WO2012124668A1 - アリールスルファターゼの活性測定方法 - Google Patents
アリールスルファターゼの活性測定方法 Download PDFInfo
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- WO2012124668A1 WO2012124668A1 PCT/JP2012/056340 JP2012056340W WO2012124668A1 WO 2012124668 A1 WO2012124668 A1 WO 2012124668A1 JP 2012056340 W JP2012056340 W JP 2012056340W WO 2012124668 A1 WO2012124668 A1 WO 2012124668A1
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- C12Q—MEASURING OR TESTING PROCESSES INVOLVING ENZYMES, NUCLEIC ACIDS OR MICROORGANISMS; COMPOSITIONS OR TEST PAPERS THEREFOR; PROCESSES OF PREPARING SUCH COMPOSITIONS; CONDITION-RESPONSIVE CONTROL IN MICROBIOLOGICAL OR ENZYMOLOGICAL PROCESSES
- C12Q1/00—Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions
- C12Q1/34—Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions involving hydrolase
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- A—HUMAN NECESSITIES
- A23—FOODS OR FOODSTUFFS; TREATMENT THEREOF, NOT COVERED BY OTHER CLASSES
- A23C—DAIRY PRODUCTS, e.g. MILK, BUTTER OR CHEESE; MILK OR CHEESE SUBSTITUTES; MAKING THEREOF
- A23C9/00—Milk preparations; Milk powder or milk powder preparations
- A23C9/12—Fermented milk preparations; Treatment using microorganisms or enzymes
- A23C9/1203—Addition of, or treatment with, enzymes or microorganisms other than lactobacteriaceae
- A23C9/1206—Lactose hydrolysing enzymes, e.g. lactase, beta-galactosidase
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- C12N9/00—Enzymes; Proenzymes; Compositions thereof; Processes for preparing, activating, inhibiting, separating or purifying enzymes
- C12N9/14—Hydrolases (3)
- C12N9/16—Hydrolases (3) acting on ester bonds (3.1)
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- 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)
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- 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)
- C12N9/2468—Hydrolases (3) acting on glycosyl compounds (3.2) hydrolysing O- and S- glycosyl compounds (3.2.1) acting on beta-galactose-glycoside bonds, e.g. carrageenases (3.2.1.83; 3.2.1.157); beta-agarase (3.2.1.81)
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- 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)
- C12N9/2468—Hydrolases (3) acting on glycosyl compounds (3.2) hydrolysing O- and S- glycosyl compounds (3.2.1) acting on beta-galactose-glycoside bonds, e.g. carrageenases (3.2.1.83; 3.2.1.157); beta-agarase (3.2.1.81)
- C12N9/2471—Beta-galactosidase (3.2.1.23), i.e. exo-(1-->4)-beta-D-galactanase
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- C12Q—MEASURING OR TESTING PROCESSES INVOLVING ENZYMES, NUCLEIC ACIDS OR MICROORGANISMS; COMPOSITIONS OR TEST PAPERS THEREFOR; PROCESSES OF PREPARING SUCH COMPOSITIONS; CONDITION-RESPONSIVE CONTROL IN MICROBIOLOGICAL OR ENZYMOLOGICAL PROCESSES
- C12Q1/00—Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions
- C12Q1/34—Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions involving hydrolase
- C12Q1/44—Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions involving hydrolase involving esterase
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- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12Y—ENZYMES
- C12Y301/00—Hydrolases acting on ester bonds (3.1)
- C12Y301/06—Sulfuric ester hydrolases (3.1.6)
- C12Y301/06001—Arylsulfatase (3.1.6.1)
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- 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)
- C12Y302/01023—Beta-galactosidase (3.2.1.23), i.e. exo-(1-->4)-beta-D-galactanase
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- C—CHEMISTRY; METALLURGY
- 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)
- C12Y302/01108—Lactase (3.2.1.108)
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- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N2333/00—Assays involving biological materials from specific organisms or of a specific nature
- G01N2333/90—Enzymes; Proenzymes
- G01N2333/914—Hydrolases (3)
- G01N2333/916—Hydrolases (3) acting on ester bonds (3.1), e.g. phosphatases (3.1.3), phospholipases C or phospholipases D (3.1.4)
Definitions
- the present invention is a highly sensitive method for measuring arylsulfatase activity and a highly active lactase preparation, and the arylsulfatase is not contaminated or contaminated by the highly sensitive activity assay method for arylsulfatase of the present invention.
- the present invention relates to a lactase preparation confirmed to be a trace amount, a method for producing such a lactase preparation, and a dairy product produced using such a lactase preparation.
- milk Since ancient times, milk has long been used as a nutritious and useful food. Milk contains lactose, a kind of sugar. Lactose is broken down in the intestine by lactase, but in some humans, as the amount of lactase secreted into the intestine decreases as it grows, milk and milk processed products (hereinafter collectively referred to as “dairy products”) ) causes so-called lactose intolerance such as abdominal pain and diarrhea. This contributed to the widespread consumption of this nutritious food.
- dairy products in which lactose has been reduced or removed in advance have been provided. Such a dairy product can be consumed without problems even by a human with lactose intolerance.
- Lactose is reduced or removed by various methods, but the most common is a method of hydrolyzing lactose by treating a dairy product with a lactase preparation.
- lactase preparation is aseptically added to sterilized milk and lactose is decomposed during distribution. This is believed to reduce the amount of lactase preparation used and contribute to cost reduction.
- Patent Document 1 describes a lactase preparation in which the amount of arylsulfatase contamination is reduced and a method for producing the same.
- arylsulfatase activity is not measured in a trace amount region of 8 units (arylsulfatase activity per 1 LLU of lactase active substance, the same shall apply hereinafter) or less, and is described as below the detection limit. It has only been done.
- Table 1 of Patent Document 1 it is described that if the activity of contaminating arylsulfatase is 19 units or less, no odor is produced in the dairy product.
- arylsulfatase contaminating the enzyme preparation In order to remove the arylsulfatase contaminating the enzyme preparation to the utmost limit, general purification methods may be combined. Or what is necessary is just to select and breed the microorganisms which produce the target enzyme, Comprising: Arylsulfatase production ability is deleted. In addition, a microorganism obtained by transforming a host that originally does not produce arylsulfatase to produce the target enzyme can also be used.
- Patent Document 1 describes a method for obtaining a microorganism having reduced ability to produce arylsulfatase by mutation treatment and a microorganism having an arylsulfatase gene deleted by genetic engineering techniques.
- a method for obtaining a microorganism in which arylsulfatase production ability has been reduced by mutation treatment has been described, there is no description of an actual acquisition example, and only the possibility has been shown. That is, it is unclear whether or not it is possible to produce a microorganism having an arylsulfatase production ability reduced by mutation treatment at an industrial level by the method described in Patent Document 1.
- yeast diploid strains useful for industrial production of lactase formulations it is necessary to obtain double mutants to disrupt the arylsulfatase gene by mutation, and such double mutants Acquisition was considered difficult in practice.
- Patent Document 1 only describes an example using a haploid strain called CBS2359 strain.
- a haploid strain called CBS2359 strain it is difficult to effectively disrupt a gene in a diploid strain of yeast useful for the production of a lactase preparation. Therefore, aryl which is a diploid strain of yeast is used. A sulfatase non-producing strain cannot be produced.
- lactase activity of the lactase preparation described in the Example of Patent Document 1 is about 5000 to 5,500 NLU / g for Maxilact (registered trademark) LG5000 (manufactured by DSM), and GODO YNL2 (manufactured by Godo Shusei Co., Ltd.).
- the present inventors have made diligent efforts to solve the above-mentioned problems, and have developed a method with higher sensitivity than the conventional method as a method for measuring arylsulfatase activity in aqueous systems.
- it is a method for measuring arylsulfatase activity with higher sensitivity than that of the conventional method, and the activity of arylsulfatase contaminated in the lactase preparation is measured by the fluorescence method in the region that was conventionally below the detection limit.
- the present inventors have completed the present invention by identifying the amount of arylsulfatase contamination to prevent undesirable taste and odor from occurring in milk and dairy products.
- the present invention comprises reacting an aryl sulfatase with its substrate, which releases a fluorophore or chromophore when the substrate is subjected to the action of the aryl sulfatase, in an aqueous reaction system having a high ionic strength.
- the present invention relates to a method for measuring the activity of arylsulfatase in an aqueous system.
- a preferred example of means for reacting in an aqueous reaction system having high ionic strength is to react with an enzyme and a substrate in an aqueous reaction system to which an inorganic salt is added, and / or a buffer that does not denature the enzyme protein.
- the reaction between an enzyme and a substrate in a liquid system is to react with an enzyme and a substrate in an aqueous reaction system to which an inorganic salt is added, and / or a buffer that does not denature the enzyme protein.
- a preferable range of the inorganic salt concentration in the aqueous reaction system is 10 to 1000 mM, a more preferable range is 50 to 500 mM, a preferable range of the buffer solution concentration is 10 to 200 mM, and a more preferable range is 50 to 200 mM. .
- the inorganic salt is preferably at least one selected from the group consisting of potassium chloride, sodium chloride and ammonium sulfate.
- the said buffer solution is a phosphate buffer solution.
- the method for measuring the activity of arylsulfatase in the aqueous system of the present invention is particularly preferably a method comprising the following steps (1) to (10): (1) A specimen in which the presence of arylsulfatase is predicted is appropriately diluted with a 100 mM potassium phosphate buffer (pH 6.5) containing 0.5 M potassium chloride to prepare a sample. (2) An aqueous solution containing 2-methylumbelliferone sulfate potassium at a concentration of 2 mM is prepared. (3) The sample and a 4-methylumbelliferone sulfate aqueous solution are mixed at 1: 1 (volume basis) and reacted at 37 ° C. for 3 hours.
- the 4-methylumbelliferone concentration of the measurement sample is calculated, divided by 3, and the reaction time is 1 hour. If so, determine the 4-methylumbelliferone concentration. Further, the amount of 4-methylumbelliferone generated during the reaction for 1 hour is calculated from the volume of the reaction solution. (9) Since the amount of 4-methylumbelliferone calculated in this way is based on the amount of sample contained in the sample prepared in (1), it is converted to the amount of 4-methylumbelliferone per gram of sample. To do. (10) When the amount of 4-methylumbelliferone produced per 1 hour of the reaction time between the substrate and the enzyme is 1 nmole, the unit is 1 unit (U). That is, it is represented by “unit (U) / g”.
- step (10) “substrate” is potassium 4-methylumbelliferone sulfate, and “enzyme” is arylsulfatase.
- the above-described method for measuring the activity of arylsulfatase in an aqueous system of the present invention can be applied to the measurement of the activity of arylsulfatase in a lactase preparation.
- the present invention also provides a yeast diploid strain having a lactase gene and a restricted arylsulfatase protein expression or a genetic recombination in which a yeast lactase gene is introduced and the expression of an arylsulfatase protein is restricted.
- the above-described lactase preparation of the present invention can also be produced without the step of removing contaminating arylsulfatase.
- the “arylsulfatase removal step” refers to a lactase protein that is a target enzyme, such as an ammonium sulfate fraction from an aqueous solution containing the target enzyme, in a fractionation and purification method carried out in this technical field. It does not include a step in which the arylsulfatase protein is purified. This refers to the process in which the target enzyme lactase protein is separated from the arylsulfatase protein.
- the arylsulfatase protein is not expressed, that is, the production amount is zero, but the arylsulfatase activity (unit: U / g) / lactase activity (unit: NLU / g) is 0.1% or less.
- the expression of the arylsulfatase protein may be limited so as to be preferably 0.02% or less.
- the lactase preparation according to the present invention has a lactase activity of 4,000 NLU / g or more, preferably 4,500 NLU / g or more, more preferably 5,000 NLU / g or more.
- the yeast diploid strain having a lactase gene and restricted expression of arylsulfatase protein may be a mutant strain obtained by a mutation treatment of a yeast diploid strain or a yeast diploid strain. It may be a mutant obtained by subjecting a body strain to deletion of an arylsulfatase gene or an arylsulfatase protein expression regulatory gene. A mutant strain whose parent strain is a diploid strain of yeast having a large production amount of lactase protein is preferred.
- the diploid strain of yeast is preferably a diploid strain of Kluyveromyces lactis or its closely related species, Kluyveromyces marxianus.
- the genetically modified microorganism into which the yeast lactase gene is introduced and the expression of the arylsulfatase protein is restricted is preferably a genetically modified microorganism into which the Klaveromyces lactis or Kriveromyces marixianus lactase gene is introduced.
- the present invention relates to a yeast diploid strain having a lactase gene and restricted expression of an arylsulfatase protein, or a genetically modified microorganism into which a yeast lactase gene has been introduced and the expression of an arylsulfatase protein is restricted. Cultivate and recover the cells or microorganisms without destroying the cell wall, destroy the cell walls and recover the culture solution together with the cells or microorganisms, or recover the culture solution without destroying the cell walls.
- the lactase preparation of the present invention (that is, the lactase activity by the FCC IV method is 4,000 NLU / g or more, without using the arylsulfatase removal step, using the recovered cells or microorganisms and / or culture solution as a raw material, and Based on the lactase activity, the aryl sulfata in the aqueous system of the present invention comprising the above steps (1) to (10) Activity was measured by the measuring method, calculated arylsulfatase activity (unit: U / g) is relates to a process for the preparation of lactase preparation characterized by preparing a lactase preparation) 0.1% or less. The case where the culture solution is collected without destroying the cell wall is a case where the genetically modified microorganism secretes lactase.
- the preparation process of the lactase preparation may include a purification process performed in the art, such as concentration of lactase protein.
- concentration of lactase protein concentration of lactase protein.
- the arylsulfatase removal step is not performed.
- a highly active lactase protein is produced, and the production of contaminating arylsulfatase protein uses a very small amount of yeast diploid strain or genetically modified microorganism. Even if it is not large, a lactase preparation with high lactase activity is obtained, and the concentration factor is not large, so that the contaminated arylsulfatase protein does not become highly active even when concentrated.
- the present invention relates to a dairy product produced using the lactase preparation according to the present invention.
- a trace amount of arylsulfatase can be measured using the activity as an index as compared with the conventional method. According to the present invention, since a highly sensitive method for measuring arylsulfatase activity was established, it became possible to accurately grasp the amount of arylsulfatase in a lactase preparation using the activity as an index.
- a diploid strain of yeast having a lactase gene and restricted expression of arylsulfatase protein, or cultivation of a genetically modified microorganism into which yeast lactase gene is introduced and expression of arylsulfatase gene protein is restricted It became possible to provide a lactase preparation having a high lactase activity in which the amount of arylsulfatase contamination is very small or does not contain arylsulfatase, using the subsequent cells or microorganisms and / or culture solution as raw materials. Since the lactase preparation of the present invention has high lactase activity, the amount of use thereof can be reduced. Therefore, when the preparation contains additives such as stabilizers or impurities, those for the intended use can be reduced. The effect of reducing the amount of carry-in is obtained.
- the lactase preparation of the present invention is used, the effect of suppressing the occurrence of unpleasant taste and odor with an uncomfortable feeling in long life milk and the like can be obtained.
- a lactase preparation having a high lactase activity is produced without removing the contaminating arylsulfatase.
- the production efficiency is high, and there is no decrease in lactase activity in the purification step for removal of arylsulfatase.
- a conventionally known method for measuring the activity of arylsulfatase is a colorimetric method using a compound in which a sulfate group is bound to a chromophore such as p-nitrophenol as a substrate.
- a chromophore such as p-nitrophenol
- absorbance the amount of chromophore released by the removal of sulfate groups from the substrate due to the reaction between the substrate and arylsulfatase is measured by absorbance.
- the amount of liberated chromophore such as p-nitrophenol is small, the change in absorbance is small and it is difficult to obtain a clear measured value.
- a fluorescence method using a compound in which a sulfate group is bound to a fluorophore, for example, 4-methylumbelliferyl sulfate as a substrate is also known (Method in Enzymology, 11/21).
- the sensitivity of the fluorescence method is generally said to be 100 times or more the sensitivity of the colorimetric method.
- the inventors of the present invention have examined measurement conditions that can make the sensitivity higher than conventional colorimetric methods and fluorescence methods as a method for measuring arylsulfatase activity in an aqueous system.
- the inventors have conceived that the arylsulfatase activity can be measured with high sensitivity by increasing the ionic strength of the reaction system between the enzyme and the substrate, and the method for measuring the arylsulfatase activity of the present invention has been established.
- the enzyme reaction is remarkably activated, and as a result, more chromophores and fluorophores are released. It has never been known so far.
- the method for measuring the activity of arylsulfatase in an aqueous system is carried out by reacting arylsulfatase with its substrate (however, when the substrate is subjected to the action of arylsulfatase, the fluorophore or chromophore is released). It is characterized by increasing the ionic strength of the system.
- a specific means for increasing the ionic strength of the reaction system is to allow an inorganic salt to coexist in the reaction system or to perform an enzyme reaction in a buffer solution system.
- Examples of inorganic salts to be added to the reaction system include potassium chloride, sodium chloride, ammonium sulfate and the like.
- concentration of such an inorganic salt is, for example, 10 to 1000 mM, preferably 50 to 500 mM in the reaction system.
- buffer systems include phosphate-potassium phosphate buffers that do not denature enzyme proteins (the concept of potassium phosphate includes potassium dihydrogen phosphate, dipotassium hydrogen phosphate, and tripotassium phosphate).
- Phosphoric acid such as sodium phosphate phosphate (including sodium dihydrogen phosphate, disodium hydrogen phosphate and trisodium phosphate), phosphate buffered saline, etc.
- a salt buffer may be mentioned.
- the concentration of such a buffer in the reaction system is, for example, 10 to 200 mM, and preferably 50 to 200 mM.
- an inorganic salt may be added to an aqueous solution of a specimen in which the presence of arylsulfatase is predicted (for example, a specimen dissolved in water or a buffer).
- an inorganic salt may be added to the aqueous solution of the substrate.
- a typical example of the method for measuring the activity of arylsulfatase according to the present invention is as follows.
- a specimen in which the presence of arylsulfatase is predicted is appropriately diluted with a 100 mM potassium phosphate buffer (pH 6.5) containing 0.5 M potassium chloride to prepare a sample.
- An aqueous solution containing 2-methylumbelliferone sulfate potassium at a concentration of 2 mM is prepared.
- the sample and a 4-methylumbelliferone sulfate aqueous solution are mixed at 1: 1 (volume basis) and reacted at 37 ° C. for 3 hours.
- To the reaction solution add the same amount (volume basis) of 0.1N sodium hydroxide aqueous solution as the reaction solution to stop the reaction and prepare a measurement sample.
- the fluorescence intensity is measured at an excitation wavelength of 360 nm and a fluorescence wavelength of 450 nm.
- (6) 4-Methylumbelliferone is dissolved in a 100 mM potassium phosphate buffer (pH 6.5) containing 0.5 M potassium chloride to obtain a solution with an appropriate concentration. An aqueous sodium oxide solution is added, and the fluorescence intensity is measured under the same conditions as in (5).
- a calibration curve is created from (6).
- the 4-methylumbelliferone concentration of the measurement sample is calculated, divided by 3, and the reaction time is 1 hour. If so, determine the 4-methylumbelliferone concentration.
- the amount of 4-methylumbelliferone generated during the reaction for 1 hour is calculated from the volume of the reaction solution. (9) Since the amount of 4-methylumbelliferone calculated in this way is based on the amount of sample contained in the sample prepared in (1), it is converted to the amount of 4-methylumbelliferone per gram of sample. To do. (10) The case where the amount of 4-methylumbelliferone produced per 1 hour of the reaction time between the substrate and the enzyme is 1 nmole is defined as 1 unit (U), and the unit is the unit amount per 1 g of the specimen, that is, the enzyme preparation, That is, it is represented by “unit (U) / g”.
- a diploid strain of yeast that produces lactase protein, has a lactase gene, and is restricted in the expression of arylsulfatase protein is used.
- the diploid strain of yeast used in the present invention produces a highly active lactase protein that can provide a lactase preparation of 4,000 NLU / g or more as it is or when concentrated.
- Such a yeast diploid strain is, for example, a mutant strain obtained by microbial mutation treatment.
- mutants can be mutated by exposing diploid strains of yeast that produce highly active lactase protein to UV irradiation or chemical mutagens, and then mutating both diploid genes.
- a method of destroying or deleting an arylsulfatase gene or an arylsulfatase protein expression regulatory gene, or a method of deleting an arylsulfatase gene or an arylsulfatase protein expression regulatory gene by genetic engineering techniques for both diploid genes Etc. can be obtained. Whether or not a desired mutant strain has been obtained may be determined by measuring the arylsulfatase activity of the cultivated yeast culture solution by the method for measuring arylsulfatase activity (fluorescence method) according to the present invention.
- Induction of mutation by ultraviolet rays is performed, for example, by irradiating a suspension of diploid yeast with ultraviolet rays.
- chemical mutagenesis is performed by adding a chemical mutagen to a suspension of diploid yeast, for example.
- chemical mutagens include 5-bromouracil, 2-aminopurine, nitrous acid, hydroxylamine, acriflavine, methanesulfonic acid compound, nitrosoguanidine and the like.
- a gene fragment having a homologous sequence of the gene to be deleted is obtained, and the fragment is subcloned into a vector and deleted.
- Ordinary genetic engineering techniques such as constructing a disruption vector for a power gene and transforming a diploid strain of yeast using the vector, may be applied.
- the production of the lactase preparation of the present invention is a genetically modified microorganism in which the yeast lactase gene is introduced so as to express the lactase protein and the expression of the arylsulfatase protein is restricted, and produces a highly active lactase protein. Can also be used.
- arylsulfatase protein is restricted
- a gene involved in the production of arylsulfatase protein is restricted, and more specifically, arylsulfatase gene and / or Because there is no aryl sulfatase protein expression regulatory gene, or because the aryl sulfatase gene (structural gene) is disrupted or the expression regulatory gene that causes the aryl sulfatase gene to express the aryl sulfatase protein is disrupted It means that arylsulfatase protein is not produced or its production amount is reduced.
- a genetically modified microorganism into which a yeast lactase gene is introduced and the expression of arylsulfatase protein is restricted can be prepared by a known method.
- a lactase gene is incorporated into a plasmid resistant to drug A and, if necessary, an expression control gene for the lactase gene is incorporated at the same time.
- the lactase expression plasmid thus prepared is used to transform a host microorganism.
- the transformed microorganism is cultured in a medium containing the drug A, and the appearing colonies are selected.
- E. coli, yeast, Bacillus subtilis, etc. can be used as a host for obtaining a genetically modified microorganism into which a yeast lactase gene has been introduced and the expression of arylsulfatase protein is restricted.
- a host for obtaining a recombinant microorganism into which a yeast lactase gene is introduced and the expression of arylsulfatase protein is restricted a host that does not have an arylsulfatase gene or an arylsulfatase protein expression regulatory gene, or an arylsulfatase A host in which a gene or an arylsulfatase protein expression regulatory gene is disrupted or deleted is desirable.
- a lactase for a lactase preparation is a yeast diploid strain that has a lactase gene and the expression of an arylsulfatase protein is restricted, or a gene set in which a yeast lactase gene is introduced and the expression of an arylsulfatase protein is restricted.
- Culture microorganisms that produce highly active lactase protein and recover cells or microorganisms without destroying the cell wall, or recover the culture solution together with cells or microorganisms by destroying the cell walls Alternatively, the culture solution is collected without destroying the cell wall, and the collected cells or microorganisms and / or the culture solution are used as raw materials without the arylsulfatase removal step.
- the concept of “culture medium” includes culture supernatant.
- Incubation of microorganisms such as yeast can be performed using an incubator such as a flask, jar, tank, etc.
- an incubator such as a flask, jar, tank, etc.
- a temperature, pH, number of stirring and the like suitable for enzyme production by the microorganisms are selected.
- a culture solution in which lactase is dissolved is usually obtained by breaking the cell wall.
- the cell wall need not be destroyed.
- the cell walls of the cells (or microorganisms) are then destroyed in distilled water, and the components inside the cells are distilled water. It is dissolved in the aqueous solution containing microbial cells or microbial cells.
- the culture solution or aqueous solution containing or not containing bacterial cells or microbial cells is usually separated into supernatant and residue by centrifugation, filtration and other appropriate methods commonly used in this technical field.
- the supernatant may be used as it is as an enzyme solution, or may be used as an enzyme solution after being concentrated using an ultrafiltration membrane or the like.
- the enzyme solution may be pulverized by a method such as spray drying or freeze drying.
- the enzyme solution itself thus obtained can also be used as a lactase preparation.
- the lactase preparation of the present invention is produced using a yeast diploid strain or microorganism that produces a highly active lactase protein and does not produce an arylsulfatase protein or produces only a trace amount. Usually, in order to remove only arylsulfatase, it is not necessary to use the culture solution or the like for one or more purification operations such as adsorption, chromatography, crystallization and the like.
- the method for producing a lactase preparation of the present invention does not include an arylsulfatase removal step.
- arylsulfatase removal step purification methods that do not separate lactase protein and arylsulfatase protein, such as solvent fractionation and ammonium sulfate fractionation, are not included in the definition of “arylsulfatase removal step”.
- the essential component of the lactase preparation according to the present invention is lactase.
- the lactase preparation contains other components as long as it is a substance that does not inhibit the activity of the lactase and does not inhibit the activity, or unless it has an undesirable effect on the intended use of the lactase preparation. May be present.
- substances that may be present include starches, dextrin, and buffering agents that are excipients for ease of use, such as metal salts that contribute to the stabilization of lactase, various sugars, ascorbic acid, glycerin, etc. Inorganic salts and the like.
- the properties of the lactase preparation are not particularly limited, and may be, for example, powder, granules, solutions and the like.
- the present invention also relates to a dairy product produced using the lactase preparation according to the present invention.
- Dairy products refer to milk such as long life milk, yogurt, fresh cream, sour cream, cheese and the like.
- the lactase preparation is used in the usual manner and amount used in this technical field (however, the amount used is calculated based on the lactase activity).
- Example 1 Examination of measuring method of arylsulfatase activity (part 1) 5 times dilution of GODO-YNL2 (Lactase preparation manufactured by Godo Sakesei Co., Ltd .; liquid) with 100 mM potassium phosphate buffer (pH 6.5) containing 0, 0.2, 0.5 or 1.0 M potassium chloride did. To 0.5 mL of each of these solutions, 0.5 mL of 100 mM potassium phosphate buffer (pH 6.5) of p-nitrophenyl sulfate was added and reacted at 37 ° C. for 3 hours. The reaction was stopped by adding 1.5 mL of a 1.5N aqueous sodium hydroxide solution, and the absorbance was measured at 410 nm. The relative values are shown in Table 1, assuming that the case of not containing potassium chloride is 100%.
- Example 2 Examination of measuring method of arylsulfatase activity (part 2) (1) 100% of GODO-YNL2 (Lactase preparation manufactured by Godo Seisei Co., Ltd .; liquid) with 100 mM potassium phosphate buffer (pH 6.5) containing 0, 125, 250, 500 or 1,000 mM sodium chloride Diluted. 0.5 mL of an aqueous solution of 2 mM 4-methylumbelliferone sulfate potassium was added to 0.5 mL of each of these solutions, and reacted at 37 ° C. for 3 hours.
- the reaction was stopped by adding 1.0 mL of a 0.1N sodium hydroxide aqueous solution, and the fluorescence intensity was measured at an excitation wavelength of 360 nm and a fluorescence wavelength of 450 nm.
- the relative values are shown in Table 2 assuming that no sodium chloride is contained as 100%.
- Example 3 Examination of measuring method of arylsulfatase activity (part 3) (1) GODO-YNL2 (Lactase preparation manufactured by Godo Shusei Co., Ltd .; liquid) was diluted 100 times with 100 mM, 125 mM, 250 mM, 500 mM, and 1,000 mM potassium phosphate buffer (pH 6.5). 0.5 mL of an aqueous solution of 2 mM 4-methylumbelliferone sulfate potassium was added to 0.5 mL of each of these solutions, and reacted at 37 ° C. for 3 hours.
- GODO-YNL2 (Lactase preparation manufactured by Godo Seisei Co., Ltd .; liquid) was diluted 100 times with 100 mM potassium phosphate buffer (pH 6.5). Separately, it was diluted 100-fold with 100 mM potassium phosphate buffer (pH 6.5) containing 0.5 M potassium chloride. 0.5 mL of an aqueous solution of 2 mM 4-methylumbelliferone sulfate potassium was added to 0.5 mL of each of these solutions, and reacted at 37 ° C. for 1 hour. The reaction was stopped by adding 1.0 mL of 0.1N aqueous sodium hydroxide solution thereto.
- each blank was prepared by adding a 0.1N aqueous sodium hydroxide solution to a diluted enzyme solution and inactivating it, and then adding an aqueous solution of 4-methylumbelliferone sulfate potassium.
- Example 5 Measurement of arylsulfatase activity by a conventionally known colorimetric method GODO-YNL2 (Lactase preparation manufactured by Godo Sakesei Co., Ltd .; liquid) was diluted with distilled water to give a 1% (w / v) solution. Got. This was diluted with 100 mM potassium phosphate buffer (pH 6.5) containing 0.5 M potassium chloride, 0.8% (w / v), 0.6% (w / v), 0.4 % (W / v) and 0.2% (w / v) solutions were obtained.
- Example 6 Measurement of arylsulfatase activity by fluorescence method: GODO-YNL2 (Lactase preparation manufactured by Godo Shusei Co., Ltd .; liquid) was diluted with 100 mM potassium phosphate buffer (pH 6.5) containing 0.5 M potassium chloride. 1% (w / v) solution was obtained. This 1% solution was diluted with the same buffer and 0.8% (w / v), 0.6% (w / v), 0.4% (w / v) and 0.2% ( w / v) A solution was obtained.
- Example 7 Comparison of colorimetric method and fluorescence method in measuring arylsulfatase activity The difference in sensitivity between the colorimetric method and fluorescence method in measuring arylsulfatase activity was examined. First, purified lactase used in this experiment was prepared.
- the plate was washed with 40 L of 10 mM potassium phosphate buffer (pH 7) containing 50 mM sodium chloride, and then lactase was eluted with 200 L of 10 mM potassium phosphate buffer (pH 7) containing 100 mM sodium chloride. At this time, the fraction was fractionated into 20 L portions.
- Lactase activity of each fraction (according to FCC IV method; Food Chemicals Codex 4th Edition, Effective July 1st, 1996, Commite on Food Chemicals Codex, p.801-802)
- the fraction reduced in arylsulfatase was collected, mixed, and concentrated using an ultrafiltration membrane (ACP membrane manufactured by Asahi Kasei Co., Ltd.) to obtain a lactase concentrate.
- Glycerin was added to this concentrated liquid so that it might become 50% (w / w), and the refined lactase formulation was obtained.
- an aqueous solution containing p-nitrophenol at a concentration of 0 to 0.5 mM was prepared.
- 0.5 mL of a 100 mM potassium phosphate buffer solution (pH 6.5) was added to 0.5 mL of each of these solutions, and 1.5 mL of a 1.5N sodium hydroxide aqueous solution was further added to obtain a measurement sample.
- Absorbance at 410 nm was measured to prepare a calibration curve.
- the lactase preparation was diluted with a 100 mM potassium phosphate buffer (pH 6.5) containing 0.5 M potassium chloride to obtain a 1% (w / v) solution.
- a 100 mM potassium phosphate buffer (pH 6.5) containing 0.5 M potassium chloride was obtained.
- 0.5 mL of 2 mM 4-methylumbelliferyl sulfate aqueous solution was added to 0.5 mL of this 1% solution and reacted at 37 ° C. for 3 hours.
- the reaction was stopped by adding 1 mL of a 0.1N sodium hydroxide aqueous solution to this, and the fluorescence intensity was measured at an excitation wavelength of 360 nm and a fluorescence wavelength of 450 nm.
- a 100 mM potassium phosphate buffer (pH 6.5) containing 0.5 M potassium chloride containing 4-methylumbelliferone at a concentration of 0 to 4 ⁇ M was prepared.
- a sample for measurement was obtained by adding 1 mL of a 0.1 N aqueous sodium hydroxide solution to 1.0 mL of each of these solutions.
- the fluorescence intensity was measured at an excitation wavelength of 360 nm and a fluorescence wavelength of 450 nm, and a calibration curve was prepared.
- WO07 / 060247 states that a lactase preparation having 19 or less contaminating arylsulfatases (units defined in WO07 / 060247) does not produce off-flavors when added to decompose lactose after sterilization of milk.
- WO07 / 060247 states that a lactase preparation having 19 or less contaminating arylsulfatases (units defined in WO07 / 060247) does not produce off-flavors when added to decompose lactose after sterilization of milk.
- this is a view based on the results of a test conducted by limiting the reaction days of lactase to 2 days.
- lactase preparations containing arylsulfatase at various contamination rates were prepared, added to milk, and the flavor was confirmed after a predetermined number of days.
- Lactase preparations A to E containing arylsulfatases with various contamination rates include the purified lactase preparation prepared in Example 7 and GODO-YNL2 containing 100 units of the selected arylsulfatase activity (units described in WO07 / 060247). (Lactase preparation manufactured by Godo Seisei Co., Ltd .; liquid) was appropriately mixed and prepared.
- the arylsulfatase activities of the prepared lactase preparations A to E were measured by the method described in WO07 / 060247 and the fluorescence method shown in Example 7 above. Moreover, the lactase activity was measured by FCC IV method. The results are shown in Table 7. Here, the unit described in WO07 / 060247 is ⁇ OD 410 ⁇ 10 6 / hour / NLU.
- each of the lactase preparations A to E was carried out so that lactase became 20,000 NLU / L-milk in commercial milk (heat pasteurized; pasteurized conditions: 130 ° C. 2 seconds). And stored at 30 ° C. After 2 days of storage, 1 month and 3 months later, a flavor sensory test was conducted on milk not added with lactase preparation and milk added with lactase preparation.
- the flavor sensory test was conducted as a blind test. Eleven to thirteen panelists sniffed the milk after storage for a certain period of time, and also judged whether it had a smell that was uncomfortable and contained in the mouth. The evaluation was made with a score of 0 (-) for those that did not feel odor, 1 (+) for those that felt odor, and 2 (++) for those that felt strong. The summarized results are shown in Table 8.
- lactase preparation A or B that is, those having arylsulfatase activity by the method of the present invention / actase activity by the FCC IV method of 0.02% or less
- lactase preparation A it became clear that the use of was more preferable.
- the arylsulfatase activity value comparable to lactase preparations A and B needs to be measured by the fluorescence analysis method described in this specification or an analysis method showing sensitivity equal to or higher than that. .
- Example 9 Acquisition of mutant strain with reduced arylsulfatase production ability Cliveromyces lactis G14-427 strain, which is a diploid strain, was added to 10 mL of YPD medium (1% yeast extract, 1% glucose, 2% peptone). 1 platinum ear inoculation was carried out, and the bacterial suspension was stored at 30 ° C. and cultured. When the logarithmic growth phase was reached, the medium was centrifuged to recover the bacterial cells. The collected cells were dispersed in sterilized water so that the absorbance at 600 nm was 0.5. The bacterial suspension was irradiated with ultraviolet rays for 15 seconds with a UV lamp.
- YPD medium 1% yeast extract, 1% glucose, 2% peptone
- the cells were collected by centrifugation and mixed and dispersed in the YPD medium. An appropriate amount was taken from the YPD medium containing the bacterial cells and applied to the YPD agar plate medium. Static culture was performed at 37 ° C. for 7 days. A small amount of the grown colonies were scraped and mixed with 1 mL of a solution containing zymolyce (manufactured by Seikagaku Biobusiness Co., Ltd.) at 1 mg / mL. The reaction was carried out at 30 ° C. for 2 hours to destroy the cell wall. Thereafter, centrifugation was performed and the supernatant was collected.
- zymolyce manufactured by Seikagaku Biobusiness Co., Ltd.
- the lactase activity (FCC IV method) and arylsulfatase activity (by the fluorescence method described in Example 7) of the supernatant were measured.
- the arylsulfatase activity / lactase activity was calculated, and the one with a small value was selected.
- mutant strain (SM1182 strain) was subjected to mutation treatment as a parent strain, and the other arylsulfatase gene also became dysfunctional, that is, a mutant strain having an arylsulfatase activity of 0 was obtained (SF-81 strain) ).
- the parent strain Kriveromyces lactis G14-427 and two mutant strains obtained as described above were each cultured with shaking in a YPD medium (70 mL / flask) at 26 ° C. for 4 days.
- Example 10 Acquisition of host strain A diploid strain, Kriveromyces lactis G14-427, was inoculated into 10 mL of YPD medium by 1 platinum ear and grown at 30 ° C until the logarithmic growth phase. The medium was centrifuged and the cells were collected. The collected cells were dispersed in sterilized water so that the absorbance at 600 nm was 0.5. The bacterial suspension was irradiated with ultraviolet rays for 15 seconds with a UV lamp. The cells were collected by centrifugation and mixed and dispersed in the YPD medium. An appropriate amount was taken from the YPD medium containing the bacterial cells and applied to the YPD agar plate medium. Static culture was performed at 37 ° C. for 4 days. The grown colonies were replicated in SD medium (east nitrogen base containing no 0.67% amino acid, 2% glucose, 2% agar), and those that did not grow were selected.
- SD medium east nitrogen base containing no 0.67% amino acid, 2% glucose, 2%
- the 7-19 strain was inoculated with 1 platinum ear in 10 mL of YPD medium and grown at 30 ° C. until the logarithmic growth phase.
- the medium was centrifuged and the cells were collected.
- the collected cells were dispersed in sterilized water so that the absorbance at 600 nm was 0.5.
- the bacterial suspension was irradiated with ultraviolet rays for 15 seconds with a UV lamp.
- the cells were collected by centrifugation and mixed and dispersed in the YPD medium. An appropriate amount was taken from the YPD medium containing the bacterial cells and applied to the YPD agar plate medium.
- Static culture was performed at 37 ° C. for 4 days. The grown colonies were replicated in an SD medium containing 20 mg / L L-methionine, and those that did not grow were selected.
- Example 11 Acquisition of a gene double disruption strain that does not produce arylsulfatase (acquisition of host strain)
- 8-23 strains which are L-histidine and L-methionine double auxotrophic mutants obtained in Example 10
- their auxotrophy is complemented by the HIS4 gene and the MET6 gene introduced by the lithium acetate method. I was sure that.
- Genomic DNA was prepared from the obtained culture broth using Gen Toroku-kun TM (for yeast) (Takara Bio Inc.). The operation was performed according to the description of Gen Torukun TM (for yeast).
- PCR was performed using the above primers under the following conditions to obtain a DNA fragment.
- Takara Ex Taq registered trademark; manufactured by Takara Bio Inc.
- the polymerase was used as the polymerase, and the operation was performed according to the attached document.
- the obtained fragment was purified by MagExtractor TM -PCR & Gel Clean up- (manufactured by Toyobo Co., Ltd.), and then ligated with a pGEM (registered trademark) -T vector (manufactured by Promega).
- pGEM registered trademark
- -T vector manufactured by Promega
- DNA Ligation Kit ⁇ Mighty Mix> manufactured by Takara Bio Inc.
- Usage was in accordance with each package insert.
- E. coli prepared by the Hanahan method (Hanahan, D., J. Mol. Biol., 166, 557 (1983)).
- a competent cell of ColiDH5 ⁇ strain was transformed, and a plasmid was extracted from the obtained transformant culture solution using MagExtractor TM -Plasmid- (manufactured by Toyobo Co., Ltd.). Usage followed the package insert. As a result, a plasmid pGSuC in which the target fragment was subcloned was obtained.
- PCR was performed using primers BGLHIS4-F and HIS4-R using genomic DNA as a template to obtain a fragment containing the HIS4 gene.
- the method described above was followed.
- the obtained fragment containing the HIS4 gene was treated with Bgl II and EcoRI and inserted into the Bgl II-EcoRI site of pGSuC.
- the plasmid constructed in this way was named pdSuC1.
- Various methods at the time of construction were the same as those described above.
- primers SuCd-M6F and SuCd-M6R were designed by adding 40 bases of the arylsulfatase gene homologous sequence to the 5 'side.
- the homologous sequence of the arylsulfatase gene was in the vicinity of the restriction enzyme ClaI site present in two places on the open reading frame.
- a fragment having an arylsulfatase homologous sequence at both ends of the MET6 gene was obtained using genomic DNA as a template.
- the obtained fragment was subcloned into pGEM (registered trademark) -T vector (Promega) to obtain pdSuCM6.
- pGEM registered trademark
- -T vector Promega
- FIG. 5 shows a schematic diagram of the construction of the transformant.
- the plasmid pdSuC1 is linearized by treatment with NcoI and AatII, and the strain 8-23 is transformed by the lithium acetate method using this, and the transformant SuCD grows in SD medium supplemented with 20 ⁇ g / ml methionine. Acquired shares.
- the plasmid pdSuCM6 was treated with ClaI to form a linear form, and the SuCD strain was transformed by the lithium acetate method using it to obtain a transformant SuCDD5-2 strain that grew on the SD medium.
- genomic DNA was prepared from the culture solution using Gentorikun TM (for yeast) (manufactured by Takara Bio Inc.).
- Gentorikun TM for yeast
- the obtained genomic DNA was digested with BamHI and then subjected to Southern analysis.
- the probe used was an AatII-EcoRI fragment of an arylsulfatase gene, and for labeling and detection of nucleic acids, AlkPhos Direct Labeling and Detection System with CDP-Star (manufactured by GE Healthcare Biosciences) was used. I followed.
- Lane 1 is the parent strain G14-427
- Lane 2 is the transformant SuCDD5-2 strain
- Lane 3 is the transformant SuCD strain.
- lane 3 a band (12.1 kb) of the fragment containing the arylsulfatase gene and the HIS4 gene was detected at the same position (7.8 kb) as in lane 1, and only one of the arylsulfatase genes was destroyed. It was confirmed that On the other hand, in lane 2, the 7.8 kb band was shifted to 5.3 kb, confirming that it was an arylsulfatase gene double disruption strain.
- the culture medium of the SuCDD5-2 strain contains lactase, but does not contain arylsulfatase, or even if it is contained, the amount of the activity may not be detected by fluorescence measurement. It became clear. That is, it was confirmed that the SuCDD5-2 strain maintained lactase productivity but had no or almost no arylsulfatase productivity.
- Example 12 Preparation of enzyme preparation using SF-81 strain and CBS2359 strain SF-81 strain (diploid mutant strain with reduced arylsulfatase production ability) and CBS2359 (haploid) obtained in Example 9
- Each of the strains was inoculated into a medium for producing lactase containing 7% corn steep liquor and 2% lactose, and cultured with shaking at 30 ° C. and 210 rpm for 96 hours, and then the cells were collected by centrifugation. .
- Sterile purified water was added to the cells, and the cell walls of the collected cells were broken with glass beads and ultrasonic waves.
- the mixture containing the microbial cells and purified water thus obtained was centrifuged, and the supernatant was collected.
- the lactase activity in the obtained supernatant was measured by the fluorescence method described in Example 7. As a result, the activity of the SF-81 strain was 100%, and the relative activity of the CBS2359 strain was 2%.
- the supernatant was fractionated with ammonium sulfate and concentrated with an ultrafiltration membrane.
- lactase having a lactase activity of about 1,000, 2,000, 3,000, 4,000, 5,000, and 6,000 NLU / g, respectively, depending on the degree of concentration, from the cells of SF-81 strain.
- a formulation was obtained.
- concentration was performed in the same manner, a preparation showing lactase activity of 1,000 NLU / g or more was not obtained from the CBS2359 strain.
- Example 14 Sensory sensory test (2) (Preparation of lactase preparations with various arylsulfatase contamination rates) The fluorescence method shown in Example 7 by appropriately mixing the lactase preparation itself produced from the SF-81 strain by the method described in Example 13 and GODO-YNL2 (Lactase preparation manufactured by Godo Shusei Co., Ltd .; liquid). Five lactase preparations having an arylsulfatase activity of 1 to 20 U / g as measured in 1 were prepared. Moreover, the lactase activity of each lactase preparation was measured by FCC IV method.
- Example 8 As in Example 8, each of the above 5 lactase preparations was added to commercially available milk so that the lactase was 20,000 NLU / L-milk and stored at 30 ° C. After 1 month of storage, a flavor sensory test was performed in the same manner as in Example 8 to compare milk without the lactase preparation and milk with the lactase preparation. The results are shown in Table 13.
- the arylsulfatase activity measured by the method according to the present invention is preferably 5 U / g or less.
- the ratio of arylsulfatase activity (unit: U / g) measured by the method according to the present invention based on lactase activity (unit: NLU / g) by FCC IV method may be 0.1% or less. It became clear that it was preferable.
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Abstract
Description
(1)アリールスルファターゼの存在が予測される検体を、0.5M塩化カリウムを含む100mMリン酸カリウム緩衝液(pH6.5)で適宜希釈し、サンプルとする。
(2)4-メチルウンベリフェロンスルフェイトカリウムを2mM濃度で含有する水溶液を調製する。
(3)サンプルと4-メチルウンベリフェロンスルフェイトカリウム水溶液とを、1:1(容量基準)で混合し、37℃にて3時間反応させる。
(4)反応液に、反応液と同量(容量基準)の0.1N水酸化ナトリウム水溶液を添加し、反応を停止させ、測定用サンプルとする。
(5)励起波長360nm、蛍光波長450nmにて、蛍光強度を測定する。
(6)4-メチルウンベリフェロンを、0.5M塩化カリウムを含む100mMリン酸カリウム緩衝液(pH6.5)に溶解させ、適切な濃度の溶液とし、(4)と同様に0.1N水酸化ナトリウム水溶液を添加し、(5)と同様の条件で蛍光強度を測定する。
(7)(6)より、検量線を作成する。
(8)(5)で測定された蛍光強度と(7)で作成された検量線から、測定用サンプルの4-メチルウンベリフェロン濃度を算出し、それを3で割り、反応時間が1時間であった場合の4-メチルウンベリフェロン濃度を求める。さらに、反応液の容量から、1時間の反応中に生じた4-メチルウンベリフェロン量を算出する。
(9)こうして算出された4-メチルウンベリフェロン量は、(1)で調製したサンプルに含有されていた検体量に基づくものであるので、検体1g当たりの4-メチルウンベリフェロン量に換算する。
(10)基質と酵素との反応時間1時間あたりの4-メチルウンベリフェロン生成量が1nmoleであった場合を1ユニット(U)とし、単位は、検体、即ち酵素製剤1g当たりのユニット量、即ち「ユニット(U)/g」で表す。
(2)4-メチルウンベリフェロンスルフェイトカリウムを2mM濃度で含有する水溶液を調製する。
(3)サンプルと4-メチルウンベリフェロンスルフェイトカリウム水溶液とを、1:1(容量基準)で混合し、37℃にて3時間反応させる。
(4)反応液に、反応液と同量(容量基準)の0.1N水酸化ナトリウム水溶液を添加し、反応を停止させ、測定用サンプルとする。
(5)励起波長360nm、蛍光波長450nmにて、蛍光強度を測定する。
(6)4-メチルウンベリフェロンを、0.5M塩化カリウムを含む100mMリン酸カリウム緩衝液(pH6.5)に溶解させ、適切な濃度の溶液とし、(4)と同様に0.1N水酸化ナトリウム水溶液を添加し、(5)と同様の条件で蛍光強度を測定する。
(7)(6)より、検量線を作成する。
(8)(5)で測定された蛍光強度と(7)で作成された検量線から、測定用サンプルの4-メチルウンベリフェロン濃度を算出し、それを3で割り、反応時間が1時間であった場合の4-メチルウンベリフェロン濃度を求める。さらに、反応液の容量から、1時間の反応中に生じた4-メチルウンベリフェロン量を算出する。
(9)こうして算出された4-メチルウンベリフェロン量は、(1)で調製したサンプルに含有されていた検体量に基づくものであるので、検体1g当たりの4-メチルウンベリフェロン量に換算する。
(10)基質と酵素との反応時間1時間あたりの4-メチルウンベリフェロン生成量が1nmoleであった場合を1ユニット(U)とし、単位は、検体、即ち酵素製剤1g当たりのユニット量、即ち「ユニット(U)/g」で表す。
GODO-YNL2(合同酒精株式会社製ラクターゼ製剤;液体)を、0、0.2、0.5又は1.0Mの塩化カリウムを含む100mMリン酸カリウム緩衝液(pH6.5)にて5倍希釈した。これらの各液0.5mLに、p-ニトロフェニルスルフェイトの100mMリン酸カリウム緩衝液(pH6.5)0.5mLを加え、37℃で3時間反応させた。これに1.5N水酸化ナトリウム水溶液1.5mLを加えて反応を停止させ、410nmにおいて吸光度を測定した。塩化カリウムを含まない場合を100%として、相対値を表1に示す。
(1) GODO-YNL2(合同酒精株式会社製ラクターゼ製剤;液体)を、0、125、250、500又は1,000mMの塩化ナトリウムを含む100mMリン酸カリウム緩衝液(pH6.5)にて100倍希釈した。これらの各液0.5mLに、2mM 4-メチルウンベリフェロンスルフェイトカリウムの水溶液0.5mLを加え、37℃で3時間反応させた。これに0.1N水酸化ナトリウム水溶液1.0mLを加えて反応を停止させ、励起波長360nm、蛍光波長450nmにて蛍光強度を測定した。塩化ナトリウムを含まない場合を100%として、相対値を表2に示す。
(1) GODO-YNL2(合同酒精株式会社製ラクターゼ製剤;液体)を、100mM、125mM、250mM、500mM及び1,000mMリン酸カリウム緩衝液(pH6.5)にて100倍希釈した。これらの各液0.5mLに、2mM 4-メチルウンベリフェロンスルフェイトカリウムの水溶液0.5mLを加え、37℃で3時間反応させた。これに0.1N水酸化ナトリウム水溶液(100mM、125mM、250mMリン酸カリウム緩衝液の場合)又は1.0N水酸化ナトリウム水溶液(500mM、1,000mMリン酸カリウム緩衝液の場合)1.0mLを加えて反応を停止させ、励起波長360nm、蛍光波長450nmにて蛍光強度を測定した。100mMリン酸カリウム緩衝液を使用した場合を100%として、相対値を表3に示す。
無機塩添加の効果が、酵素反応の亢進によるものであるか、蛍光団の蛍光強度の増強によるものであるのかを確認した。
GODO-YNL2(合同酒精株式会社製ラクターゼ製剤;液体)を蒸留水で希釈し、1%(w/v)溶液を得た。これを、0.5M塩化カリウムを含む100mMリン酸カリウム緩衝液(pH6.5)を用いて希釈し、0.8%(w/v)、0.6%(w/v)、0.4%(w/v)及び0.2%(w/v)溶液を得た。各溶液0.5mLに20mM p-ニトロフェニルスルフェイトの100mMリン酸カリウム緩衝液(pH6.5)溶液0.5mLを加え、37℃で3時間反応させた。これに1.5N水酸化ナトリウム水溶液1.5mLを加えて反応を停止させ、410nmにおける吸光度を測定した。
GODO-YNL2(合同酒精株式会社製ラクターゼ製剤;液体)を0.5M塩化カリウムを含む100mMリン酸カリウム緩衝液(pH6.5)にて希釈し、1%(w/v)溶液を得た。この1%溶液を、同緩衝液を用いて希釈し、0.8%(w/v)、0.6%(w/v)、0.4%(w/v)及び0.2%(w/v)溶液を得た。
アリールスルファターゼ活性測定における比色法と蛍光法との感度の相違を検討した。先ず、この実験で使用する精製ラクターゼを調製した。
GODO-YNL2(合同酒精株式会社製ラクターゼ製剤;液体)50kgを、限外ろ過膜(旭化成株式会社製ACP膜)を用いてその導電率が3mSv以下となるまで加水脱塩した。これに水を加えて全量125Lとした。次いで、あらかじめ10mMリン酸カリウム緩衝液(pH7)にて平衡化しておいたイオン交換樹脂(トーソー株式会社製DEAEトヨパール650M、40cmφ、50L)に吸着させた。50mM塩化ナトリウムを含む10mMリン酸カリウム緩衝液(pH7)40Lにて洗浄し、次いで100mM塩化ナトリウムを含む10mMリン酸カリウム緩衝液(pH7)200Lでラクターゼを溶出させた。この際、フラクションを20Lずつに分画した。各フラクションのラクターゼ活性(FCC IV法による; Food Chemicals Codex 4th Edition, Effective July 1st, 1996, Committee on Food Chemicals Codex, p.p.801-802)及びアリールスルファターゼ活性(蛍光法による;詳細は下記のとおり)を測定し、アリールスルファターゼの低減した画分を回収、混合し、限外ろ過膜(旭化成株式会社製ACP膜)を用いて濃縮し、ラクターゼ濃縮液を得た。この濃縮液に50%(w/w)となるようグリセリンを加え、精製ラクターゼ製剤を得た。
上記のようにして調製した精製ラクターゼ製剤と、GODO-YNL2(合同酒精株式会社製ラクターゼ製剤;液体)を適宜混合して、様々なアリールスルファターゼ夾雑率のラクターゼ製剤を調製し、ラクターゼ活性(FCC IV法による)とアリールスルファターゼ活性(比色法及び蛍光法による)とを測定した。
ラクターゼ製剤0.5mLに20mM p-ニトロフェニルスルフェイトの100mMリン酸カリウム緩衝液(pH6.5)溶液0.5mLを加え、37℃で3時間反応させた。これに1.5N水酸化ナトリウム水溶液1.5mLを加えて反応を停止させ、410nmにおける吸光度を測定した。
ラクターゼ製剤を0.5M塩化カリウムを含む100mMリン酸カリウム緩衝液(pH6.5)で希釈し、1%(w/v)溶液を得た。この1%溶液0.5mLに2mM 4-メチルウンベリフェリルスルフェイトカリウム水溶液0.5mL加え、37℃で3時間反応させた。これに0.1N水酸化ナトリウム水溶液1mLを加えて反応を停止させ、励起波長360nm、蛍光波長450nmにて蛍光強度を測定した。
結果を表6に示す。比色法では、アリールスルファターゼの含有量が少なくなると、測定することができなかったが、蛍光法では、比色法の測定限界の約1/100の濃度域まで正確に測定することができた。
WO07/060247には、夾雑するアリールスルファターゼが19単位(WO07/060247において規定された単位)以下のラクターゼ製剤は、牛乳の滅菌後に乳糖を分解させるために添加された場合に異臭を生じさせない旨が記載されている。しかし、これは、ラクターゼの反応日数を2日間と限定して行った試験の結果に基づく見解である。一方、現実のロングライフミルクにラクターゼ製剤を添加した場合、1ヶ月以上の長期にわたって酵素反応が進行すると考えられる。そこで、様々な夾雑率でアリールスルファターゼを含有するラクターゼ製剤を調製し、それらを牛乳に添加し、所定の日数経過後に風味の確認を行った。
様々な夾雑率のアリールスルファターゼを含有するラクターゼ製剤A乃至Eは、実施例7で調製した精製ラクターゼ製剤と、選択されたアリールスルファターゼ活性を100単位(WO07/060247に記載の単位)含むGODO-YNL2(合同酒精株式会社製ラクターゼ製剤;液体)を適宜混合して調製した。
WO07/060247の実施例4を参照し、市販牛乳(加熱殺菌したもの;殺菌条件:130℃ 2秒)に、ラクターゼが20,000NLU/L-牛乳となるように、ラクターゼ製剤A~Eの各々を加え、30℃に保存した。保存2日後、1ヶ月後及び3ヶ月後に、ラクターゼ製剤を添加していない牛乳とラクターゼ製剤を添加した牛乳の風味官能試験を行った。
二倍体菌株であるクリベロマイセス・ラクティスG14-427株を、YPD培地(1%酵母エキス、1%グルコース、2%ペプトン)10mLに、1白金耳植菌し、この菌懸濁液を30℃に保存して培養し、対数増殖期となったらその培地を遠心分離し、菌体を回収した。回収した菌体を、600nmにおける吸光度が0.5となるように滅菌水に分散させた。この菌懸濁液に、紫外線を、UVランプにて15秒間照射した。遠心分離によって菌体を回収し、YPD培地に混合分散させた。菌体を含むYPD培地から適量を採り、YPD寒天平板培地に塗布した。37℃にて7日間、静置培養を行った。生育してきたコロニーを少量かきとり、これをザイモリエース(生化学バイオビジネス株式会社製)を1mg/mLで含有する溶液1mLに混合した。30℃にて2時間反応させ、細胞壁を破壊した。その後、遠心分離を行い、上清を回収した。
二倍体菌株であるクリベロマイセス・ラクティスG14-427株を、YPD培地10mLに、1白金耳植菌し、30℃にて対数増殖期まで生育させた。培地を遠心分離し、菌体を回収した。回収した菌体を、600nmにおける吸光度が0.5となるように滅菌水に分散させた。この菌懸濁液に、紫外線を、UVランプにて15秒間照射した。遠心分離によって菌体を回収し、YPD培地に混合分散させた。菌体を含むYPD培地から適量を採り、YPD寒天平板培地に塗布した。37℃にて4日間、静置培養を行った。生育してきたコロニーをSD培地(0.67%アミノ酸を含まないイーストナイトロジェンベース、2%グルコース、2%寒天)にレプリカし、生育してこないものを選択した。
(宿主株の取得)
実施例10で取得したL-ヒスチジン、L-メチオニン二重栄養要求性変異株である8-23株について、それぞれの栄養要求性が、酢酸リチウム法にて導入したHIS4遺伝子及びMET6遺伝子により相補されることを確認した。
二倍体菌株であるクリベロマイセス・ラクティスG14-427株をYPD培地にて培養した。得られた培養液より、GenとるくんTM(酵母用)(タカラバイオ株式会社製)を用いてゲノムDNAを調製した。操作は、GenとるくんTM(酵母用)の説明書の記載に従って行った。
アリールスルファターゼ遺伝子のオープン・リーディング・フレームが含まれた断片が取得されるように、プライマーSuC-F及びSuC-Rを設計した。これらを含む、使用したプライマーの配列は、表11に示すとおりであった。
Stage1(1サイクル) 94℃ 3分
Stage2(30サイクル) 94℃ 1分
54℃ 1分
72℃ 3分
Stage3(1サイクル) 72℃ 10分
4℃に保持
図5に、形質転換体構築の模式図を示す。プラスミドpdSuC1を、NcoI及びAatIIで処理して直鎖状にし、それを用いて8-23株を酢酸リチウム法により形質転換し、20μg/mlのメチオニンを添加したSD培地で生育する形質転換体SuCD株を取得した。
得られた形質転換体を、それぞれYPD培地にて培養し、その培養液よりGenとるくんTM(酵母用)(タカラバイオ株式会社製)を用いてゲノムDNAを調製した。得られたゲノムDNAをBamHIで消化後、サザン解析を行った。プローブはアリールスルファターゼ遺伝子のAatII-EcoRI断片を用い、核酸の標識と検出には、AlkPhos Direct Labelling and Detection System with CDP-Star(GEヘルスケア バイオサイエンス株式会社製)を用い、使用法は添付文書に従った。
親株である二倍体菌株のクリベロマイセス・ラクティスG14-427株及び上記のようにして構築したSuCDD5-2株を、それぞれYPD培地に接種し、30℃、210rpmにて72時間、振とう培養した。培養液に2mg/mlとなるようにザイモリエース(生化学バイオビジネス株式会社製)を加え、30℃に2時間反応させ、細胞壁を破壊した。遠心分離により上清を回収し、FCC IV法によってラクターゼ活性を、そして実施例7に記載の方法でアリールスルファターゼ活性を測定した。結果を表12に示す。
実施例9で得たSF-81株(アリールスルファターゼ産生能が低減された二倍体変異株)及びCBS2359(一倍体菌株)を、それぞれ、7%コーンスチーブリカー、2%乳糖を含有するラクターゼ生産用培地に接種し、30℃、210rpmにて96時間、振とう培養し、その後、遠心分離により菌体を回収した。菌体に滅菌精製水を加え、ガラスビーズと超音波により、回収菌体の細胞壁を破壊した。このようにして得られた菌体と精製水等を含む混合物を遠心分離にかけ、上清を回収した。得られた上清中のラクターゼ活性を、実施例7に記載の蛍光法で測定した。その結果、SF-81株の活性を100%として、CBS2359株の相対活性は2%であった。
SF-81株を、7%コーンスチーブリカー、2%乳糖を含有するラクターゼ生産用培地に接種し、30℃、210rpmにて96時間、振とう培養後、遠心分離により菌体を回収した。菌体に滅菌精製水を加え、ガラスビーズと超音波により、回収菌体の細胞壁を破壊し、遠心分離により上清を回収した。上清を硫安分画し、限外ろ過膜で濃縮することにより、ラクターゼ活性が約5,000NLU/gのラクターゼ製剤を得た。このラクターゼ製剤のアリールスルファターゼ活性は、本発明の測定法(蛍光法)によると、1U/g以下であった。
(様々なアリールスルファターゼ夾雑率のラクターゼ製剤の調製)
実施例13に記載の方法でSF-81株から製造したラクターゼ製剤そのもの、及びこれにGODO-YNL2(合同酒精株式会社製ラクターゼ製剤;液体)を適宜混合して、実施例7に示した蛍光法で測定したアリールスルファターゼ活性が1乃至20U/gのラクターゼ製剤5種を調製した。また、各ラクターゼ製剤のラクターゼ活性を、FCC IV法によって測定した。
実施例8同様、市販牛乳に、ラクターゼが20,000NLU/L-牛乳となるように、上記ラクターゼ製剤5種の各々を加え、30℃に保存した。保存1ヶ月後に、ラクターゼ製剤を添加していない牛乳とラクターゼ製剤を添加した牛乳を比較する風味官能試験を、実施例8と同様の方法で行った。結果を表13に示す。
Claims (15)
- アリールスルファターゼを、その基質であって、当該基質がアリールスルファターゼの作用を受けると蛍光団又は発色団を遊離するものとを、イオン強度の高い水系反応系中で反応させることを特徴とする、水系でのアリールスルファターゼの活性測定方法。
- イオン強度の高い水系反応系中で反応させる手段が、無機塩が添加されてなる水系反応系中で酵素と基質と反応させることであるか、及び/又は、酵素蛋白を変性させない緩衝液系中で酵素と基質とを反応させることである、請求項1に記載の水系でのアリールスルファターゼの活性測定方法。
- 水系反応系中の無機塩濃度が50乃至500mMである、及び/又は、緩衝液濃度が50乃至200mMである、請求項2に記載の水系でのアリールスルファターゼの活性測定方法。
- 無機塩が、塩化カリウム、塩化ナトリウム及び硫酸アンモニウムからなる群から選択される一種以上である、請求項2又は3に記載の水系でのアリールスルファターゼの活性測定方法。
- 緩衝液がリン酸塩緩衝液である、請求項2乃至4のいずれか一項に記載の水系でのアリールスルファターゼの活性測定方法。
- 以下の工程(1)乃至(10)を含む、請求項1に記載の水系でのアリールスルファターゼの活性測定方法:
(1)アリールスルファターゼの存在が予測される検体を、0.5M塩化カリウムを含む100mMリン酸カリウム緩衝液(pH6.5)で適宜希釈し、サンプルとする。
(2)4-メチルウンベリフェロンスルフェイトカリウムを2mM濃度で含有する水溶液を調製する。
(3)サンプルと4-メチルウンベリフェロンスルフェイトカリウム水溶液とを、1:1(容量基準)で混合し、37℃にて3時間反応させる。
(4)反応液に、反応液と同量(容量基準)の0.1N水酸化ナトリウム水溶液を添加し、反応を停止させ、測定用サンプルとする。
(5)励起波長360nm、蛍光波長450nmにて、蛍光強度を測定する。
(6)4-メチルウンベリフェロンを、0.5M塩化カリウムを含む100mMリン酸カリウム緩衝液(pH6.5)に溶解させ、適切な濃度の溶液とし、(4)と同様に0.1N水酸化ナトリウム水溶液を添加し、(5)と同様の条件で蛍光強度を測定する。
(7)(6)より、検量線を作成する。
(8)(5)で測定された蛍光強度と(7)で作成された検量線から、測定用サンプルの4-メチルウンベリフェロン濃度を算出し、それを3で割り、反応時間が1時間であった場合の4-メチルウンベリフェロン濃度を求める。さらに、反応液の容量から、1時間の反応中に生じた4-メチルウンベリフェロン量を算出する。
(9)こうして算出された4-メチルウンベリフェロン量は、(1)で調製したサンプルに含有されていた検体量に基づくものであるので、検体1g当たりの4-メチルウンベリフェロン量に換算する。
(10)基質と酵素との反応時間1時間あたりの4-メチルウンベリフェロン生成量が1nmoleであった場合を1ユニット(U)とし、単位は、検体、即ち酵素製剤1g当たりのユニット量、即ち「ユニット(U)/g」で表す。 - ラクターゼ製剤中のアリールスルファターゼの活性測定方法である、請求項1乃至6のいずれか一項に記載の水系でのアリールスルファターゼの活性測定方法。
- ラクターゼ遺伝子を有し且つアリールスルファターゼ蛋白の発現が制限されている酵母の二倍体菌株又は酵母のラクターゼ遺伝子が導入され且つアリールスルファターゼ蛋白の発現が制限されている遺伝子組換え微生物の培養後の菌体又は微生物体及び/又は培養液を原料として製造されたラクターゼ製剤であって、当該ラクターゼ製剤は、FCC IV法によるラクターゼ活性が4,000NLU/g以上であり、且つ、当該ラクターゼ活性を基準として、請求項6に記載の方法で測定し、計算したアリールスルファターゼ活性(単位:U/g)が0.1%以下であることを特徴とするラクターゼ製剤。
- アリールスルファターゼの除去工程なしに製造されたものである、請求項8に記載のラクターゼ製剤。
- FCC IV法によるラクターゼ活性(単位:NLU/g)を基準としたアリールスルファターゼ活性(単位:U/g)が0.02%以下である、請求項8又は9に記載のラクターゼ製剤。
- ラクターゼ遺伝子を有し且つアリールスルファターゼ蛋白の発現が制限されている酵母の二倍体菌株が、ラクターゼ遺伝子を有する酵母の二倍体菌株の変異処理によって取得された変異株である、請求項8乃至10のいずれか一項に記載のラクターゼ製剤。
- ラクターゼ遺伝子を有し且つアリールスルファターゼ蛋白の発現が制限されている酵母の二倍体菌株が、ラクターゼ遺伝子を有する酵母の二倍体菌株の、アリールスルファターゼ遺伝子又はアリールスルファターゼ蛋白発現調節遺伝子の欠失操作によって得られた変異株である、請求項8乃至10のいずれか一項に記載のラクターゼ製剤。
- 酵母の二倍体菌株が、クリベロマイセス・ラクティス又はクリベロマイセス・マリキシアヌスである、請求項8乃至12のいずれか一項に記載のラクターゼ製剤。
- ラクターゼ遺伝子を有し且つアリールスルファターゼ蛋白の発現が制限されている酵母の二倍体菌株又は酵母のラクターゼ遺伝子が導入され且つアリールスルファターゼ蛋白の発現が制限されている遺伝子組換え微生物を培養し、細胞壁を破壊せずに菌体又は微生物体を回収するか、細胞壁を破壊して菌体又は微生物体と共に培養液を回収するか、あるいは、細胞壁を破壊せずに培養液を回収し、回収した菌体又は微生物体及び/又は培養液を原料として、アリールスルファターゼの除去工程なしに、FCC IV法によるラクターゼ活性が4,000NLU/g以上であり、且つ、当該ラクターゼ活性を基準として、請求項6に記載の方法で測定し、計算したアリールスルファターゼ活性(単位:U/g)が0.1%以下であるラクターゼ製剤を製造することを特徴とする、ラクターゼ製剤の製造方法。
- 請求項8乃至13のいずれか一項に記載されたラクターゼ製剤を用いて製造されたことを特徴とする乳製品。
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DK12758277.3T DK2687598T3 (en) | 2011-03-14 | 2012-03-13 | Method for assaying arylsulfatase activity |
ES12758277.3T ES2617508T3 (es) | 2011-03-14 | 2012-03-13 | Método para determinar actividad de arilsulfatasa |
US14/004,687 US20140087404A1 (en) | 2011-03-14 | 2012-03-13 | Method for assaying arylsulfatase activity |
JP2013504727A JP6013321B2 (ja) | 2011-03-14 | 2012-03-13 | アリールスルファターゼの活性測定方法 |
EP12758277.3A EP2687598B1 (en) | 2011-03-14 | 2012-03-13 | Method for assaying arylsulfatase activity |
US15/296,254 US20170029865A1 (en) | 2011-03-14 | 2016-10-18 | Method for assaying arylsulfatase activity |
US16/129,495 US20190040446A1 (en) | 2011-03-14 | 2018-09-12 | Method for assaying arylsulfatase activity |
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WO2014185364A1 (ja) * | 2013-05-13 | 2014-11-20 | 合同酒精株式会社 | ラクターゼ含有組成物の製造法 |
EP2687598B1 (en) | 2011-03-14 | 2017-02-15 | Godo Shusei Co., Ltd. | Method for assaying arylsulfatase activity |
WO2017073723A1 (ja) * | 2015-10-29 | 2017-05-04 | 合同酒精株式会社 | 乳または乳製品 |
JP2019528740A (ja) * | 2016-09-19 | 2019-10-17 | プロラクタ バイオサイエンス,インコーポレイテッド | 精製ヒトミルクオリゴ糖組成物 |
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CA2946614C (en) | 2005-11-28 | 2021-01-26 | Dsm Ip Assets B.V. | Enzyme preparations yielding a clean taste |
CN110632052A (zh) * | 2019-10-25 | 2019-12-31 | 山西师范大学 | 土壤芳基硫酸酯酶活性的荧光光谱检测法 |
CN110749489B (zh) * | 2019-11-21 | 2021-11-02 | 中南林业科技大学 | 一种快速检测葛仙米种子活性的方法 |
JPWO2023038057A1 (ja) * | 2021-09-07 | 2023-03-16 |
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Cited By (7)
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EP2687598B1 (en) | 2011-03-14 | 2017-02-15 | Godo Shusei Co., Ltd. | Method for assaying arylsulfatase activity |
WO2014185364A1 (ja) * | 2013-05-13 | 2014-11-20 | 合同酒精株式会社 | ラクターゼ含有組成物の製造法 |
JPWO2014185364A1 (ja) * | 2013-05-13 | 2017-02-23 | 合同酒精株式会社 | ラクターゼ含有組成物の製造法 |
WO2017073723A1 (ja) * | 2015-10-29 | 2017-05-04 | 合同酒精株式会社 | 乳または乳製品 |
JP2019004701A (ja) * | 2015-10-29 | 2019-01-17 | 合同酒精株式会社 | 乳または乳製品 |
JP2019528740A (ja) * | 2016-09-19 | 2019-10-17 | プロラクタ バイオサイエンス,インコーポレイテッド | 精製ヒトミルクオリゴ糖組成物 |
JP7143286B2 (ja) | 2016-09-19 | 2022-09-28 | プロラクタ バイオサイエンス,インコーポレイテッド | 精製ヒトミルクオリゴ糖組成物 |
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DK2687598T3 (en) | 2017-05-22 |
EP2687598A4 (en) | 2014-09-24 |
JP2016208998A (ja) | 2016-12-15 |
US20140087404A1 (en) | 2014-03-27 |
US20190040446A1 (en) | 2019-02-07 |
ES2617508T3 (es) | 2017-06-19 |
JP6013321B2 (ja) | 2016-10-25 |
EP2687598A1 (en) | 2014-01-22 |
EP2687598B1 (en) | 2017-02-15 |
JPWO2012124668A1 (ja) | 2014-07-24 |
US20170029865A1 (en) | 2017-02-02 |
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