DK146941B - GLUCOAMYLASE AND PROCEDURE FOR PREPARING A HIGH GLUCOSE CONTENT OF SYRUP BY SUCCARIFICATION OF MELTED STARCH - Google Patents
GLUCOAMYLASE AND PROCEDURE FOR PREPARING A HIGH GLUCOSE CONTENT OF SYRUP BY SUCCARIFICATION OF MELTED STARCH Download PDFInfo
- Publication number
- DK146941B DK146941B DK303379AA DK303379A DK146941B DK 146941 B DK146941 B DK 146941B DK 303379A A DK303379A A DK 303379AA DK 303379 A DK303379 A DK 303379A DK 146941 B DK146941 B DK 146941B
- Authority
- DK
- Denmark
- Prior art keywords
- enzyme
- glucoamylase
- starch
- glucoamylases
- strain
- Prior art date
Links
- 102100022624 Glucoamylase Human genes 0.000 title description 54
- 108010073178 Glucan 1,4-alpha-Glucosidase Proteins 0.000 title description 33
- 229920002472 Starch Polymers 0.000 title description 30
- 235000019698 starch Nutrition 0.000 title description 30
- 239000008107 starch Substances 0.000 title description 29
- WQZGKKKJIJFFOK-GASJEMHNSA-N Glucose Natural products OC[C@H]1OC(O)[C@H](O)[C@@H](O)[C@@H]1O WQZGKKKJIJFFOK-GASJEMHNSA-N 0.000 title description 25
- 238000000034 method Methods 0.000 title description 14
- 239000008103 glucose Substances 0.000 title description 11
- 239000006188 syrup Substances 0.000 title description 4
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- WQZGKKKJIJFFOK-VFUOTHLCSA-N beta-D-glucose Chemical compound OC[C@H]1O[C@@H](O)[C@H](O)[C@@H](O)[C@@H]1O WQZGKKKJIJFFOK-VFUOTHLCSA-N 0.000 description 24
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- 239000000243 solution Substances 0.000 description 19
- 239000002609 medium Substances 0.000 description 18
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- 230000000694 effects Effects 0.000 description 13
- 238000006243 chemical reaction Methods 0.000 description 12
- 239000000758 substrate Substances 0.000 description 12
- FAPWRFPIFSIZLT-UHFFFAOYSA-M Sodium chloride Chemical compound [Na+].[Cl-] FAPWRFPIFSIZLT-UHFFFAOYSA-M 0.000 description 10
- 239000007853 buffer solution Substances 0.000 description 10
- 235000002639 sodium chloride Nutrition 0.000 description 10
- 241000233866 Fungi Species 0.000 description 9
- CSNNHWWHGAXBCP-UHFFFAOYSA-L Magnesium sulfate Chemical compound [Mg+2].[O-][S+2]([O-])([O-])[O-] CSNNHWWHGAXBCP-UHFFFAOYSA-L 0.000 description 8
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- 230000007935 neutral effect Effects 0.000 description 8
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- 241000228212 Aspergillus Species 0.000 description 6
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- 241000228245 Aspergillus niger Species 0.000 description 4
- IJGRMHOSHXDMSA-UHFFFAOYSA-N Atomic nitrogen Chemical compound N#N IJGRMHOSHXDMSA-UHFFFAOYSA-N 0.000 description 4
- OKTJSMMVPCPJKN-UHFFFAOYSA-N Carbon Chemical compound [C] OKTJSMMVPCPJKN-UHFFFAOYSA-N 0.000 description 4
- 240000007594 Oryza sativa Species 0.000 description 4
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- WCUXLLCKKVVCTQ-UHFFFAOYSA-M Potassium chloride Chemical compound [Cl-].[K+] WCUXLLCKKVVCTQ-UHFFFAOYSA-M 0.000 description 4
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- 235000019341 magnesium sulphate Nutrition 0.000 description 4
- 239000000203 mixture Substances 0.000 description 4
- 235000009566 rice Nutrition 0.000 description 4
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- BFNBIHQBYMNNAN-UHFFFAOYSA-N ammonium sulfate Chemical compound N.N.OS(O)(=O)=O BFNBIHQBYMNNAN-UHFFFAOYSA-N 0.000 description 2
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- 238000010908 decantation Methods 0.000 description 2
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- 238000000502 dialysis Methods 0.000 description 2
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- CZMRCDWAGMRECN-UGDNZRGBSA-N Sucrose Chemical compound O[C@H]1[C@H](O)[C@@H](CO)O[C@@]1(CO)O[C@@H]1[C@H](O)[C@@H](O)[C@H](O)[C@@H](CO)O1 CZMRCDWAGMRECN-UGDNZRGBSA-N 0.000 description 1
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Classifications
-
- 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
- C12N9/2408—Glucanases acting on alpha -1,4-glucosidic bonds
- C12N9/2411—Amylases
- C12N9/2428—Glucan 1,4-alpha-glucosidase (3.2.1.3), i.e. glucoamylase
-
- 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
- C12P19/20—Preparation of compounds containing saccharide radicals produced by the action of an exo-1,4 alpha-glucosidase, e.g. dextrose
Description
i 146941in 146941
Opfindelsen angår en hidtil ukendt glucoamylase og en fremgangsmåde til fremstilling af en sirup med højt glucoseindhold ved saccharificering af smeltet stivelse til glucose.The invention relates to a novel glucoamylase and to a process for preparing a high glucose syrup by saccharifying molten starch to glucose.
5 Når der i dag skal fremstilles glucose industrielt ud fra stivelse, anvendes til saccharificeringsprocessen hovedsageligt glucoamylaser produceret af mikroorganismer tilhørende slægterne Rhizopus og Aspergillus. Betingelserne, hvorunder disse glucoamylaser anvendes, er pH 5,0 og 10 55 °C for enzymer fra Rhizopus-stammer og pH 4,5 og 60 °C for enzymer fra Aspergillus-stammer.5 In order to produce glucose industrially from starch today, the saccharification process is mainly used by glucoamylases produced by microorganisms belonging to the genera Rhizopus and Aspergillus. The conditions under which these glucoamylases are used are pH 5.0 and 55 ° C for Rhizopus strain enzymes and pH 4.5 and 60 ° C for Aspergillus strain enzymes.
Desuden er hydrolysatets maksimale glucoseindhold omkring 96% (på tørstofbasis), når disse glucoamylaser reagerer med enzymsmeltet stivelse i en koncentration på 30%. En 15 grund til, at glucoseudbyttet ikke når 100% er, at der dannes isomaltose på grund af en omvendt reaktion af disse glucoamylaser. Imidlertid er der for nylig offentliggjort en rapport (US patentskrift nr. 3 897 305) om, at den omvendte reaktion af glucoamylaser er yderst lille i nær-20 heden af det neutrale område, og at glucoseudbyttet således kan hæves til omkring 98% ved udførelse af reaktionen ved omkring neutral pH-værdi under samtidig anvendelse af pullulanase. Pullulanasen har den virkning at afgrene stivelsen og forøge hastigheden af gluco-25 amylasevirkningen under disse næsten neutrale betingelser. Hvad angår neutrale glucoamylaser, er der kun rapporteret én til dato, nemlig den glucoamylase, som produceres af den rissvidnings-forårsagende svamp CPiricularia oryzae; Kazuo Matsuda et al.; Amylase Symposium, Vol. 9, 30 1974), men denne glucoamylase har lav varmestabilitet og kan således ikke anvendes under industrielle betingelser.In addition, the maximum glucose content of the hydrolyzate is about 96% (on a dry matter basis) when these glucoamylases react with the enzyme-melted starch at a concentration of 30%. One reason why glucose yield does not reach 100% is that isomaltose is formed due to a reverse reaction of these glucoamylases. However, a recent report (U.S. Patent No. 3,897,305) has recently published that the reverse reaction of glucoamylases is extremely small in the vicinity of the neutral range and that glucose yield can thus be raised to about 98% when performed. of the reaction at about neutral pH while using pullulanase. The pullulanase has the effect of branching out the starch and increasing the rate of glucamylase action under these near-neutral conditions. With regard to neutral glucoamylases, only one has been reported to date, namely the glucoamylase produced by the waxy-causing fungus CPiricularia oryzae; Kazuo Matsuda et al .; Amylase Symposium, Vol. 9, 1974), but this glucoamylase has low heat stability and thus cannot be used under industrial conditions.
Opfindelsens formål er at tilvejebringe en glucoamylase, som er aktiv ved næsten neutral pH-værdi og har tilstrækkelig varmestabilitet til, at den kan anvendes under in- 2 146941 dustrielle reaktionsbetingelser, og som endvidere reagerer med stivelseshydrolysat til opnåelse af høje udbytter af glucose.The object of the invention is to provide a glucoamylase which is active at near neutral pH and has sufficient heat stability for use under industrial reaction conditions and which also reacts with starch hydrolyzate to obtain high yields of glucose.
Der er fundet en mikroorganismestamme, som producerer 5 en hidtil ukendt glucoamylase med optimal aktivitet ved en pH-værdi på 6,0 - 6,5 og god varmestabilitet.A microorganism strain has been found which produces a novel glucoamylase with optimum activity at a pH of 6.0 - 6.5 and good heat stability.
Denne glucoamylase er i stand til at omdanne en 30 vægt-% opløsning af en 10 D.E. (dextrose-ækvivalent) smeltet stivelse til et produkt indeholdende mindst ca. 96% glu-10 cose, når den omsættes med stivelseshydrolysatet ved pHThis glucoamylase is capable of converting a 30 wt% solution of a 10 D.E. (dextrose equivalent) molten starch to a product containing at least about 96% glucose when reacted with the starch hydrolyzate at pH
6,0 - 6,5 ved 55 °C.6.0 - 6.5 at 55 ° C.
I overensstemmelse hermed er glucoamylasen i-r følge opfindelsen ejendommelig ved, at den er identisk med den glucoamylase, der dannes ved dyrkning af stammen 15 Stachybotrys subsimplex, FRI 4377.Accordingly, the glucoamylase i-r of the invention is peculiar in that it is identical to the glucoamylase formed by the cultivation of strain 15 Stachybotrys subsimplex, FRI 4377.
Glucoamylasen ifølge opfindelsen kan således fremstilles ved, at mikroorganismestammen Stachybotrys subsimplex, FRI 4377 dyrkes i et næringsmedium, og at enzymet udvindes fra dyrkningsvæsken.Thus, the glucoamylase of the invention can be prepared by culturing the Stachybotrys sub-organism strain FRI 4377 in a nutrient medium and extracting the enzyme from the culture fluid.
På tegningen viser 20 fig. 1 sammenhængen mellem pH-værdien og enzymaktiviteten for enzymet ifølge opfindelsen og de konventionelle glucoamylaser produceret af mikroorganismerne Rhizopus niveus og Aspergillus niger; fig. 2 sammenhængen mellem temperaturen og enzymaktivi-25 teten for enzymet ifølge opfindelsen og glucoamylasen fra Piricularia oryzae; fig. 3 inaktiveringskurverne for enzymet ifølge opfindelsen, når det behandles ved forskellige pH-niveauer; 3 146941 fig. 4 en sammenligning af enzymet ifølge opfindelsen og de konventionelle glucoamylaser produceret af mikroorganismerne R. niveus, A. niger og P. oryzae, med hensyn til deres relative varmestabi1iteter.In the drawing, FIG. 1 shows the relationship between the pH value and the enzyme activity of the enzyme of the invention and the conventional glucoamylases produced by the microorganisms Rhizopus niveus and Aspergillus niger; FIG. 2 shows the relationship between the temperature and the enzyme activity of the enzyme of the invention and the glucoamylase from Piricularia oryzae; FIG. 3 the inactivation curves of the enzyme of the invention when treated at various pH levels; FIG. 4 is a comparison of the enzyme of the invention and the conventional glucoamylases produced by the microorganisms R. niveus, A. niger and P. oryzae, with respect to their relative heat stability.
5 I det følgende anføres egenskaberne af den hidtil ukendte neutrale glucoamylase ifølge opfindelsen i detaljer, og dens egenskaber stilles op imod de hidtil kendte gluco-amylasers.In the following, the properties of the novel neutral glucoamylase according to the invention are set out in detail and its properties are compared with those of the known glucoamylases.
Betegnelsen "D.E." er en forkortelse for "dextrose ækvi-10 valent", og anvendes til at betegne et materiales indhold af reducerende sukker,beregnet som D-glucose og udtrykt som procent af det totale tørstof.The term "D.E." is an abbreviation for "dextrose equivalent", and is used to denote a material's content of reducing sugar, calculated as D-glucose and expressed as a percentage of the total dry matter.
Betegnelsen "stivelsehydrolysat" anvendes alment til at betegne sirup eller et tørt produkt, som er fremstillet 15 ved delvis hydrolyse af stivelse. Et sådant produkt kan fremstilles ved sur eller enzymatisk hydrolyse.The term "starch hydrolyzate" is generally used to denote syrup or a dry product made by partial hydrolysis of starch. Such a product can be prepared by acidic or enzymatic hydrolysis.
Betegnelsen "smeltet stivelse" anvendes til at betegne et stivelsehydrolysat med lavt D.E. (D.E. fra omkring 2 til omkring 20).The term "molten starch" is used to denote a low starch hydrolyzate. (D.E. from about 2 to about 20).
20 1. Aktivitet og substrat-specifitet20 1. Activity and substrate specificity
Enzymet ifølge opfindelsen er i stand til at hydrolysere sådanne carbonhydratforbindelser som stivelse, opløselig stivelse, amylose, amylopectin og glycogen, og at danne dextrose derudfra. Udbyttet af dextrose fra hvert af 25 disse substrater er 100%, når substratkoncentrationen er 1%. Mutarotationen af den producerede dextrose er positiv.The enzyme of the invention is capable of hydrolyzing such carbohydrate compounds as starch, soluble starch, amylose, amylopectin and glycogen, and to generate dextrose therefrom. The yield of dextrose from each of these 25 substrates is 100% when the substrate concentration is 1%. The mutarotation of the dextrose produced is positive.
Dette enzym er således en glucoamylase. Enzymets reaktionshastighed blev sammenlignet med de hastigheder, som udvises af de glucoamylaser, som produceres af mikroorga-30 nismer tilhørende Rhizopus og Aspergillus i forbindelse med forskellige substrater. Resultaterne er anført i ta- 4 146941 bel I. Som det ses af denne tabel, er aktiviteten af enzymet ifølge opfindelsen mærkbart højere end aktiviteterne af de andre to glucoamylaser, især i forbindelse med hydrolysen af pullulan.Thus, this enzyme is a glucoamylase. The reaction rate of the enzyme was compared with the rates exhibited by the glucoamylases produced by Rhizopus and Aspergillus microorganisms in association with various substrates. The results are set out in Table I. As can be seen from this table, the activity of the enzyme of the invention is noticeably higher than the activities of the other two glucoamylases, especially in the hydrolysis of pullulan.
5 TABEL ITABLE I
Substrat-specifitet a ) _Reaktionshastighed_Substrate Specificity a) Reaction Rate_
Enzym Asperaillus niger RhizopusEnzyme Asperaillus niger Rhizopus
Substrat ifølqe , , b) niveus opf. Slug*n^lase,,, ^5imylase1 10 Dextrin (D.E. 10) 100 100 100Substrate According to,, b) Level Up. Slug * n ^ lase ,,, ^ 5imylase1 Dextrin (D.E. 10) 100 100 100
Amylopectin 104 113 91Amylopectin 104 113 91
Opløselig stivelse 122 95 112Soluble starch 122 95 112
Pullulan 9 2 2Pullulan 9 2 2
Glycogen 102 100 91 15 Maltotriose 6 12 8Glycogen 102 100 91 15 Maltotriose 6 12 8
Maltohexose 91 100 146Maltohexose 91 100 146
Panose 44 47 48 .Maltose 14 26 19 a) de enzymatiske aktiviteter af hver glucoamylase blev 20 bestemt med substraterne tilstede i en koncentration på 1%; hvert enzyms aktivitet i forbindelse med dextrin blev tildelt værdien 100, og aktiviteterne på de andre substrater angives som relative værdier.Panose 44 47 48 .Maltose 14 26 19 a) the enzymatic activities of each glucoamylase were determined with the substrates present at a concentration of 1%; each enzyme's activity in relation to dextrin was assigned the value 100, and the activities on the other substrates are given as relative values.
b) forhandlet af Enzyme Development Corporation, 2 Penn 25 Plaza, New York, N.Y.b) Negotiated by Enzyme Development Corporation, 2 Penn 25 Plaza, New York, N.Y.
"Sumyzyme" forhandlet af Sumitomo Shoji Kaisha, Ltd., 1, Kanda Mitoshiro-Cho, Chiyoda-ku, Tokyo, Japan."Sumyzyme" negotiated by Sumitomo Shoji Kaisha, Ltd., 1, Kanda Mitoshiro-Cho, Chiyoda-ku, Tokyo, Japan.
5 146941 2. pH-optimum og stabilt pH-område5 146941 2. pH optimum and stable pH range
Afhængigheden mellem den enzymatiske aktivitet (relativ værdi) af enzymet ifølge opfindelsen og reaktionens pH blev undersøgt og derpå sammenlignet med de tilsvarende 5 afhængigheder for de konventionelle kendte glucoamylaser produceret af Rhizopus- og Aspergillus-mikroorganismerne. Resultaterne er anført i fig. 1. Som vist i figuren er pH-optimet for dette enzym ved 60° C 6,0 - 6,5, hvilket er betydeligt højere end pH-optimet for de andre enzymer.The dependence between the enzymatic activity (relative value) of the enzyme of the invention and the pH of the reaction was investigated and then compared with the corresponding 5 dependencies for the conventional known glucoamylases produced by the Rhizopus and Aspergillus microorganisms. The results are shown in FIG. 1. As shown in the figure, the pH optimum for this enzyme at 60 ° C is 6.0 - 6.5, which is significantly higher than the pH optimum for the other enzymes.
10 Desuden viser dette enzym sin bedste stabilitet i nærheden af pH 6,0, men der ses ingen inaktivering af denne glucoamylase over pH-område 4-11, selv når den efterlades på substratet i 24 timer ved stuetemperatur.Furthermore, this enzyme shows its best stability in the vicinity of pH 6.0, but no inactivation of this glucoamylase over pH range 4-11 is seen, even when left on the substrate for 24 hours at room temperature.
3. Styrkebestemmelse 15 En 0,5 ml aliquot af en passende fortyndet enzymopløsning sattes til 0,5 ml af en 2% opløsning af en sprøjtetørret maltodextrin (D. E. ca. 10) i 0,1 M acetat pufferopløsning (pH 6,0), og blandingen blev inkuberet ved 60° C i præcis 10 minutter. Enzymreaktionen blev derpå standset ved 20 opvarmning af blandingen i 5 minutter i et kogende vandbad. Den producerede mængde dektrose blev bestemt ved glucoseoxidasemetoden. Den mængde enzym, som producerede et mikromol dextrose pr. minut blev defineret som l enhed.3. Strength Assay 15 A 0.5 ml aliquot of a suitably diluted enzyme solution was added to 0.5 ml of a 2% solution of a spray-dried maltodextrin (DE about 10) in 0.1 M acetate buffer solution (pH 6.0), and the mixture was incubated at 60 ° C for exactly 10 minutes. The enzyme reaction was then quenched by heating the mixture for 5 minutes in a boiling water bath. The amount of dextrose produced was determined by the glucose oxidase method. The amount of enzyme that produced one micromole of dextrose per minute was defined as 1 unit.
25 4. Temperaturområde for optimal reaktion25 4. Temperature range for optimal reaction
Temperaturvirkningen på den relative enzymatiske aktivitet af enzymet ifølge opfindelsen ved pH 6,0 blev sammenlignet med den relative aktivitet for den kendte glucoamylase fra rissvidningssvampen, Piricularia oryzae. Denne sammenligning er vist i fig. 2. Det fremgår klart, at den op- 30 timale temperatur for reaktionen af enzymet ifølge opfindelsen under disse betingelser er 65° C, ca. 10° C højere 6 146941 end den optimale temperatur for enzymet fra Piricularia oryzae, 5. Inaktivering på grund af pH- og temperaturbetingelserThe temperature effect on the relative enzymatic activity of the enzyme of the invention at pH 6.0 was compared with the relative activity of the known glucoamylase from the rice welding fungus, Piricularia oryzae. This comparison is shown in FIG. 2. It is clear that, under these conditions, the optimum temperature for the reaction of the enzyme of the invention is 65 ° C, ca. 10 ° C higher 6 146941 than the optimal temperature for the enzyme from Piricularia oryzae, 5. Inactivation due to pH and temperature conditions
Fig. 3 viser inaktiveringskurver for den relative enzyma-5 tiske aktivitet af enzymet ifølge opfindelsen, når det blev behandlet i 60 minutter ved 60° C og over et pH-område på 3- 8. Som det ses af figuren er dette enzym mest stabilt ved pH 6, og det inaktiveres fuldstændigt ved denne behandling i 30 minutter ved pH 3 og i 1 time ved pH 10 4. Desuden viser fig. 4 en sammenligning af varmestabili teten af enzymet ifølge opfindelsen og glucoamylaseme fra Rhizopus-, Aspergillus- og Piricularia-mikroorganismer-ne. Fig. 4 giver inaktiveringskurver for disse enzymer, når de blev behandlet ved 60° C, medens de holdtes ved 15 deres respektive pH-optima for stabilitet. Det kan ses, at varmestabiliteten af enzymet ifølge opfindelsen er dårligere end varmestabiliteten af glucoamylasen fra Aspergillus, men er bedre end varmestabiliteten af glucoamylaseme fra Rhizopus- og Piricularia-mikroorganismeme.FIG. 3 shows inactivation curves for the relative enzymatic activity of the enzyme of the invention when treated for 60 minutes at 60 ° C and over a pH range of 3- 8. As seen in the figure, this enzyme is most stable at pH 6, and it is completely inactivated by this treatment for 30 minutes at pH 3 and for 1 hour at pH 10 4. In addition, FIG. 4 is a comparison of the heat stability of the enzyme of the invention and the glucoamylases of the Rhizopus, Aspergillus and Piricularia microorganisms. FIG. 4 provides inactivation curves for these enzymes when treated at 60 ° C while maintained at their respective pH optima for stability. It can be seen that the heat stability of the enzyme of the invention is inferior to the heat stability of the glucoamylase from Aspergillus, but is better than the heat stability of the glucoamylases of Rhizopus and Piricularia microorganisms.
20 6. Inhibering, aktivering og stabilisering20 6. Inhibition, Activation and Stabilization
Enzymet ifølge opfindelsen kræver ingen specielle aktiverings- eller stabiliseringsmidler. Men, som det er tilfældet for de fleste andre glucoamylaser, inhiberes dette enzym af kviksølv(Il)-chlorid, kaliummanganat, jern(II)-25 chlorid, andre metalsalte og "tris".The enzyme of the invention requires no special activating or stabilizing agents. However, as is the case for most other glucoamylases, this enzyme is inhibited by mercury (II) chloride, potassium manganate, iron (II) -25 chloride, other metal salts and "tris".
7. Rensningsprocedure7. Purification procedure
Enzymet ifølge opfindelsen kan renses ved hjælp af en kombination af enhver af de almene rensningsmetoder, såsom ammoniumsulfatffraktionering, organisk-opløsningsmiddel-30 fraktionering, stivelseadsorption og forskellige chroma-tografier. Et belysende eksempel på en sådan rensningsprocedure er anført nedenfor.The enzyme of the invention can be purified by a combination of any of the general purification methods such as ammonium sulfate fractionation, organic solvent fractionation, starch adsorption and various chromatography. An illustrative example of such a cleaning procedure is given below.
7 1469417 146941
Cellerne og andet uopløseligt materiale fjernes fra dyrkningsmaterialet, og dyrkningsvsesken fryses natten over ved -20° C. Den smeltes derpå ved stuetemperatur, og det uopløselige materiale fjernes ved centrifugering. Derefter 5 tilsættes 2 volumener koldt isopropanol, og blandingen får lov at stå en nat over ved 4 °c. Enzymbundfaldet befries for overvæsken ved dekantering. Bundfaldet opløses derpå i en 0,05 M tris/HCl-puf fer opløsning (pH 7,5) indeholdende I.jdM EDTA, og det opløste materiale dialyseres derefter 10 en nat over ved 4° C over den samme puffer. Derpå sættes DEAE-cellulose, som er blevet ækvilibreret med den samme pufferopløsning til denne dialyserede enzymopløsning, således at enzymet adsorberes dertil. Efter vaskning af denne DEAE-cellulose med den samme puffer elueres 15 enzymet fra harpiksen med et præparat af den samme puffer indeholdende 0,3 NaCl. Enzymet udfældes derpå ved tilsætning af 2 volumener koldt isopropanol til eluatet, og det udfældede materiale udvindes ved centrifugering.The cells and other insoluble material are removed from the culture material and the culture liquid is frozen overnight at -20 ° C. It is then melted at room temperature and the insoluble material is removed by centrifugation. Then 2 volumes of cold isopropanol are added and the mixture is allowed to stand overnight at 4 ° C. The enzyme precipitate is freed from the supernatant by decantation. The precipitate is then dissolved in a 0.05 M tris / HCl buffer solution (pH 7.5) containing I.jdM EDTA, and the dissolved material is then dialyzed overnight at 4 ° C over the same buffer. Then DEAE cellulose which has been equilibrated with the same buffer solution is added to this dialyzed enzyme solution so that the enzyme is adsorbed thereto. After washing this DEAE cellulose with the same buffer, the enzyme is eluted from the resin with a preparation of the same buffer containing 0.3 NaCl. The enzyme is then precipitated by adding 2 volumes of cold isopropanol to the eluate and the precipitated material is recovered by centrifugation.
Bundfaldet opløses i 0,05 M tris/HCl-pufferopløsningen 20 (pH 7,5) indeholdende 1 mM EDTA efterfulgt af dialyse natten over overfor den samme puffer. Den dialyserede enzymopløsning sættes derefter på en DEAE-cellulose-søjle, som er blevet ækvilibreret med den samme 0,05 M tris/HCl-puffer (pH 7,5) indeholdende 1 mM edta. Enzymet elueres 25 fra denne søjle ved hjælp af en lineær koncentrationsgradient af den samme puffer indeholdende NaCl op til 0,5 M.The precipitate is dissolved in the 0.05 M tris / HCl buffer solution 20 (pH 7.5) containing 1 mM EDTA followed by overnight dialysis against the same buffer. The dialyzed enzyme solution is then loaded onto a DEAE cellulose column which has been equilibrated with the same 0.05 M tris / HCl buffer (pH 7.5) containing 1 mM edta. The enzyme is eluted from this column by a linear concentration gradient of the same buffer containing NaCl up to 0.5 M.
De eluerede fraktioner, som indeholder enzymet, hældes sammen, og enzymet koncentreres ved hjælp af isopropanol-udfældningsteknikken. Dette koncentrerede enzym sættes 30 derefter på en søjle af tværbunden dextrangel "Sephadej^ G-150", som er blevet ækvilibreret med en 0,05 M tris/HCl-puf fer (pH 7,0) indeholdende 1 mM EDTA, og elueringen udføres med den samme pufferopløsning. Efter denne procedure viste det rensede enzym et enkelt bånd ved .skiveelektroforese.The eluted fractions containing the enzyme are pooled and the enzyme is concentrated by the isopropanol precipitation technique. This concentrated enzyme is then loaded onto a column of cross-linked dextrangel "Sephadej G-150" which has been equilibrated with a 0.05 M tris / HCl buffer (pH 7.0) containing 1 mM EDTA and the elution is performed with the same buffer solution. Following this procedure, the purified enzyme showed a single band by disk electrophoresis.
35 8. Molekylvægt8. Molecular Weight
Molekylvægten af enzymet ifølge opfindelsen blev under- 8 146941 søgt ved anvendelse af en "Sephadex (¾ -150"-søjle i overensstemmelse med den procedure, som er beskrevet af Dunker/ A.K. and Rueckert, R.R. J. Biol. Chem. 244, 5074 (1969). Resultaterne viste, at dette enzyms molekylvægt 5 er omkring 50 000.The molecular weight of the enzyme of the invention was tested using a "Sephadex (¾ -150") column in accordance with the procedure described by Dunker / AK and Rueckert, RRJ Biol. Chem. 244, 5074 (1969 The results showed that the molecular weight of this enzyme 5 is about 50,000.
I det følgende forklares forskellene mellem enzymet ifølge opfindelsen og de konventionelt kendte glucoamylaser og grundene til, at dette enzym må anses for et hidtil ukendt enzym med sit pH-optimum i nærheden af neutralitet.The following explains the differences between the enzyme of the invention and the conventionally known glucoamylases and the reasons why this enzyme must be considered a novel enzyme with its pH optimum near neutrality.
10 Det ses af de i fig. 1 og tabel II anførte data, at de eneste glucoamylaser, som har deres pH-optima nær ved den neutrale zone, er enzymet ifølge opfindelsen og den gluco-amylase, som produceres af rissvidnings-mikroorganismen, Piricularia oryzae. Imidlertid fremgår det af fig. 2 og ta-15 bel II, at enzymet ifølge opfindelsen og rissvidnings- glucoamylasen har yderst forskellige optimale reaktionstemperaturer. Desuden viser de i fig. 4 angivne kurver, at varmestabiliteten af enzymet ifølge opfindelsen er langt bedre end af rissvidnings-glucoamylasen. Endvidere 20 viser tabel II, at molekylvægten af enzymet ifølge opfindelsen er meget mindre end molekylvægten af de kendte glucoamylaser.10 It can be seen from the 1 and Table II, the data indicated that the only glucoamylases having their pH optima close to the neutral zone are the enzyme of the invention and the glucoamylase produced by the rice widening microorganism, Piricularia oryzae. However, as shown in FIG. 2 and Table II, that the enzyme of the invention and the rice widening glucoamylase have extremely different optimum reaction temperatures. In addition, they show in FIG. 4 shows that the heat stability of the enzyme according to the invention is far better than that of the rice welding glucoamylase. Furthermore, Table II shows that the molecular weight of the enzyme of the invention is much less than the molecular weight of the known glucoamylases.
TABEL IITABLE II
Sammenligning af forskellige glucoamylaser med hensyn til 25 . pH-optimum, optimumtemperatur og molekylvægt 9 146941 pH-optimum Temperatur- Molekylvægt3^Comparison of various glucoamylases with respect to 25. pH optimum, optimum temperature and molecular weight 9 146941 pH optimum temperature Molecular weight3
a) optimum °Ca) optimum ° C
Glucoamylase _ a)_ _Glucoamylase _ a) _ _
Enzym ifølge opfindelsen (Stachybotrys subsiirplex) 6,0-6,5* 65X 50 000*Enzyme of the Invention (Stachybotry's Subirplex) 6.0-6.5 * 65X 50,000 *
Rhizopus sp. ("Sumyzyme") 5,0X 60x 70 OOO*5^ 5 Aspergillus niger 4,5X 70x 97 000°^ j \Rhizopus sp. ("Sumyzyme") 5.0X 60x 70 000 * 5 ^ 5 Aspergillus niger 4.5X 70x 97 000 °
Endcmyces sp. 5,0 - 64 000 p)Endcmyces sp. 5.0 - 64,000 p)
Endomyces fibuligera 5,5 60Endomyces fibuligera 5.5 60
Trichoderma viride^ 5,0 60 75 000Trichoderma viride ^ 5.0 60 75 000
Cephalosporium 10 charticolag^ 5,4 60 69 000 U \Cephalosporium 10 charticolag ^ 5.4 60 69 000 U \
Piricularia oryzae ' 6,5 55 94 000 (rissvidnings-org.) a) Alle værdier undtagen dem, der mærket med en stjerne (x), er taget fra følgende referencer: 15 b) Hiromi et al.: Biochem. Biophys. Acta 302, (1973).Piricularia oryzae '6.5 55 94 000 (Scratch welding org.) A) All values except those marked with an asterisk (x) are taken from the following references: 15 b) Hiromi et al .: Biochem. Biophys. Acta 302, (1973).
c) J.H. Pazur et al.: J. Biol. Chem. 237, 1002 (1962).c) J.H. Pazur et al .: J. Biol. Chem. 237, 1002 (1962).
d) Hattori et al.: Agr. Biol. Chem. 25, 895 (1061).d) Hattori et al .: Agr. Biol. Chem. 25, 895 (1061).
e) Harada et al.: J. Ferment. Tech. 53_, 559 (1975).e) Harada et al .: J. Ferment. Tech. 53, 559 (1975).
f) Okada; J. Jap. Soc. Starch Sci. 21, 283 (1974).f) Okada; J. Jap. Soc. Starch Sci. 21, 283 (1974).
20 g) h. Urbanek et a.: Appl. Micro. 30, 163 (1975.20 g) h. Urbanek et al.: Appl. Micro. 30, 163 (1975).
h) Matsuda et al.: Amylase Symposium £, 105 (1974).h) Matsuda et al .: Amylase Symposium, 105 (1974).
På basis af de ovenstående data kan det konkluderes, at glucoamylasen ifølge opfindelsen er en ny neutral glucoamylase, som har været ukendt til dato.On the basis of the above data, it can be concluded that the glucoamylase of the invention is a new neutral glucoamylase which has been unknown to date.
25 Den følgende forklaring skal nærmere belyse fremgangs måden til fremstilling af enzymet ifølge opfindelsen.The following explanation is intended to illustrate in more detail the process of producing the enzyme of the invention.
Den glucoamylase-producerende mikroorganisme, stammen G. 30-1140, FRI 4377, blev isoleret fra jorden af opfinderne i denne sag. Identifikationen af denne stamme skal 30 først angives. Stammens morphologiske egenskaber blev be stemt i overensstemmelse med de metoder, der er beskrevet af de nedenfor anførte forskere: ίο 146941The glucoamylase-producing microorganism, strain G. 30-1140, FRI 4377, was isolated from the soil by the inventors in this case. The identification of this strain must first be indicated. The morphological characteristics of the strain were determined according to the methods described by the researchers listed below: ίο 146941
Glimen, J. C. A MANUAL OF SOIL FUNGI. The Iowa State Uni-versity Press, Ames. 1971.Glimen, J. C. A MANUAL OF SOIL FUNGI. The Iowa State Uni- versity Press, Ames. 1,971th
Clements, F. E. and Shear, C. L. THE GENERA OF FUNGI.Clements, F. E. and Shear, C. L. THE GENERA OF FUNGI.
Haf ner, New York. 1964.Down, New York. 1964th
5 Barnett, H. L. ILLUSTRATED GENERA OF IMPERFECT FUNGI.5 Barnett, H. L. ILLUSTRATED GENERA OF IMPERFECT FUNGI.
2nd ed. Burgess, Minneapolis. 1968.2nd ed. Burgess, Minneapolis. 1968th
Bisby, G. R. Trans. Br. Myco. Soc. 26, 133-43 (1943).Bisby, G. R. Trans. Br. Myco. Soc. 26, 133-43 (1943).
Ainsworth, G. C. DICTIONARY OF THE FUNGI. 6th ed. Common-wealth Mycological Institute, Kew, Surrey. 1971.Ainsworth, G. C. DICTIONARY OF THE FUNGI. 6th ed. Common-wealth Mycological Institute, Kew, Surrey. 1,971th
10 9. Morphologiske egenskaber af stammen G30-114010 9. Morphological properties of strain G30-1140
Stammen blev dyrket på 5 slags medier i Petri-skåle. De følgende afsnit angiver de morphologiske egenskaber, som blev iagttaget for isolerede kolonier.The strain was grown on 5 kinds of media in Petri bowls. The following sections indicate the morphological characteristics observed for isolated colonies.
a) Czapek-agar-medium 15 Efter inkubation ved 30° C i ti dage er kolonierne tynde og runde med en diameter på 4-5 cm. De vegetative hypher er glasklare og viser ringe vækst med sorte conidieklyn-ger spredt som pulver over koloniernes overflade. Koloniernes undersider er brune, og et lysebrunt pigment udskil-20 les til mediet.a) Czapek agar medium 15 After incubation at 30 ° C for ten days, the colonies are thin and round with a diameter of 4-5 cm. The vegetative hyphae are clear and show little growth with black conidia clusters scattered like powder over the colonies. The undersides of the colonies are brown and a light brown pigment is excreted to the medium.
De vegetative hypher består af forgrenede fibre, som sjældent har nogle septa; conidiestrukturen er ensartet understøttet af fibrene. Conidiophorerne, som har septa, rager frem fra denne i rette vinkler. Conidiophorernes længde 25 er sædvanligvis 40-60 ^um, men somme tider når de mere end 100 ^um. Diameteren af disse er fra omkring 3 til omkring 6 yum, og selv om der er tilfælde, hvor deres grund- 11 146941 areal er glat, er det meste af deres overflade vortet, dækket med fine granulære fremspring. Disse conidiophorer er glasklare og de fleste er ikke forgrenet.The vegetative hyphae consist of branched fibers, which rarely have some septa; the conidia structure is uniformly supported by the fibers. The conidiophores, which have septa, protrude from this at right angles. The length 25 of the conidiophores is usually 40-60 µm, but sometimes reaches more than 100 µm. The diameter of these is from about 3 to about 6 µm, and although there are cases where their basic area is smooth, most of their surface is wart covered with fine granular projections. These conidiophores are glass clear and most are not branched.
På spidsen af conidiophorerne danner glasklare phialider 5 snoninger på 3-8 enheder. Phialidernes form er ægformet el ler kolbe-lignende; de er 8-15 /um lange og har en diameter på 2-6 /um; deres overflade er glat. Conidierne dannes ved spidsen af phialideme og er ovale 3-5 /um x 5-10 yum og har en glat overflade. Disse er glasklare ved tids-10 punktet for deres dannelse, men bliver sortgrønne, efter hånden som de modner.At the tip of the conidiophores, clear glass phialids form 5 twists of 3-8 units. The shape of the phialides is egg-shaped or flask-like; they are 8-15 µm long and have a diameter of 2-6 µm; their surface is smooth. The conidia form at the tip of the phialides and are oval 3-5 µm x 5-10 yum and have a smooth surface. These are crystal clear at the time-10 point of their formation but become black-green as they mature.
Conidiernes overflade er dækket med en stor mængde viskøst materiale. Af denne grund klæber conidierne sammen og danner store conidieklynger ved spidsen af conidiopho-15 rerne. Det viskøse materiale er transparent på dannelses tidspunktet, men bliver derefter gradvis sort.The surface of the conidia is covered with a large amount of viscous material. For this reason, the conidia cleave together and form large conidia clusters at the tip of the conidiophores. The viscous material is transparent at the time of formation but then gradually becomes black.
b) Modificeret Czapek-agar-mediumb) Modified Czapek agar medium
ProcentPercentage
Opløselig stivelse 1,0Soluble Starch 1.0
Majsstøbevæske (tørstof-basis) 0,1 20 NaNO^ 0,2 k2hpo4 0,1 KC1 0,05Maize casting liquid (dry matter basis) 0.1 NaNO ^ 0.2 k2hpo4 0.1 KCl 0.05
MgS04’7H20 0,05MgSO4'7H20 0.05
FeS04*7H20 0,001 25 Agar 2,0FeSO 4 * 7H 2 O 0.001 Agar 2.0
pH til 0,7 med NaOHpH to 0.7 with NaOH
Koloniernes vækst på dette medium er en smule langsommere end på det ovenfor beskrevne Czapek-medium, idet de når omkring 3 cm, når de inkuberes i 10 dage ved 30° C.The growth of the colonies on this medium is slightly slower than on the Czapek medium described above, reaching about 3 cm when incubated for 10 days at 30 ° C.
12 14694112 146941
Kolonierne er cirkulære og tynde, og deres overflader har strålende ud fra deres centre et sort viskøst materiale, som er i form af olielignende dråber med diametre, der når 1-3 mm. Disse stammer fra sammensmeltningen af 5 conidieklynger, som er indesluttet i det viskøse materiale og derved danner oliedråbelignende legemer. Koloniernes undersider viser en mørkere brun farve end det ses med det ovenstående Czapek-medium, og en lille mængde brunt pigment udskilles til mediet.The colonies are circular and thin, and their surfaces radiate from their centers a black viscous material which is in the form of oil-like drops with diameters reaching 1-3 mm. These arise from the fusion of 5 conidia clusters, which are enclosed in the viscous material, thereby forming oil droplet-like bodies. The undersides of the colonies show a darker brown color than seen with the above Czapek medium, and a small amount of brown pigment is excreted into the medium.
10 . c) Kartoffel-dextrose-agar-medium10. c) Potato dextrose agar medium
Koloniernes vækst på dette medium er en smule langsommere end på det ovenfor beskrevne Czapek-medium, idet den når 3-4 cm, når de inkuberes i 10 dage ved 30°C.The growth of the colonies on this medium is slightly slower than on the Czapek medium described above, reaching 3-4 cm when incubated for 10 days at 30 ° C.
Disse kolonier er også cirkulære, men de har en noget 15 større tykkelse end kolonierne på Czapek-mediet. Væksten af de vegetative celler er god, og den udvikler sig i et strålemønster. Koloniernes overflader er sorte med et svagt grønt skær og er rige på hypher, conidieklynger osv.These colonies are also circular, but they have a somewhat greater thickness than the colonies on the Czapek medium. The growth of the vegetative cells is good and it develops in a radiation pattern. The colonies' surfaces are black with a faint green tinge and are rich in hypher, conidia clusters, etc.
Efter 14 dages inkubation har de gamle koloniers over-20 flader udstrålende formationer af synnemata, der står omkring 1-3 mm opret. Disse koloniers undersider viser en sortbrun farve, og en stor mængde brunt pigment udskilles til mediet.After 14 days of incubation, the surfaces of the ancient colonies have radiating formations of synnemata standing about 1-3 mm upright. The undersides of these colonies show a blackish brown color and a large amount of brown pigment is excreted to the medium.
d) Special-agar-medium 25 Procentd) Special Agar Medium 25 Percent
Opløselig stivelse 1,0Soluble Starch 1.0
Majsstøbevæske (tørstof-basis) 0,2Corn molding liquid (dry matter basis) 0.2
Bomuldsfrøoliepresserester 0,1 Gærekstrakt 0,1 30 K2HP04 0,1Cotton seed oil residue 0.1 Yeast extract 0.1 K2HP04 0.1
MgS04*7H2D 0,05MgSO4 * 7H2D 0.05
Agar 2,0Agar 2.0
pH til 7,0 med NaOHpH to 7.0 with NaOH
146941 13146941 13
Kolonierne på dette medium har efter 10 dages inkubation ved 30°C diametre på 5-6 cm og er runde og tynde. De vegetative hypher viser god vækst og har et sort skær. Co-nidievæksten er dårligere end på de ovennævnte medier.The colonies of this medium, after 10 days of incubation at 30 ° C, have diameters of 5-6 cm and are round and thin. The vegetative hyphae show good growth and have a black tinge. Co-nidia growth is poorer than on the aforementioned media.
5 Koloniernes undersider er lysebrune, og et lysebrunt pig ment frigøres til mediet.5 The undersides of the colonies are light brown and a light brown pigment is released to the medium.
e) Påvis' gær-salt-agar-mediume) Detect yeast-salt-agar medium
Kolonierne på dette medium har efter 10 dages inkubation ved 30°C diametre på 2-3 cm og er mere ovale end runde 10 af form. Hypherne er lysebrune med et anstrøg af hvidt og danner noget tykke kolonier, som er fløjlsagtige. Koloniernes undersider er lysebrune, men der udskilles absolut intet pigment til mediet.The colonies of this medium, after 10 days of incubation at 30 ° C, have diameters of 2-3 cm and are more oval than round 10 of shape. The hyphae are light brown with a tinge of white and form somewhat thick colonies which are velvety. The undersides of the colonies are light brown, but no pigment is secreted into the medium.
10. Fysiologiske egenskaber af stamme G30-1140 15 a) Væksttemperatur10. Physiological properties of strain G30-1140 15 a) Growth temperature
Denne stamme er i stand til at vokse over et temperaturområde på 10-37°C, men dens optimale væksttemperatur er i nærheden af 30°C.This strain is capable of growing over a temperature range of 10-37 ° C, but its optimum growth temperature is near 30 ° C.
b) Vækst-pHb) Growth pH
20 Denne stamme er i stand til at vokse over et pH-område på 3 - 10, men dens optimale vækst-pH er i nærheden af pH 7.This strain is capable of growing over a pH range of 3 - 10, but its optimum growth pH is in the vicinity of pH 7.
c) Carbonkilderc) Carbon sources
Denne stamme er i stand til at udnytte sådanne carbonkil-25 der som dextrose, fructose, galactose, mannose, saccha rose, maltose og stivelse til at understøtte væksten.This strain is capable of utilizing such carbon sources as dextrose, fructose, galactose, mannose, saccha rose, maltose and starch to support growth.
14 146941 På basis af ovenstående mikrobiologiske konstateringer blev stamme 630-1140 identificeret som Gliobotrys albovirides efter opslag i genera of fungi og a manual of SOIL FUNGI. Imidlertid er denne organisme ifølge DICTI0__ 5 NARY OF FUNGI og G.R. Bisby (Trans. Br. Mycol. Soc. 26, 133-43 (1943) den samme som Stachybotrys subsimplex, og af denne grund blev stamme G30-1140 identificeret som Stachybotrys subsimplex.14 146941 Based on the above microbiological findings, strain 630-1140 was identified as Gliobotry's albovirides after posting in the genera of fungi and a manual of SOIL FUNGI. However, according to DICTI0__ 5 NARY OF FUNGI and G.R. Bisby (Trans. Br. Mycol. Soc. 26, 133-43 (1943) the same as Stachybotry's subsimplex, and for this reason strain G30-1140 was identified as Stachybotry's subsimplex).
Stamme G30-1140 har conidiophorer, som står opret fra dens 10 vegetative hypher, forgreninger eksisterer næsten ikke, og de har s.epta. Der er tilfælde, hvor basisdelen er glat, men spidsen er dækket med fremspring. Ved spidsen danner et niveau af phialider en spiral på 3-8 enheder. Conidier med glatte aflange overflader deler sig ud fra disse phia-15 lider, og de er indesluttet i et rigt viskøst stof. Disse egenskaber stemmer godt overens med dem, der er beskrevet for Stachybotrys subsimplex af G. R. Bisby (Trans.Strain G30-1140 has conidiophores that arise from its 10 vegetative hypers, branches hardly exist and they have s.epta. There are cases where the base is smooth but the tip is covered with protrusions. At the apex, a level of phialids forms a spiral of 3-8 units. Conidia with smooth oblong surfaces divide from these phia-15 sufferers and are enclosed in a rich viscous substance. These properties are in good agreement with those described for Stachybotry's subsimplex by G. R. Bisby (Trans.
Br. Mycol. Soc. 26, 133-43 (1943)).Br. Mycol. Soc. 26, 133-43 (1943)).
Denne Stachybotrys subsimplex stamme G30-1140 er deponeret 20 i The Fermentation Research Institute, Agency of IndustrialThis Stachybotry subsimplex strain G30-1140 is deposited 20 in The Fermentation Research Institute, Agency of Industrial
Science & Technology, Chiba City, Japan under nr. 4377.Science & Technology, Chiba City, Japan under No. 4377.
Med hensyn til dyrkningen afidenne mikroorganisme kan anvendes den almindelige viden og teknik inden for dyrkningen af svampe.With regard to the cultivation of this microorganism, the general knowledge and technique in the cultivation of fungi can be used.
25 Som næringsmedium er det muligt at anvende de medier, som bruges til dyrkningen af almindelige svampe. F. eks. kan der som carbonkilder anvendes forskellige stivelser, sti-velseshydrolysater, majsmel, hvedemel, melasse osv., medens nitrogenkravene kan opfyldes i form af pepton, bomulds-3Q frøolierester, kødekstrakt, gærekstrakt, casein, majs- støbevæske, maltekstrakt, sojabønnerester, skummetmælk, uorganiske ammoniumsalte, uorganiske nitrater osv. Som u- U6941 15 organiske salte er det muligt at anvende calciumchlorid, magnesiumsulfat, phosphater, natriumchlorid, kaliumchlo-rid osv. Endvidere kan disse carbonkilder, nitrogenkilder og uorganiske salte anvendes enten enkeltvis eller i pas-5 sende kombinationer. Desuden er det, hvis man ønsker at fremme mikroorganismens vækst og frembringe en forøgelse i dens enzymproduktion, muligt at anvende spormængder af metalsalte, vitaminer, aminosyrer osv.25 As a nutrient medium it is possible to use the media used for the cultivation of ordinary mushrooms. For example, various starches, starch hydrolysates, corn flour, wheat flour, molasses, etc. can be used as carbon sources, while the nitrogen requirements can be met in the form of peptone, cotton 3Q seed oil residues, meat extract, yeast extract, casein, corn dust liquid, malt extract, soybean residues, skimmed milk, inorganic ammonium salts, inorganic nitrates, etc. As in organic salts, it is possible to use calcium chloride, magnesium sulfate, phosphates, sodium chloride, potassium chloride, etc. Furthermore, these carbon sources, nitrogen sources and inorganic salts can be used either suitable combinations. In addition, if one wishes to promote the growth of the microorganism and produce an increase in its enzyme production, it is possible to use trace amounts of metal salts, vitamins, amino acids, etc.
De dyrkningsbetingelser, der sædvanligvis anvendes for 10 svampe, kan også anvendes ved dyrkningen af denne mikro organisme. Hvis mikroorganismen dyrkes i væskekultur i 7 -14 dage ved pH 5 - 8 og ved 20 - 37 "C og under omrøring til at give luftning, akkumuleres enzymet ifølge opfindelsen i dyrkningsvæsken. Hvis der anvendes faste materialer så-15 som klid, er det også muligt at udføre fast dyrkning.The cultivation conditions usually used for 10 fungi can also be used in the cultivation of this micro organism. If the microorganism is grown in liquid culture for 7-14 days at pH 5 - 8 and at 20 - 37 ° C and with stirring to give aeration, the enzyme of the invention accumulates in the culture liquid. If solid materials such as bran are used, it is also possible to perform solid cultivation.
I det følgende anføres et eksempel på en fremgangsmåde, hvorved den hidtil ukendte neutrale glucoamylase ifølge opfindelsen kan udvindes fra dyrkningsmaterialet. I tilfælde af væskekultur fjernes myceliet ved enhver af 2o de almindeligt kendte metoder. Derpå kan filtratet kon centreres under formindsket tryk, eller enzymet kan udsaltes sammen med de andre proteiner ved tilsætning af uorganiske salte, såsom ammoniumsulfat, til filtratet, eller enzymet kan udfældes og koncentreres ved tilsætning af et 25 organisk opløsningsmiddel, såsom acetone eller isopro- panol.The following is an example of a method by which the novel neutral glucoamylase of the invention can be recovered from the culture material. In the case of liquid culture, the mycelium is removed by any of the generally known methods. Then, the filtrate can be concentrated under reduced pressure, or the enzyme can be salted out with the other proteins by addition of inorganic salts, such as ammonium sulfate, to the filtrate, or the enzyme can be precipitated and concentrated by the addition of an organic solvent such as acetone or isopropanol. .
I tilfælde af en fast kultur ekstraheres enzymet først fra dyrkningsmaterialet ved anvendelse af vand eller en pufferopløsning. Derpå er det som ved væskekulturen mu-ligt at opnå enzymet i koncentreret form.In the case of a solid culture, the enzyme is first extracted from the culture material using water or a buffer solution. Then, as in the liquid culture, it is possible to obtain the enzyme in concentrated form.
De på denne måde opnåede rå præparater kan derpå renses ved udførelse af den førnævnte rensningsteknik.The crude compositions thus obtained can then be purified by carrying out the aforementioned purification technique.
16 14694116 146941
Det er muligt at anvende glucoamylasen ifølge opfindelsen til saccharificering af smeltet stivelse, når der skal produceres dextrose ud fra stivelse. Især sker der ved anvendelse af enzymet ifølge opfindelsen til saccha-5 rificering ved en pH-værdi på 6,0 - 6,5 som tidligere nævnt kun lidt omvendt reaktion, og dette resulterer i et forøget udbytte af dextrose i sammenligning med, hvad der er tilfældet ved anvendelse af de konventionelle glu-coamylaser og udførelse af saccharificeringen under sure 10 betingelser.It is possible to use the glucoamylase of the invention for the saccharification of molten starch to produce dextrose from starch. In particular, when using the enzyme of the invention for saccharification at a pH of 6.0 - 6.5, as previously mentioned, only a slight reverse reaction occurs, and this results in an increased yield of dextrose in comparison with what is is the case using the conventional glucoamylases and performing the saccharification under acidic conditions.
I overensstemmelse hermed er fremgangsmåden til fremstilling af en sirup med højt glucoseindhold ved saccharificering af smeltet stivelse til glucose ejendommelig ved, at den smeltede stivelse saccharificeres ved en pH-værdi 15 på 6,0 - 6,5 i nærvær af glucoamylasen ifølge opfindelsen.Accordingly, the process of preparing a high glucose syrup by saccharifying molten starch to glucose is peculiar in that the molten starch is saccharified at a pH of 6.0 - 6.5 in the presence of the glucoamylase of the invention.
Saccharificeringen udføres fortrinsvis ved en temperatur på fra omkring 50 til omkring 65 °C.The saccharification is preferably carried out at a temperature of from about 50 to about 65 ° C.
Opfindelsen belyses nærmere ved de følgende eksempler, hvori alle dele og procenter er beregnet på vægt, med 20 mindre andet er anført.The invention is further illustrated by the following examples, in which all parts and percentages are by weight, unless otherwise stated.
EKSEMPEL 1EXAMPLE 1
Et flydende dyrkningsmedium indeholdende 5% opløselig stivelse, 2% majsstøbevæske, 0,5% bomuldsfrøolierester, 0,5% gærekstrakt, 0,1% dikaliumphosphat, 0,05% magne-25 siumsulfat og 0,01% calciumchlorid blev indstillet til pH 7,0, og 100 ml af dette medium blev anbragt i en 500 ml Erlenmeyer-kolbe. Mediet blev steriliseret ved 121°. C i 10 minutter, podet med Stachybotrys subsimplex stamme G30-1140, FRI 4377, og inkuberet ved 30® C i 7 dage på 30 en ryster. Efter fuldførelse af dyrkningen blev myceliet fjernet fra dyrkningsvæsken ved filtrering. Filtratet fandtes at indeholde 70 enheder glucoamylase-aktivitet pr. ml.A liquid culture medium containing 5% soluble starch, 2% maize casting liquid, 0.5% cotton seed oil residue, 0.5% yeast extract, 0.1% dicalcium phosphate, 0.05% magnesium sulfate and 0.01% calcium chloride was adjusted to pH 7 , 0, and 100 ml of this medium were placed in a 500 ml Erlenmeyer flask. The medium was sterilized at 121 °. C for 10 minutes, seeded with Stachybotry's subsimplex strain G30-1140, FRI 4377, and incubated at 30 ° C for 7 days on 30 shakes. After completion of the culture, the mycelium was removed from the culture fluid by filtration. The filtrate was found to contain 70 units of glucoamylase activity per ml. ml.
17 14694117 146941
Dette filtrat blev frosset en nat igennem ved -20° C og derpå optøet ved stuetemperatur. Det uopløselige materiale blev fjernet ved centrifugering. Derpå sattes 2 volumener koldt isopropanol til denne opløsning,og den fik lov at 5 stå ved 4° C en nat igennem, således at enzymet blev udfældet. Overvæsken blev fjernet ved dekantering og bundfaldet opløst i en 0,05 M tris-HCl-puf feropløsning indeholdende 1 mM EDTA og med en pH-værdi på 7»5. Denne en-zymholdige opløsning blev derpå dialyseret overfor den 10 samme puffer ved 4° C en nat igennem. DEÅE-cellulose, som var blevet ækvilibreret med den samme pufferopløsning, sattes derefter til den dialyserede enzymopløsning, og enzymet blev adsorberet til denne bærer. Efter vaskning af DEAE-cellulosen med den samme puffer blev enzymet elueret 15 fra den under anvendelse af en opløsning af den samme puffer indeholdende NaCl i en koncentration på 0,3 M.This filtrate was frozen overnight at -20 ° C and then thawed at room temperature. The insoluble material was removed by centrifugation. Then 2 volumes of cold isopropanol were added to this solution and allowed to stand at 4 ° C for one night so that the enzyme precipitated. The supernatant was removed by decantation and the precipitate dissolved in a 0.05 M tris-HCl buffer solution containing 1 mM EDTA and with a pH of 7 »5. This enzyme-containing solution was then dialyzed against the same buffer at 4 ° C overnight. DEÅE cellulose which had been equilibrated with the same buffer solution was then added to the dialyzed enzyme solution and the enzyme was adsorbed to this carrier. After washing the DEAE cellulose with the same buffer, the enzyme was eluted from it using a solution of the same buffer containing NaCl at a concentration of 0.3 M.
Derefter sattes to volumener koldt isopropanol til eluatet for at udfælde enzymet, og bundfaldet blev opsamlet ved centrif ugering. Dette bundfald blev opløst i 0,05 M tris/HCl-20 pufferen (pH 7,5) indeholdende 1 mM EDTA, efterfulgt af dialyse en nat igennem overfor den samme pufferopløsning.Then, two volumes of cold isopropanol were added to the eluate to precipitate the enzyme and the precipitate was collected by centrifugation. This precipitate was dissolved in 0.05 M tris / HCl-20 buffer (pH 7.5) containing 1 mM EDTA, followed by overnight dialysis against the same buffer solution.
Den dialyserede enzymopløsning sattes på en søjle af DEAE-cellulose, som var blevet ækvilibreret med den samme 0,05 M tris/HCl-puffer (pH 7,5) indeholdende 1 mM EDTA.The dialyzed enzyme solution was loaded onto a column of DEAE cellulose which had been equilibrated with the same 0.05 M tris / HCl buffer (pH 7.5) containing 1 mM EDTA.
25 Eluering af enzymet fra denne søjle blev udført ved lineært at forøge koncentrationen af NaCl i den samme puffer-opløsning op til 0,5 M. De fraktioner af eluatet, som indeholdt enzymet blev derpå hældt sammen, og der tilsattes to volumener koldt isopropanol for at udfælde enzymet fra 30 denne opløsning og koncentrere det. Det koncentrerede enzym sattes derefter på en søjle af "Sephadex ™G-150", 18 146941 som var blevet ækvilibreret med en 0,05 M tris/HCl-pufferopløsning (pH 7,0) indeholdende 1 mM ΕΚΤΑ, og elueringen udførtes med den samme puffer. De eluerede fraktioner, som viste enzymaktivitet, blev derpå hældt sammen, og 5 der tilsattes to volumener koldt isopropanol for at udfælde enzymet. Dette resulterede i udvindingen af enzymet i renset og koncentreret form. Det rensede enzyms specifikke aktivitet fandtes at være 127 enheder pr. mg protein.Elution of the enzyme from this column was performed by linearly increasing the concentration of NaCl in the same buffer solution up to 0.5 M. The fractions of the eluate containing the enzyme were then pooled and two volumes of cold isopropanol were added to to precipitate the enzyme from this solution and concentrate it. The concentrated enzyme was then loaded onto a column of "Sephadex ™ G-150", which had been equilibrated with a 0.05 M tris / HCl buffer solution (pH 7.0) containing 1 mM ΕΚΤΑ, and eluted with the same buffer. The eluted fractions showing enzyme activity were then pooled and two volumes of cold isopropanol were added to precipitate the enzyme. This resulted in the recovery of the enzyme in purified and concentrated form. The specific activity of the purified enzyme was found to be 127 units per mg of protein.
EKSEMPEL 2 10 Til en 30% opløsning af en sprøjtetørret maltodextrin (D.E. omkring 10) i 0,05 M acetatpuffer ved pH 6,5 sattes den rensede glucoamylase fra eksempel 1. Enzymet tilsattes i en dosering på 0,20 enheder enzym pr. g substrat på tørstofbasis. Efter at opløsning var inkuberet ved 55° C i 15 72 timer var dextroseindholdet i det filtrerede hydroly sat, bestemt ved højydelsevæskchromatografi, 96,5% af det totale carbonhydrat.EXAMPLE 2 To a 30% solution of a spray-dried maltodextrin (D.E. about 10) in 0.05 M acetate buffer at pH 6.5, the purified glucoamylase of Example 1. The enzyme was added at a dosage of 0.20 units of enzyme per ml. g of dry matter substrate. After the solution was incubated at 55 ° C for 72 hours, the dextrose content of the filtered hydrolyz, as determined by high performance liquid chromatography, was 96.5% of the total carbohydrate.
EKSEMPEL 5EXAMPLE 5
Stivelse blev omdannet til et 10,2 D.E. stivelsehydroly-20 sat ved anvendelse af bakterie-a-amylase fra B. licheni-formis ifølge den almene procedure, som er anvendt i US patentskrift nr. 3 912 590. Opløsningen blev kogt i 5 minutter efter indstilling pH-værdien til 2,0. med 2 NHCl for at inaktivere den resterende α-amylase. Stivelsehydro-25 lysatopløsningen blev derpå indstillet til pH 6,2 og fortyndet til den ønskede koncentration før behandling med 0,20 enheder af den rensede glucoamylase fra eksempel 1 pr. g substrat (tørstofbasis). Opløsningen blev inkuberet ved 55° C i et tilproppet reagensglas. pH-værdien blev 30 indstillet til 6,2 efter 5 timer og efter 48 timer. Efter at opløsningen var blevet inkuberet i ?2 timer var dextro-seindholdet i det filtrerede hydrolysat, bestemt ved høj-ydelsesvæskechromatografi, 97,6% af det totale carbonhy- 19 146941 drat. Den endelige koncentration af opløsningen var 31,2% på tørstofbasis.Starch was transformed into a 10.2 D.E. starch hydrolyzed using bacterial α-amylase from B. licheni formis according to the general procedure used in U.S. Patent No. 3,912,590. The solution was boiled for 5 minutes after adjusting the pH to 2.0 . with 2 NHCl to inactivate the residual α-amylase. The starch hydrolyzate solution was then adjusted to pH 6.2 and diluted to the desired concentration before treatment with 0.20 units of the purified glucoamylase of Example 1 per ml. g substrate (dry matter basis). The solution was incubated at 55 ° C in a plugged test tube. The pH was adjusted to 6.2 after 5 hours and after 48 hours. After the solution was incubated for 2 hours, the dextrose content of the filtered hydrolyzate, as determined by high performance liquid chromatography, was 97.6% of the total hydrocarbon. The final concentration of the solution was 31.2% on a dry matter basis.
Når der udførtes saccharificeringsprøvninger ved den samme substratkoncentration med kommerciel glucoamylase 5 fra A. niger under dens optimumsbetingelser (pH 4,3 ved 60° C) var det tilsvarende dextroseudbytte 96,5%. På lignende måde gav glucoamylasen fra R. niveaus ved pH 5,0 og 55° C et dextr oseudbytte på 97%. Dextr oseudbytterne var omkring 1% lavere, når saccharificeringsprøvningerne udførtes 10 med de kommercielle glucoamylaser under de betingelser, som anvendes for enzymet ifølge opfindelsen. Disse resultater viser, at den hidtil ukendte glucoamylase ifølge opfindelsen giver højere udbytter af dextrose end de kommercielle glucoamy laser, selv når hvert enzym anvendes 15 under dets optimale reaktionsbetingelser.When saccharification tests were performed at the same substrate concentration with A. niger commercial glucoamylase 5 under its optimum conditions (pH 4.3 at 60 ° C), the corresponding dextrose yield was 96.5%. Similarly, the glucoamylase from R. levels at pH 5.0 and 55 ° C gave a dextr ose yield of 97%. The dextrase yields were about 1% lower when the saccharification tests were performed with the commercial glucoamylases under the conditions used for the enzyme of the invention. These results show that the novel glucoamylase of the invention provides higher yields of dextrose than the commercial glucoamy laser, even when each enzyme is used under its optimal reaction conditions.
Applications Claiming Priority (4)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| JP8781278 | 1978-07-20 | ||
| JP8781278A JPS5515720A (en) | 1978-07-20 | 1978-07-20 | Industrially usable novel heat resistant neutral glucoamylase and method |
| US06/055,717 US4254225A (en) | 1978-07-20 | 1979-07-09 | Novel neutral glucoamylase and method for its production |
| US5571779 | 1979-07-09 |
Publications (3)
| Publication Number | Publication Date |
|---|---|
| DK303379A DK303379A (en) | 1980-01-21 |
| DK146941B true DK146941B (en) | 1984-02-20 |
| DK146941C DK146941C (en) | 1984-07-30 |
Family
ID=26429060
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| DK303379A DK146941C (en) | 1978-07-20 | 1979-07-19 | GLUCOAMYLASE AND PROCEDURE FOR PREPARING A HIGH GLUCOSE CONTENT OF SYRUP BY SUCCARIFICATION OF MELTED STARCH |
Country Status (9)
| Country | Link |
|---|---|
| AR (1) | AR225420A1 (en) |
| AU (1) | AU527668B2 (en) |
| CA (1) | CA1131142A (en) |
| DK (1) | DK146941C (en) |
| ES (2) | ES482625A1 (en) |
| GB (1) | GB2025978B (en) |
| IT (1) | IT1193794B (en) |
| MX (1) | MX6277E (en) |
| MY (1) | MY8400139A (en) |
Families Citing this family (2)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US4536477A (en) * | 1983-08-17 | 1985-08-20 | Cpc International Inc. | Thermostable glucoamylase and method for its production |
| ATE95837T1 (en) * | 1984-08-06 | 1993-10-15 | Genencor Inc | ENZYMATIC HYDROLYSIS OF GRANULAR STARCH DIRECTLY TO GLUCOSE. |
-
1979
- 1979-07-17 IT IT7924432A patent/IT1193794B/en active
- 1979-07-18 GB GB7925069A patent/GB2025978B/en not_active Expired
- 1979-07-18 AU AU49044/79A patent/AU527668B2/en not_active Ceased
- 1979-07-18 AR AR277356A patent/AR225420A1/en active
- 1979-07-19 ES ES482625A patent/ES482625A1/en not_active Expired
- 1979-07-19 ES ES482619A patent/ES482619A1/en not_active Expired
- 1979-07-19 MX MX798207U patent/MX6277E/en unknown
- 1979-07-19 DK DK303379A patent/DK146941C/en not_active IP Right Cessation
- 1979-07-20 CA CA332,250A patent/CA1131142A/en not_active Expired
-
1984
- 1984-12-30 MY MY139/84A patent/MY8400139A/en unknown
Also Published As
| Publication number | Publication date |
|---|---|
| GB2025978A (en) | 1980-01-30 |
| ES482625A1 (en) | 1980-04-16 |
| GB2025978B (en) | 1982-12-22 |
| CA1131142A (en) | 1982-09-07 |
| MX6277E (en) | 1985-03-05 |
| DK146941C (en) | 1984-07-30 |
| AR225420A1 (en) | 1982-03-31 |
| ES482619A1 (en) | 1980-04-16 |
| IT7924432A0 (en) | 1979-07-17 |
| DK303379A (en) | 1980-01-21 |
| MY8400139A (en) | 1984-12-31 |
| AU527668B2 (en) | 1983-03-17 |
| IT1193794B (en) | 1988-08-24 |
| AU4904479A (en) | 1980-01-24 |
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