able to ferment TalaromYces emersonil (formerly known as Penicillium emersonii) in order to produce another enzyme, a pentosanase, which will catalyze the degradation of pentosans, particularly pentosans derived from wheat The class of such enzymes is generally known and various individual enzymes have been used in, inter alias baking, starch manufacture, farming, brewing, the extraction of vegetable tissue and the manufacture lo of vegetable coloring materials. However, in many of these applications, high temperatures are routinely employed and there is a need for a thermos table pentosanase which will retain good activity over a wide range of elevated temperatures.
Thus in one aspect of the present invention we provide an enzyme obtainable by fermentation from a strain of the species Talaromyces emersonii, in particular from TalaromYces emersonii Stork, sync Penicillium emersonii Stork IMP 116815, or a mutant thereof, which is capable of catalyzing the degradation of pentosans~ The new enzyme has been found lo, be produced in good yield and at a concentration highly satisfactory for commercial use.
In a particular aspect of the invention we provide an enzyme obtainable by fermentation from a strain of the species T. emersonii, in particular T. emersonii IMP ]16815, or a mutant thereof, which is capable of catalyzing the degradation of Dylan.
Dylan is a polymer of the Penrose Zulus.
The new enzyme has been found to be thermos table, i.e. it retains good activity at elevated temperatures, and hence is of particular value in the high temperature degradation of pentosans. For example, in stability measurements, using enzyme prepared according to the procedure of Example l described hereinafter, the enzyme still retained 50% of its initial activity Al ~2~i~35 after heating at 95~C for six minutes at pi 5.0 in the absence of substrate. The enzyme also exhibits an advantageous temperature-activity relationship, with optimum activity using oat hull Dylan as substrate at 87 + 2C and retention of 45% of optimum activity at 95C. This is unusual in an enzyme of finagle origin, and contrasts for example, with the ~-glucanase described above which has a poorly defined optimum at 60-70C and only retains 40~ of this peak activity 0 at 80C~
The enzyme according to the invention has the following characteristics, measured using a crude enzyme preparation obtained by the procedure of Example 1 described hereinafter: 5 (a) the pi for the optimum activity of the new enzyme is 5.0, measured at 50C and using oat hull Dylan as the pentosan substrate;
(b) the temperature for the optimum activity of the new enzyme is 87+2C, measured at pi 5.0 using oat hull Dylan as the pentosan substrate;
(c) the presence of previously added Zulus, glucose or maltose has no effect on enzyme activity when subsequently assayed at pi 5.0 and 50C using oat hull Dylan substrate.
The enzyme according to the invention may generally be prepared by fermenting an inoculum of T. emersonii, for example T. Emerson IMP 116815 or a mutant thereof in a nutrient medium therefore.
However, we have further found that the amount of pentosanase naturally produced may be increased relative to the amount of 3-glucanase produced by suitable modification of the fermentation medium.
An enzyme preparation obtained directly by the fermentation of Talaromyces emersonii, desirably T. emersonii IMP 116815 in which the level of pentosanase activity relative to any ~-1,4/~-1,3-glucanase activity is higher as a result of such modification than that which may conventionally be obtained is a preferred feature of the invention, as is a process for its preparation.
The fermentation may be carried out by methods well-known in the fermentation industry. Thus the strain of T. emersonii may be cultured under aerobic conditions, preferably in submerged culture, with agitation or stirring with air or oxygen.
The fermentation medium employed should contain an assimilable source of carbon, a digestible source of nitrogen and, if desired, growth-promoting substances as well as inorganic salts.
Suitable carbon sources include materials rich in pentosans, for example, cereals such as barley and wheat, distillers solubles or other malt-or grain-distillation by-products, cellulose e.g. Polka Floe, or Dylan.
Suitable nitrogen sources include, for example, barley, distillers solubles or other malt- or grain-distillation by-products, soya meal, nitrates or ammonium salts such as ammonium dihydrogen phosphate.
Where it is desired to increase the level of pentosanase activity relative to any ~-glucanase activity, a carbon or nitrogen source selected from Scotagran (a mix of solubles with dried barley grains), ammonium nitrate, pot ale syrup, maize pellets (dried maize grains mixed with solubles), Curve syrup and corn steep liquor will desirably be used.
Inorganic salts which may be used in the fermentation medium may be, for example, sulfites or chlorides of potassium, magnesium or sodium.
Growth promoting substances which may be used include trace elements such as manganese, iron, zinc, copper or phosphorus.
Advantageously, the fermentation medium contains barley in a concentration in the range 0.2 to 3.5 w/v, distillers solubles or other malt or grain distillation by-products in a concentration in the range 0.4 to 5.5% w/v, and 0.2 to 3.0% w/v cellulose.
Culturing conditions such as temperature, pi and fermentation time are selected such that the strain employed may accumulate a maximum amount of the desired enzyme For example, the fermentation is advantageously carried out at a temperature ranging from 35-60C, preferably 50-54C, at a pi from 3.5-4.5 and for from 1-20 days, preferably 7-10 days.
The crude culture liquid can be used directly for its enzymatic action, or if desired the whole culture broth may be dried and the resulting powder used. If desired, some purification of the pentosanase may be carried out, e.g. by chromatographic techniques, to provide an enzyme preparation having increased pentosanase activity relative to any ~-1,4/1,3-glucanase activity and a method for effecting such purification and the product obtained comprise further aspects of the invention.
Alternatively, the enzyme, which is exocellular, may be extracted from the fermentation product by, for example, conventional methods. Thus for example a first stage is normally to filter off the Muslim formed, preferably by means of precut filtration, i.e. using a filter which has been coated with a filter aid. The resulting filtrate may be used directly, or, conveniently, may be concentrated, preferably in vacua to yield the enzyme in a liquid concentrate form. The liquid concentrate may itself be employed as the enzyme source. Materials such as sodium chloride, sodium bonniest or sodium metabisulphite which confer enzyme storage stability, enzyme thermostability and/or bacteriological stability may if desired be added to such liquid concentrates. Alternatively, the liquid concentrate may be absorbed in a suitable solid, for example ground wheat or barley, optionally in the presence of a carrier such as sodium carboxymethyl cellulose, and the resulting damp mass dried to yield an active enzyme product. If desired, the liquid concentrate itself may be dried, e.g. by spray drying, freeze drying or roller drying to yield a dry enzyme composition.
Unless the extraction is rigorous, which for commercial purposes is usually avoided for economic reasons and is not necessary given the range of uses to which a cruder composition can be put, the composition will usually contain other enzyme activities.
Where a solid enzyme product is desired, this may be obtained from the filtrate or a liquid concentrate thereof by conventional methods, such as precipitation by addition for example of an excess of a water-miscible organic solvent such as an alcohol e.g. ethanol or a kitten e.g. acetone.
Either direct precipitation or precipitation onto a carrier may be used typical carriers including for example starch methyl cellulose or sodium carboxymethyl cellulose.
The inoculum ox T. emersonii used in the . .
fermentation may be obtained by, for example, scaling up from a surface culture of the organism. Scaling up to productive fermentation may conveniently be effected by carrying out a laboratory stage of vegetative growth, followed by one or more seed stages in stirred fermentation vessels.
Thus, in a typical inoculum preparation, the organism is streaked onto a solid nutrient medium, e.g. an ajar medium containing petunia (e.g. 0.5~ w/v), sodium chloride (e.g. 0.4% wove), ;226~35 glycerol (e.g. 0.75~ w/v), molasses twig 0.8~
w/v), potassium dihydrogen phosphate (e.g. 0.006%
w/v) and magnesium sulfite (e.g. 0.005% McCoy w/v) which has previously been sterilized, e.g.
by autoclaving at about 120C for 15 minutes, and allowed to cool. Incubation is preferably carried out at about 37C for about 10 days, after which the spores produced are used to inoculate a liquid medium for vegetative growth, sterilized by e.g.
autoclaving, at about 120C for 15 minutes, and containing malt extract (e.g. 3.3~ w/v), yeast extract (e.g. 2.0~ w/v) and ammonium dihydrogen phosphate (e.g. 0.6~ w/v). The culture is preferably effected until good mycelial growth is present, for example, when using about 500ml of medium, for about 72 hours at 45C.
The resulting vegetative culture is then used to inoculate a first stirred seed stage.
The medium for this stage preferably contains similar components to those described previously for the main fermentation medium, and is preferably prepared by sterilizing all the ingredients together in the seed stage vessel e.g. by steam injection.
A typical medium for the seed stage is 'Medium A' shown hereinafter in Table 1. Using about 40 liters of medium, culturing is preferably effected at about 50C for about 76 hours with stirring, e.g. at 420 rum and aeration, e.g. 50 litres/minute of air.
The seed culture thus obtained may then be used to inoculate a producing stage as described above or, if more seed is required, may be used in further seed stages, identical in nature to be first.
Mutants of T. emersonii for use in the above fermentation processes may be obtained by conventional methods of strain improvements, e.g. by the use I
of ionizing radiation (for example X and y-rays;
us light; or us light in the presence of a photo-sensitizing agent such as 8-methoxypsoralen), chemicals (e.g. nitrous oxide; hydroxylamine; pyrimidine base analogies such as 5-bromouracil; assuredness;
alkylating agents such as ethyl methanesulphonate or mustard gas; hydrogen peroxide; phenols or formal-Dodd), heat or genetic techniques (ego recombination, transduction, transformation, lysogenisation, lysogenic conversion and selective techniques for spontaneous mutants).
The desired enzyme activity may be determined in the culture liquid or at any point in an isolation procedure by a simple test designed to determine the reducing sugars released by the action of the enzyme on a pentosan substrate. Thus, in one test, a sample of the enzyme preparation to be measured is suitably diluted and is then incubated for 10 minutes with an excess of the pentosan Dylan, at 50C in pi 5.0 acetate buffer. The sugar released is determined as a maltose equivalent by adding alkaline 3,5-dinitrosalicylic acid reagent, heating for 5 minutes on a boiling water bath, quenching in ice water, measuring the absorption of the solution at 540nm and converting this to a maltose equivalent by reference to a standard calibration graph obtained by preparing standard dilutions of maltose of known moisture content and reacting these with the donator-salicylic reagent under the conditions lust described.
As used herein, one unit of enzyme releases 1 my of maltose equivalent per minute under the test conditions at 50C and pi 5Ø
The enzyme according to the invention is useful for a variety of purposes for which other pentosanases are used. Thus, for example, it may be used in baking, to reduce the natural pentosan content of wheat flour and so improve the keeping qualities of bread. It may be used in starch manufacture and hydrolysis, to lower the pentosan content of cereals and reduce the viscosity of starch slurries which otherwise adversely affect the efficiency and cost of starch recovery and subsequent hydrolysis It may be used in farming, to upgrade the quality of mixed silage and animal feeds. It may be used in brewing, for the improved production and extraction of fermentable sugars when the mash includes e.g.
wheat or sorghum, and for the prevention or treatment of certain types of haze. It may be used for the extraction of vegetable tissue, for example in the extraction of tea, coffee and fruits; and to extract alginates from seaweed; and in the manufacture of natural vegetable coloring materials. In some of these applications, the thermostability of the enzyme is particularly advantageous in view of the temperatures at which the processes are conducted.
In a further aspect of the invention, therefore, we provide a method of reducing the pentosan content of a pentosan-containing material which comprises contacting the said material with an enzyme of the invention.
Typical pentosans which may be degraded with the enzyme of the invention include those found in cereals such as wheat and oats; plants such as tea and coffee and in extracts thereof; fruits;
vegetables; seaweed and sorghum. In one example, the pentosan may be Dylan, for example an oat hull Dylan. In a preferred embodiment, the pentosan-containing material which is to be degraded is derived from wheat.
In a further embodiment of the invention we provide a method of reducing the Dylan content of a xylan-containing material wherein the material is contacted with an enzyme according to the invention.
The enzyme or composition according to the 33~
invention may be used employing methods customarily found in enzyme technology. Thus for example the enzyme may be contacted with an aqueous medium containing the substrate either in suspension, admix or in a solution. The reaction temperature will vary according to the exact nature of the reaction but will in general be in the range 35-95C, advantageously at the higher end of the range, in some applications at 90C and above The pi of the reaction mixture may be for example in the range 4.0-6.5, preferably 4.5-5.5 and in particular at pi 5Ø If desired, the reaction mixture may contain other added enzymes, for example aimless.
The strain of Toolers emersonii which we have used is a sub-culture of that which was deposited at the Commonwealth Mycological Institute, Knew, England under Number IMP 116815 in 1972 before the Budapest Treaty on the International Recognition of the Deposit of Microorganisms for the purposes of Patent Procedure (Budapest 1977) was signed.
We have recently redeposited this strain (on 1984) under slumber IMP 290604 at the same depository but under the conditions of the Treaty of Budapest and it is our belief that the two strains are identical and that either strain may be used.
The following Examples illustrate the invention.
All temperatures are in C. All percentages are in w/v.
I
E _ pie 1 Talaromyces emersonii IMP 116815 was cultured at 37 for 10 days on an ajar medium sterilized in an autoclave and containing 0.5% petunia, 0.4~
Nail, 0.75% glycerol, 0.8% molasses, 0.006% KH2PO4 and 0.005~ McCoy).
The spores produced were used to inoculate flasks of a liquid medium sterilized by autoclaving and containing 3.3% malt extract, 2.0% yeast extract and 0.6% ammonium dihydrogen phosphate. The flasks were placed on a rotary shaker (210 rev/min; 4.9 cm throw) for 3 days at 45.
The resulting vegetative culture (400 ml) was used to inoculate 40 liters of Medium A) Table 1 sterilized by steam injection in a 50 lithe capacity stainless steel fermenter. The culture was stirred at 420 rev/min and aerated at 50 litres/min for 75 hours at 50.
The resulting culture (4.5 L) was used to inoculate 40 liters of Medium A (Table 1) sterilized by steam injection in a 50 lithe capacity stainless steel fermenter. The culture was stirred at 420 rev/min and aerated at 50 litres/min for 75 hours at 50.
The resulting culture (4.5 L) was used to inoculate 40 liters of Medium A sterilized by steam injection in a 50 lithe capacity stainless steel fermenter. The culture was stirred at 420 rev/min and aerated at 50 litres/min for 36 hours at 50.
The resulting culture (16 L) was used to inoculate 32 liters of Medium B (Table 1) sterilized by steam injection in a 50 lithe capacity stainless steel fermenter.
The culture was aerated at 50 litres/min.
35 and stirred intermittently at 420 rev/min. at 50 for 10 days. Sterile water was added at an average rate of 1.5 liters per day.
Assay of the exocellular fluid yielded a concentration of the enzyme according to the invention Of 36 u/
Table 1 Ingredient Medium A (~) Medium B (~) Ground Barley 1.0 3.38 Distillers Solubles 2.25 5.06 Polka Floe 2025 2.53 ( H4)2 H2PO4 0.34 0 77 K2SO4 0.12 0.27 M9S04'7H20 0.01 0.11 Nail 0.11 0.11 MnSO4-4H2o .S 0.001 15 Phase 0.004 0.008 ZnSO4.7H2O 0.004 0.008 QUIZ 0 0005 0.001 POW 0.5 1.02 Water to 100 Example 2 Demonstration of variation in pentosanase: glucanase ratio on fermentation a) Spores were produced as in Example 1 and used to inoculate a seed stage in 250 ml flasks containing 40 ml of Medium A sterilized by autoclaving. The flasks were incubated at 45 for 72 hours, shaking at 200 rev/min.
The resulting culture (4 ml) was used to inoculate 40 ml of Medium B sterilized by autoclaving in 250 ml flasks. after incubating at 45 for 12 days, shaking at 200 rev/min, the exocellular culture fluid was assayed or pentosanase (P) and barley ~-glucanase (G) activities and the P : G ratio was calculated.
b) Using essentially the same system as in a) above.
I
Omitting the Polka Floe and including oat spells Dylan (2.2%) gave a P : G ratio 71%
higher than that obtained in a).
Example 3 In order to demonstrate pentosanase activity in the enzyme produced in Example 1, a 1% pentosan solution was incubated at 50 in buffer at pi 5.0 in the presence of added enzyme (test system) or with the addition of an equivalent amount of water (control system). The pentosan substrate used was Dylan, obtained from oat hulls.
Samples of the test system were withdrawn after 10 minutes, 30 minutes and 22.5 hours, quenched to prevent any further reaction and then spotted on to 20 cm square thin layer chromatography plates covered with 0.25 mm kieselgel. Spots of selected standard sugar solutions and of the control system were also applied.
The mobile phase was n-butanol:pyridine:ethanol:
water (20:15:25:10). Detection was by spraying the dried plates with 5% ammonium molybdate in 5% sulfuric acid followed by heating at 105 for 15 miss.
All the test samples showed inter aria a spot of identical Of value to that given by the standard sugar solution Zulus.
Since the control sample gave only a single spot on the origin, this test spot can not have derived either from Zulus contamination of the substrate or from its chemical hydrolysis: it must have arisen by enzymic degradation of the pentosan.
Example 4 The following comparative test was designed to illustrate the potential utility of the enzyme according to the invention in an enzymatic wheat ;26~35 starch digestion process:
Enzyme (2 ml) prepared according to Example 1, low grade wheat flour (155 g), sodium chlorite (2 9), calcium chloride (0.17 g), 'Termamyl' bacterial alpha aimless (Nova Industry A/S) (1 ml) and water (250 ml) were shaken thoroughly in a glass flask.
The pi was adjusted to 6.5 using caustic soda.
The neck of the container was covered to minimize evaporation and the flask was held for 5 hours at a temperature of 90. Starch hydrolysis occurred (negative iodine test result) and the divest viscosity was 43 cups.
In a control experiment omitting the enzyme of the invention the final viscosity of the digest was 127 cups.
The following Examples illustrate experiments performed to characterize the enzyme according to the invention In each Example, the enzyme used was prepared according to the method of Example 1 except that small amounts of sodium bonniest and sodium met:abisulphite were added to the exocellular fluid as bacteriological stabilizers. Enzyme activity was determined in each Example using an excess of 1% aqueous oat hull. Dylan as the pentosan substrate and measuring the increase in reducing activity after a 10 mix incubation, against a Zulus calibration curve. The pi and temperature of each incubation are stated in the Examples.
-Example 5 The pH-activity relationship was obtained at a temperature of 50 pi 4.0 4.5 5.0 5.5 6.0 6.5 .
% Maximum Activity 62 85 100 84 70 47 _ _ __ I_._ _ _ _ _ _ _ ._ _ _ _ ._ _ _ , _ _. _ _ _ _ _ ___ _ __ __ _ ago Pry' I
Significant hydrolysis occurs throughout the range illustrated.
Example 6 Thermal stability was studied by holding samples at temperatures of 60, 70, 80, 90 and 95 in the absence of substrate and withdrawing amounts at timed intervals to obtained a family of residual activity-time curves. The activity remaining was measured at pi 5.0 and 50:
- at 60, there was no detectable loss in activity after 80 miss, - at 70, 70~ of the initial activity was still present after 1 h, 15 - at 80, 70% of the initial activity was still present after 30 miss, - at 90, 50~ of the initial activity was still present after 8 miss, - at 95, 50% of the initial activity was still present after 6 miss.
Example 7 The temperature - activity relationship was obtained at a pi of 5Ø Inspection of the activity-temperature curve showed that peak activity occurred at 87+2. Activities at the individual temperatures studied, expressed as percentages of this maximum, were as follows:
% Maximum Activity 13 24 41 57 86 [100] 90 45 Temperature 40 50 60 70 80 [87+2] 90 95 The results confirm the inherent thermal stability of the new enzyme, as shown in example 5. The enzyme can clearly be used at temperatures in excess of 90.
~6~33~
This contrasts with a poorly defined optimum of 60-70 for the barley ~-glucanase of British Specification 1,421,127. At 80, only 40% of peak activity is recorded.
Example 8 In a preliminary study to determine whether activity of the enzymes was affected by products of the reaction and/or other sugars present in a typical digest in an industrial process, three simple sugars (Zulus, glucose and maltose) were separately added to the enzyme, which was then assayed at 50 and pi 5Ø Each sugar was added in an amount equivalent to the amount of Zulus liberated from the substrate under the assay conditions.
There was no inhibition or promotion of enzyme activity, and thus, on this evidence, there would be no interference with enzyme activity from the accumulation of simple sugars that will occur in many industrial applications.
This invention relates to a novel process for the biodegradation of pentosans, to an enzyme useful therefore and a process for obtaining a composition containing it.
Pentosans are a class of polymers of one or more naturally-occurring pentoses. They occur in a variety of natural sources, such as cereals, e.g. wheat and oats, plants erg. tea and coffee, seaweed, fruits, vegetables and sorghum, and their presence is undesirable in a number of applications to which the natural source may be put. Thus, for example, pentosans occur in cereal flour, in which they bind water, and they contribute to stiffening or staling of bread after baking. reduction in the pentosan content of the flour reduces the liability to stiffening in this situation. In another example, pentosans occur in coffee and occur in soluble gums co-extracted with the coffee in the manufacture of instant coffee granules or powder. Reducing the pentosan content of such materials enables higher solid levels to be achieved in the extraction with consequent economies in the manufacturing process.
In our British Patent Specification No. 1421127, we describe a method for the production of enzymes which will degrade ~-glucans derived from barley and related B-1,4/~-1,3 glucans. Roy principal enzyme obtained is a 4/3~1,3-glucanase, of particular value in the treatment of barley, although other ~-glucanase, laminarinase, hydroxyethyl cellulose, cellulose and aimless activities are said also to be able to be present. Microorganisms of the species Penicillium emersonii are employed as the enzyme source, and in particular the strain which was deposited with the Commonwealth Mycological Institute, Knew, England under the number IMP 116815.
I! I I
We have now been able to ferment TalaromYces emersonil (formerly known as Penicillium emersonii) in order to produce another enzyme, a pentosanase, which will catalyze the degradation of pentosans, particularly pentosans derived from wheat The class of such enzymes is generally known and various individual enzymes have been used in, inter alias baking, starch manufacture, farming, brewing, the extraction of vegetable tissue and the manufacture lo of vegetable coloring materials. However, in many of these applications, high temperatures are routinely employed and there is a need for a thermos table pentosanase which will retain good activity over a wide range of elevated temperatures.
Thus in one aspect of the present invention we provide an enzyme obtainable by fermentation from a strain of the species Talaromyces emersonii, in particular from TalaromYces emersonii Stork, sync Penicillium emersonii Stork IMP 116815, or a mutant thereof, which is capable of catalyzing the degradation of pentosans~ The new enzyme has been found lo, be produced in good yield and at a concentration highly satisfactory for commercial use.
In a particular aspect of the invention we provide an enzyme obtainable by fermentation from a strain of the species T. emersonii, in particular T. emersonii IMP ]16815, or a mutant thereof, which is capable of catalyzing the degradation of Dylan.
Dylan is a polymer of the Penrose Zulus.
The new enzyme has been found to be thermos table, i.e. it retains good activity at elevated temperatures, and hence is of particular value in the high temperature degradation of pentosans. For example, in stability measurements, using enzyme prepared according to the procedure of Example l described hereinafter, the enzyme still retained 50% of its initial activity Al ~2~i~35 after heating at 95~C for six minutes at pi 5.0 in the absence of substrate. The enzyme also exhibits an advantageous temperature-activity relationship, with optimum activity using oat hull Dylan as substrate at 87 + 2C and retention of 45% of optimum activity at 95C. This is unusual in an enzyme of finagle origin, and contrasts for example, with the ~-glucanase described above which has a poorly defined optimum at 60-70C and only retains 40~ of this peak activity 0 at 80C~
The enzyme according to the invention has the following characteristics, measured using a crude enzyme preparation obtained by the procedure of Example 1 described hereinafter: 5 (a) the pi for the optimum activity of the new enzyme is 5.0, measured at 50C and using oat hull Dylan as the pentosan substrate;
(b) the temperature for the optimum activity of the new enzyme is 87+2C, measured at pi 5.0 using oat hull Dylan as the pentosan substrate;
(c) the presence of previously added Zulus, glucose or maltose has no effect on enzyme activity when subsequently assayed at pi 5.0 and 50C using oat hull Dylan substrate.
The enzyme according to the invention may generally be prepared by fermenting an inoculum of T. emersonii, for example T. Emerson IMP 116815 or a mutant thereof in a nutrient medium therefore.
However, we have further found that the amount of pentosanase naturally produced may be increased relative to the amount of 3-glucanase produced by suitable modification of the fermentation medium.
An enzyme preparation obtained directly by the fermentation of Talaromyces emersonii, desirably T. emersonii IMP 116815 in which the level of pentosanase activity relative to any ~-1,4/~-1,3-glucanase activity is higher as a result of such modification than that which may conventionally be obtained is a preferred feature of the invention, as is a process for its preparation.
The fermentation may be carried out by methods well-known in the fermentation industry. Thus the strain of T. emersonii may be cultured under aerobic conditions, preferably in submerged culture, with agitation or stirring with air or oxygen.
The fermentation medium employed should contain an assimilable source of carbon, a digestible source of nitrogen and, if desired, growth-promoting substances as well as inorganic salts.
Suitable carbon sources include materials rich in pentosans, for example, cereals such as barley and wheat, distillers solubles or other malt-or grain-distillation by-products, cellulose e.g. Polka Floe, or Dylan.
Suitable nitrogen sources include, for example, barley, distillers solubles or other malt- or grain-distillation by-products, soya meal, nitrates or ammonium salts such as ammonium dihydrogen phosphate.
Where it is desired to increase the level of pentosanase activity relative to any ~-glucanase activity, a carbon or nitrogen source selected from Scotagran (a mix of solubles with dried barley grains), ammonium nitrate, pot ale syrup, maize pellets (dried maize grains mixed with solubles), Curve syrup and corn steep liquor will desirably be used.
Inorganic salts which may be used in the fermentation medium may be, for example, sulfites or chlorides of potassium, magnesium or sodium.
Growth promoting substances which may be used include trace elements such as manganese, iron, zinc, copper or phosphorus.
Advantageously, the fermentation medium contains barley in a concentration in the range 0.2 to 3.5 w/v, distillers solubles or other malt or grain distillation by-products in a concentration in the range 0.4 to 5.5% w/v, and 0.2 to 3.0% w/v cellulose.
Culturing conditions such as temperature, pi and fermentation time are selected such that the strain employed may accumulate a maximum amount of the desired enzyme For example, the fermentation is advantageously carried out at a temperature ranging from 35-60C, preferably 50-54C, at a pi from 3.5-4.5 and for from 1-20 days, preferably 7-10 days.
The crude culture liquid can be used directly for its enzymatic action, or if desired the whole culture broth may be dried and the resulting powder used. If desired, some purification of the pentosanase may be carried out, e.g. by chromatographic techniques, to provide an enzyme preparation having increased pentosanase activity relative to any ~-1,4/1,3-glucanase activity and a method for effecting such purification and the product obtained comprise further aspects of the invention.
Alternatively, the enzyme, which is exocellular, may be extracted from the fermentation product by, for example, conventional methods. Thus for example a first stage is normally to filter off the Muslim formed, preferably by means of precut filtration, i.e. using a filter which has been coated with a filter aid. The resulting filtrate may be used directly, or, conveniently, may be concentrated, preferably in vacua to yield the enzyme in a liquid concentrate form. The liquid concentrate may itself be employed as the enzyme source. Materials such as sodium chloride, sodium bonniest or sodium metabisulphite which confer enzyme storage stability, enzyme thermostability and/or bacteriological stability may if desired be added to such liquid concentrates. Alternatively, the liquid concentrate may be absorbed in a suitable solid, for example ground wheat or barley, optionally in the presence of a carrier such as sodium carboxymethyl cellulose, and the resulting damp mass dried to yield an active enzyme product. If desired, the liquid concentrate itself may be dried, e.g. by spray drying, freeze drying or roller drying to yield a dry enzyme composition.
Unless the extraction is rigorous, which for commercial purposes is usually avoided for economic reasons and is not necessary given the range of uses to which a cruder composition can be put, the composition will usually contain other enzyme activities.
Where a solid enzyme product is desired, this may be obtained from the filtrate or a liquid concentrate thereof by conventional methods, such as precipitation by addition for example of an excess of a water-miscible organic solvent such as an alcohol e.g. ethanol or a kitten e.g. acetone.
Either direct precipitation or precipitation onto a carrier may be used typical carriers including for example starch methyl cellulose or sodium carboxymethyl cellulose.
The inoculum ox T. emersonii used in the . .
fermentation may be obtained by, for example, scaling up from a surface culture of the organism. Scaling up to productive fermentation may conveniently be effected by carrying out a laboratory stage of vegetative growth, followed by one or more seed stages in stirred fermentation vessels.
Thus, in a typical inoculum preparation, the organism is streaked onto a solid nutrient medium, e.g. an ajar medium containing petunia (e.g. 0.5~ w/v), sodium chloride (e.g. 0.4% wove), ;226~35 glycerol (e.g. 0.75~ w/v), molasses twig 0.8~
w/v), potassium dihydrogen phosphate (e.g. 0.006%
w/v) and magnesium sulfite (e.g. 0.005% McCoy w/v) which has previously been sterilized, e.g.
by autoclaving at about 120C for 15 minutes, and allowed to cool. Incubation is preferably carried out at about 37C for about 10 days, after which the spores produced are used to inoculate a liquid medium for vegetative growth, sterilized by e.g.
autoclaving, at about 120C for 15 minutes, and containing malt extract (e.g. 3.3~ w/v), yeast extract (e.g. 2.0~ w/v) and ammonium dihydrogen phosphate (e.g. 0.6~ w/v). The culture is preferably effected until good mycelial growth is present, for example, when using about 500ml of medium, for about 72 hours at 45C.
The resulting vegetative culture is then used to inoculate a first stirred seed stage.
The medium for this stage preferably contains similar components to those described previously for the main fermentation medium, and is preferably prepared by sterilizing all the ingredients together in the seed stage vessel e.g. by steam injection.
A typical medium for the seed stage is 'Medium A' shown hereinafter in Table 1. Using about 40 liters of medium, culturing is preferably effected at about 50C for about 76 hours with stirring, e.g. at 420 rum and aeration, e.g. 50 litres/minute of air.
The seed culture thus obtained may then be used to inoculate a producing stage as described above or, if more seed is required, may be used in further seed stages, identical in nature to be first.
Mutants of T. emersonii for use in the above fermentation processes may be obtained by conventional methods of strain improvements, e.g. by the use I
of ionizing radiation (for example X and y-rays;
us light; or us light in the presence of a photo-sensitizing agent such as 8-methoxypsoralen), chemicals (e.g. nitrous oxide; hydroxylamine; pyrimidine base analogies such as 5-bromouracil; assuredness;
alkylating agents such as ethyl methanesulphonate or mustard gas; hydrogen peroxide; phenols or formal-Dodd), heat or genetic techniques (ego recombination, transduction, transformation, lysogenisation, lysogenic conversion and selective techniques for spontaneous mutants).
The desired enzyme activity may be determined in the culture liquid or at any point in an isolation procedure by a simple test designed to determine the reducing sugars released by the action of the enzyme on a pentosan substrate. Thus, in one test, a sample of the enzyme preparation to be measured is suitably diluted and is then incubated for 10 minutes with an excess of the pentosan Dylan, at 50C in pi 5.0 acetate buffer. The sugar released is determined as a maltose equivalent by adding alkaline 3,5-dinitrosalicylic acid reagent, heating for 5 minutes on a boiling water bath, quenching in ice water, measuring the absorption of the solution at 540nm and converting this to a maltose equivalent by reference to a standard calibration graph obtained by preparing standard dilutions of maltose of known moisture content and reacting these with the donator-salicylic reagent under the conditions lust described.
As used herein, one unit of enzyme releases 1 my of maltose equivalent per minute under the test conditions at 50C and pi 5Ø
The enzyme according to the invention is useful for a variety of purposes for which other pentosanases are used. Thus, for example, it may be used in baking, to reduce the natural pentosan content of wheat flour and so improve the keeping qualities of bread. It may be used in starch manufacture and hydrolysis, to lower the pentosan content of cereals and reduce the viscosity of starch slurries which otherwise adversely affect the efficiency and cost of starch recovery and subsequent hydrolysis It may be used in farming, to upgrade the quality of mixed silage and animal feeds. It may be used in brewing, for the improved production and extraction of fermentable sugars when the mash includes e.g.
wheat or sorghum, and for the prevention or treatment of certain types of haze. It may be used for the extraction of vegetable tissue, for example in the extraction of tea, coffee and fruits; and to extract alginates from seaweed; and in the manufacture of natural vegetable coloring materials. In some of these applications, the thermostability of the enzyme is particularly advantageous in view of the temperatures at which the processes are conducted.
In a further aspect of the invention, therefore, we provide a method of reducing the pentosan content of a pentosan-containing material which comprises contacting the said material with an enzyme of the invention.
Typical pentosans which may be degraded with the enzyme of the invention include those found in cereals such as wheat and oats; plants such as tea and coffee and in extracts thereof; fruits;
vegetables; seaweed and sorghum. In one example, the pentosan may be Dylan, for example an oat hull Dylan. In a preferred embodiment, the pentosan-containing material which is to be degraded is derived from wheat.
In a further embodiment of the invention we provide a method of reducing the Dylan content of a xylan-containing material wherein the material is contacted with an enzyme according to the invention.
The enzyme or composition according to the 33~
invention may be used employing methods customarily found in enzyme technology. Thus for example the enzyme may be contacted with an aqueous medium containing the substrate either in suspension, admix or in a solution. The reaction temperature will vary according to the exact nature of the reaction but will in general be in the range 35-95C, advantageously at the higher end of the range, in some applications at 90C and above The pi of the reaction mixture may be for example in the range 4.0-6.5, preferably 4.5-5.5 and in particular at pi 5Ø If desired, the reaction mixture may contain other added enzymes, for example aimless.
The strain of Toolers emersonii which we have used is a sub-culture of that which was deposited at the Commonwealth Mycological Institute, Knew, England under Number IMP 116815 in 1972 before the Budapest Treaty on the International Recognition of the Deposit of Microorganisms for the purposes of Patent Procedure (Budapest 1977) was signed.
We have recently redeposited this strain (on 1984) under slumber IMP 290604 at the same depository but under the conditions of the Treaty of Budapest and it is our belief that the two strains are identical and that either strain may be used.
The following Examples illustrate the invention.
All temperatures are in C. All percentages are in w/v.
I
E _ pie 1 Talaromyces emersonii IMP 116815 was cultured at 37 for 10 days on an ajar medium sterilized in an autoclave and containing 0.5% petunia, 0.4~
Nail, 0.75% glycerol, 0.8% molasses, 0.006% KH2PO4 and 0.005~ McCoy).
The spores produced were used to inoculate flasks of a liquid medium sterilized by autoclaving and containing 3.3% malt extract, 2.0% yeast extract and 0.6% ammonium dihydrogen phosphate. The flasks were placed on a rotary shaker (210 rev/min; 4.9 cm throw) for 3 days at 45.
The resulting vegetative culture (400 ml) was used to inoculate 40 liters of Medium A) Table 1 sterilized by steam injection in a 50 lithe capacity stainless steel fermenter. The culture was stirred at 420 rev/min and aerated at 50 litres/min for 75 hours at 50.
The resulting culture (4.5 L) was used to inoculate 40 liters of Medium A (Table 1) sterilized by steam injection in a 50 lithe capacity stainless steel fermenter. The culture was stirred at 420 rev/min and aerated at 50 litres/min for 75 hours at 50.
The resulting culture (4.5 L) was used to inoculate 40 liters of Medium A sterilized by steam injection in a 50 lithe capacity stainless steel fermenter. The culture was stirred at 420 rev/min and aerated at 50 litres/min for 36 hours at 50.
The resulting culture (16 L) was used to inoculate 32 liters of Medium B (Table 1) sterilized by steam injection in a 50 lithe capacity stainless steel fermenter.
The culture was aerated at 50 litres/min.
35 and stirred intermittently at 420 rev/min. at 50 for 10 days. Sterile water was added at an average rate of 1.5 liters per day.
Assay of the exocellular fluid yielded a concentration of the enzyme according to the invention Of 36 u/
Table 1 Ingredient Medium A (~) Medium B (~) Ground Barley 1.0 3.38 Distillers Solubles 2.25 5.06 Polka Floe 2025 2.53 ( H4)2 H2PO4 0.34 0 77 K2SO4 0.12 0.27 M9S04'7H20 0.01 0.11 Nail 0.11 0.11 MnSO4-4H2o .S 0.001 15 Phase 0.004 0.008 ZnSO4.7H2O 0.004 0.008 QUIZ 0 0005 0.001 POW 0.5 1.02 Water to 100 Example 2 Demonstration of variation in pentosanase: glucanase ratio on fermentation a) Spores were produced as in Example 1 and used to inoculate a seed stage in 250 ml flasks containing 40 ml of Medium A sterilized by autoclaving. The flasks were incubated at 45 for 72 hours, shaking at 200 rev/min.
The resulting culture (4 ml) was used to inoculate 40 ml of Medium B sterilized by autoclaving in 250 ml flasks. after incubating at 45 for 12 days, shaking at 200 rev/min, the exocellular culture fluid was assayed or pentosanase (P) and barley ~-glucanase (G) activities and the P : G ratio was calculated.
b) Using essentially the same system as in a) above.
I
Omitting the Polka Floe and including oat spells Dylan (2.2%) gave a P : G ratio 71%
higher than that obtained in a).
Example 3 In order to demonstrate pentosanase activity in the enzyme produced in Example 1, a 1% pentosan solution was incubated at 50 in buffer at pi 5.0 in the presence of added enzyme (test system) or with the addition of an equivalent amount of water (control system). The pentosan substrate used was Dylan, obtained from oat hulls.
Samples of the test system were withdrawn after 10 minutes, 30 minutes and 22.5 hours, quenched to prevent any further reaction and then spotted on to 20 cm square thin layer chromatography plates covered with 0.25 mm kieselgel. Spots of selected standard sugar solutions and of the control system were also applied.
The mobile phase was n-butanol:pyridine:ethanol:
water (20:15:25:10). Detection was by spraying the dried plates with 5% ammonium molybdate in 5% sulfuric acid followed by heating at 105 for 15 miss.
All the test samples showed inter aria a spot of identical Of value to that given by the standard sugar solution Zulus.
Since the control sample gave only a single spot on the origin, this test spot can not have derived either from Zulus contamination of the substrate or from its chemical hydrolysis: it must have arisen by enzymic degradation of the pentosan.
Example 4 The following comparative test was designed to illustrate the potential utility of the enzyme according to the invention in an enzymatic wheat ;26~35 starch digestion process:
Enzyme (2 ml) prepared according to Example 1, low grade wheat flour (155 g), sodium chlorite (2 9), calcium chloride (0.17 g), 'Termamyl' bacterial alpha aimless (Nova Industry A/S) (1 ml) and water (250 ml) were shaken thoroughly in a glass flask.
The pi was adjusted to 6.5 using caustic soda.
The neck of the container was covered to minimize evaporation and the flask was held for 5 hours at a temperature of 90. Starch hydrolysis occurred (negative iodine test result) and the divest viscosity was 43 cups.
In a control experiment omitting the enzyme of the invention the final viscosity of the digest was 127 cups.
The following Examples illustrate experiments performed to characterize the enzyme according to the invention In each Example, the enzyme used was prepared according to the method of Example 1 except that small amounts of sodium bonniest and sodium met:abisulphite were added to the exocellular fluid as bacteriological stabilizers. Enzyme activity was determined in each Example using an excess of 1% aqueous oat hull. Dylan as the pentosan substrate and measuring the increase in reducing activity after a 10 mix incubation, against a Zulus calibration curve. The pi and temperature of each incubation are stated in the Examples.
-Example 5 The pH-activity relationship was obtained at a temperature of 50 pi 4.0 4.5 5.0 5.5 6.0 6.5 .
% Maximum Activity 62 85 100 84 70 47 _ _ __ I_._ _ _ _ _ _ _ ._ _ _ _ ._ _ _ , _ _. _ _ _ _ _ ___ _ __ __ _ ago Pry' I
Significant hydrolysis occurs throughout the range illustrated.
Example 6 Thermal stability was studied by holding samples at temperatures of 60, 70, 80, 90 and 95 in the absence of substrate and withdrawing amounts at timed intervals to obtained a family of residual activity-time curves. The activity remaining was measured at pi 5.0 and 50:
- at 60, there was no detectable loss in activity after 80 miss, - at 70, 70~ of the initial activity was still present after 1 h, 15 - at 80, 70% of the initial activity was still present after 30 miss, - at 90, 50~ of the initial activity was still present after 8 miss, - at 95, 50% of the initial activity was still present after 6 miss.
Example 7 The temperature - activity relationship was obtained at a pi of 5Ø Inspection of the activity-temperature curve showed that peak activity occurred at 87+2. Activities at the individual temperatures studied, expressed as percentages of this maximum, were as follows:
% Maximum Activity 13 24 41 57 86 [100] 90 45 Temperature 40 50 60 70 80 [87+2] 90 95 The results confirm the inherent thermal stability of the new enzyme, as shown in example 5. The enzyme can clearly be used at temperatures in excess of 90.
~6~33~
This contrasts with a poorly defined optimum of 60-70 for the barley ~-glucanase of British Specification 1,421,127. At 80, only 40% of peak activity is recorded.
Example 8 In a preliminary study to determine whether activity of the enzymes was affected by products of the reaction and/or other sugars present in a typical digest in an industrial process, three simple sugars (Zulus, glucose and maltose) were separately added to the enzyme, which was then assayed at 50 and pi 5Ø Each sugar was added in an amount equivalent to the amount of Zulus liberated from the substrate under the assay conditions.
There was no inhibition or promotion of enzyme activity, and thus, on this evidence, there would be no interference with enzyme activity from the accumulation of simple sugars that will occur in many industrial applications.
Claims (13)
PROPERTY OR PRIVILEGE IS CLAIMED ARE DEFINED AS FOLLOWS:
1. An enzyme obtainable by fermentation from a strain of the species Talaromyces emersonii or a mutant thereof which is capable of catalysing the degradation of pentosans.
2. An enzyme as claimed in claim 1 which has a pH for optimum activity of about 5.0 measured at 50°C, and a temperature for optimum activity at 87?2°C measured at pH 5.0 and which retains about 50% of its initial activity after heating at 95°C for six minutes at pH 5.0, all measured using oat hull xylan as pentosan substrate.
3. An enzyme composition comprising an enzyme as claimed in claim 1 in a mixture with a .beta.-1,4/.beta.-1,3-glucanase and wherein the level of pentosanase activity has been increased relative to the level of .beta.-1,4/.beta.-1,3-glucanase activity by modification of the fermentation medium in which each is produced.
4. An enzyme or composition as claimed in claim 1, 2 or 3 wherein the strain employed is Talaromyces emersonii IMI 116815, IMI 290604, or a mutant thereof.
5. A process for the preparation of an enzyme composition having pentosanase activity which comprises fermenting a micro-organism strain of the species Talaromyces emersonii in a nutrient medium therefor whereby a broth containing said enzyme is produced.
6. A process as claimed in claim 5 wherein the level of pentosanase activity relative to the level of .beta.-1,4/.beta.-1,3-glucanase activity is increased by modification of the nutrient medium.
7. A process as claimed in claim 5 wherein the level of pentosanase activity relative to the level of .beta.-1,4-/.beta.-1,3-glucanase activity is increased by a purification step subsequent to the fermentation.
8. A process as claimed in claim 5, 6 or 7 wherein the strain is Talaromyces emersonii IMI 116815, IMI 290604, or a mutant thereof.
9. A method of reducing the pentosan content of a pentosan-containing material which comprises contacting the said material with an enzyme or composition as claimed in claim 1, 2 or 3.
10. A method of reducing the pentosan content of a pentosan-containing material wherein said pentosan-containing material is a cereal selected from wheat and oats, a plant selected from tea and coffee or an extract thereof, a fruit or a vegetable, which method comprises contacting the said material with an enzyme or compo-sition as claimed in claim 1, 2 or 3.
11. A method of reducing the pentosan content of starch which method comprises contacting the starch with an enzyme or compo-sition as claimed in claim 1, 2 or 3.
12. A method of reducing the pentosan content of wheat or a wheat-derived product which method comprises contacting the wheat or wheat-derived product with an enzyme or composition as claimed in claim 1, 2 or 3.
13. A method of reducing the pentosan content of a pentosan-containing material which comprises contacting said material with an enzyme or composition as claimed in claim 1, 2 or 3 wherein the enzyme or composition is contacted with the pentosan-containing material in an aqueous medium at a temperature of from 35-95°C and at a pH of from 4.0 to 6.5.
Applications Claiming Priority (4)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| GB838331719A GB8331719D0 (en) | 1983-11-28 | 1983-11-28 | Biochemical process |
| GB8331719 | 1983-11-28 | ||
| GB8405323 | 1984-02-29 | ||
| GB848405323A GB8405323D0 (en) | 1984-02-29 | 1984-02-29 | Biochemical process |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| CA1226835A true CA1226835A (en) | 1987-09-15 |
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| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| CA000468659A Expired CA1226835A (en) | 1983-11-28 | 1984-11-27 | Biochemical process and composition |
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| BE (1) | BE901138A (en) |
| CA (1) | CA1226835A (en) |
| DE (1) | DE3443204A1 (en) |
| DK (1) | DK560884A (en) |
| FR (1) | FR2555602B1 (en) |
| GB (1) | GB2150933B (en) |
| IT (1) | IT1178263B (en) |
| NL (1) | NL8403600A (en) |
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| CA1280704C (en) * | 1985-12-03 | 1991-02-26 | Paul Ducroo | Production of beer |
| FI93859C (en) * | 1985-12-03 | 1995-06-12 | Gist Brocades Nv | Process for the production of glucose syrups and purified starches from pentosans containing starches of wheat and other cereal plants |
| US5200215A (en) * | 1988-04-20 | 1993-04-06 | Nabisco, Inc. | Enzyme treated low moisture content comestible products |
| FI884668A (en) * | 1988-10-11 | 1990-04-12 | Suomen Sokeri Oy | FOERFARANDE FOER FOERBAETTRANDE AV FRAMSTAELLNINGSPROCESSEN HOS TORRA SAEDESPRODUKTER MED HJAELP AV ENZYMBEHANDLING. |
| US5176927A (en) * | 1988-10-11 | 1993-01-05 | Cultor Ltd. | Method of improving the production process of dry cereal products by enzyme addition |
| GB8906837D0 (en) * | 1989-03-23 | 1989-05-10 | Unilever Plc | Bread improvers |
| NL9001388A (en) * | 1990-06-19 | 1992-01-16 | Unilever Nv | RECOMBINANT DNA, CELL CONTAINING DERIVED DNA, ENZYME FOR WHICH THE RECOMBINANT CODES DNA AND USES THEREOF. |
| US5108764A (en) * | 1990-09-07 | 1992-04-28 | Nabisco Brands, Inc. | Production of crackers with reduced or no added fat |
| EP0915985A1 (en) * | 1996-08-05 | 1999-05-19 | Mogen International N.V. | Improved process for the production of alcoholic beverages using maltseed |
| IES20060090A2 (en) * | 2006-02-10 | 2007-06-13 | Nat Univ Ireland | Talaromyces emersonii enzyme systems |
| CN109699766A (en) * | 2017-10-25 | 2019-05-03 | 勐海茶业有限责任公司 | The method for preparing fermented tea, the fermented tea prepared with this method and its application |
| CN111534685B (en) * | 2020-05-27 | 2020-12-08 | 中国安全生产科学研究院 | Method for treating complex sulfide concentrate |
| EP4285728A1 (en) * | 2022-05-31 | 2023-12-06 | Kerry Group Services International Limited | Dough composition comprising non-starch polysaccharide degrading enzymes |
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| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US2821501A (en) * | 1953-12-08 | 1958-01-28 | Ca Nat Research Council | Recovery of starch |
| GB1216556A (en) * | 1967-04-03 | 1970-12-23 | Delmar Chem | Baking additive and method for producing baked goods |
| BE795716A (en) * | 1972-02-22 | 1973-08-21 | Glaxo Lab Ltd | THERMOSTABLE ENZYMATIC COMPOSITIONS |
-
1984
- 1984-11-27 BE BE0/214061A patent/BE901138A/en not_active IP Right Cessation
- 1984-11-27 IT IT49212/84A patent/IT1178263B/en active
- 1984-11-27 FR FR848418061A patent/FR2555602B1/en not_active Expired - Fee Related
- 1984-11-27 DE DE19843443204 patent/DE3443204A1/en not_active Withdrawn
- 1984-11-27 GB GB08429910A patent/GB2150933B/en not_active Expired
- 1984-11-27 DK DK560884A patent/DK560884A/en unknown
- 1984-11-27 NL NL8403600A patent/NL8403600A/en not_active Application Discontinuation
- 1984-11-27 CA CA000468659A patent/CA1226835A/en not_active Expired
Also Published As
| Publication number | Publication date |
|---|---|
| DE3443204A1 (en) | 1985-08-29 |
| NL8403600A (en) | 1985-06-17 |
| BE901138A (en) | 1985-05-28 |
| GB2150933A (en) | 1985-07-10 |
| IT1178263B (en) | 1987-09-09 |
| GB2150933B (en) | 1987-08-19 |
| IT8449212A0 (en) | 1984-11-27 |
| FR2555602A1 (en) | 1985-05-31 |
| GB8429910D0 (en) | 1985-01-03 |
| DK560884D0 (en) | 1984-11-27 |
| DK560884A (en) | 1985-05-29 |
| FR2555602B1 (en) | 1990-05-11 |
| IT8449212A1 (en) | 1986-05-27 |
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