WO2007003027A1 - A method of the removal of monosaccharide in oligosaccharides production - Google Patents

A method of the removal of monosaccharide in oligosaccharides production Download PDF

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Publication number
WO2007003027A1
WO2007003027A1 PCT/CA2005/001023 CA2005001023W WO2007003027A1 WO 2007003027 A1 WO2007003027 A1 WO 2007003027A1 CA 2005001023 W CA2005001023 W CA 2005001023W WO 2007003027 A1 WO2007003027 A1 WO 2007003027A1
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WO
WIPO (PCT)
Prior art keywords
oligosaccharides
yeast
monosaccharide
removal
content
Prior art date
Application number
PCT/CA2005/001023
Other languages
French (fr)
Inventor
Zhensheng Zhong
Jianhua Zhu
Xiaolin Li
Xiaoyan Xu
Xiaomei Mu
Original Assignee
Advance Will Technology Ltd.
1172592 Alberta Ltd.
Priority date (The priority date is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the date listed.)
Filing date
Publication date
Application filed by Advance Will Technology Ltd., 1172592 Alberta Ltd. filed Critical Advance Will Technology Ltd.
Priority to PCT/CA2005/001023 priority Critical patent/WO2007003027A1/en
Publication of WO2007003027A1 publication Critical patent/WO2007003027A1/en

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    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12PFERMENTATION OR ENZYME-USING PROCESSES TO SYNTHESISE A DESIRED CHEMICAL COMPOUND OR COMPOSITION OR TO SEPARATE OPTICAL ISOMERS FROM A RACEMIC MIXTURE
    • C12P19/00Preparation of compounds containing saccharide radicals
    • C12P19/02Monosaccharides

Definitions

  • the present invention relates to a method for the removal of monosaccharide in oligosaccharides production.
  • the method is used to remove monosaccharide from oligosaccharides by yeast fermentation reaction.
  • the oligosaccharides are a new generation of functional food or health food ingredient with special physiological effects which can promote the proliferation of colonic Liacteria of genus Bifidobacterium to balance the microbial ecology of the microflora in gastrointestinal tract of human being, suppress the growth of undesirable bacteria and function as an anti-dental caries.
  • Oligosaccharides are a type of sweetener that is not absorbed or digested in the small intestine of man. Oligosaccharides are low in calories and can be used as conventional diet sweeteners such as those used by middle-age and older people who are on special diets due to diabetes.
  • Oligosaccharides are carbohydrates consisting of 3 to 5 monosaccharides linked together. There are two main methods to produce oligosaccharides. One method involves the application of retrosynthetic reaction of amylase with which the monosaccharides (glucose) are condensed to oligosaccharides. Normally the content of G3 to G5 in the final product is 20% - 30% with some other complicated components. G3 and G5 refer to Glucose units. By way of example, G3 refers to a sugar which is comprised of three glucose units linked together as one component.
  • the other way to make oligosaccharides is the enzymatic hydrolysis method in which the starch is hydrolyzed to polysaccharides first by ⁇ -amylases, and then the polysaccharides are further hydrolyzed to oligosaccharides by glucosidase or other enzymes with transglucosylation function.
  • the enzymatic hydrolysis method is the main process. It is based on starch as raw material. The process comprises two steps. The first step is to get the maltose syrup through starch hydrolysis with ⁇ -amylases. The second step is to get the target product through transglucosylation with the co-reaction of two or three kinds of enzymes, and then the routine filtration, decolouration, desalting and concentration processes are applied to get the final product.
  • oligosaccharides Currently, the normal content of oligosaccharides is about 50% - 60%.
  • the other main components are glucose and maltose which make about 50% of the final product.
  • the glucose and maltose can disturb the two main health benefits of oligosaccharides product.
  • One is the proliferation of beneficial microbiota Bifidobacteria species in the gastrointestinal tract of humans, and the other is the anti-dental caries benefit. As a result, the health benefits and commercial value of the oligosaccharides product are significantly reduced.
  • oligosaccharides with high purity can be obtained by a separation process from the raw oligosaccharides product.
  • the membrane separation process removes the monosaccharides and disaccharide from the product and keeps the other sugars components with bigger molecular weights, so that the content of oligosaccharides is increased to about 80%.
  • the other method is the adsorption separation process.
  • the absorption separation process involves removing the monosaccharide and disaccharide by ion exchange columns.
  • the content of oligosaccharides can be increased to 60% - 70% by one recycle operation.
  • the disadvantage of this method is that capacity of the columns is low for the single recycle so that multiple recycle adsorption processes are needed to get the high purity oligosaccharides product.
  • a method for removal of the monosaccharide in oligosaccharides production includes the step of culturing the yeast.
  • a further step involves mixing 8%- 12% (WAV) of yeast based on the weight of oligosaccharides and 0.1%-O.5% (WAV) of carbamide as nitrogen source with raw oligosaccharide syrup, and then adjusting the pH value to 4.5 - 6.0.
  • a further step involves culturing the above oligosaccharides syrup at 23 0 C - 26°C for 20 -30 hours with intermittent agitation.
  • the method removes the monosaccharide and disaccharide from raw oligosaccharides by microbial metabolism technology so that the purity and the content of G3 to G5 in oligosaccharides are significantly increased. Oligosaccharides with high purity are thereby obtained at a low cost in terms of equipment and operation.
  • the method can utilize the raw material economically and simplify the commercial process to produce oligosaccharides with high purity.
  • the present invention provides a method for removal of the monosaccharide in oligosaccharides production with selectively microbial metabolism by yeast, with which the purity and the content of G3 to G5 in oligosaccharides is significantly increased.
  • the oligosaccharides with high purity can be obtained at a low cost in terms of equipment and operation.
  • the method economically utilizes the raw material and simplifies the industrial process to produce oligosaccharides with high purity.
  • the method for removal of the monosaccharide in oligosaccharides production involves the step of activating the yeast with malt extract medium, and then culturing the yeast with glucose growth medium. A further step involves mixing 8% - 12% of the yeast
  • Another step involves fermenting the oligosaccharides mixture for 20 to 30 hours at temperature of between 23 0 C - 26 °C with intermittent agitation.
  • the yeast is As 2.109 Yeast.
  • the oligosaccharide is the isomaltooligosaccharides with 75% of solid content and the chemical used for pH adjustment is hydrogen chloride.
  • oligosaccharides Based on the weight of oligosaccharides with content of 75%, As 2.109 yeast was first activated with malt extract medium, and then the yeast was cultured with glucose growth medium. Then 10% (V yeast /Monosaccha r ides) of the yeast was added to the raw oligosaccharides liquid, followed by 0.2% (W C arbmide/W o iig O s ⁇ ciiarides) of carbamide as nitrogen source was mixed with this oligosaccharides liquid. Hydrogen chloride was used to adjust the pH to 5.2. The oligosaccharides mixture was fermented for 22 hours at temperature of 23 0 C with intermittent agitation. The samples were analyzed on-line by
  • G2 was 4.2%, and the content of oligosaccharides was 92.56%.
  • oligosaccharides Based on the weight of oligosaccharides with content of 75%, As 2.109 yeast was first activated with malt extract medium, and then the yeast was cultured with glucose growth medium. Then 9.0 % (VyeastA/Oiigosaccha ⁇ des) of the yeast was added into the raw oligosaccharides liquid, and followed by 0.5% (Wcarbamide/Woiigosacoha ⁇ des ) of carbamide as nitrogen source was mixed with this oligosaccharides liquid. Hydrogen chloride was used to adjust the pH to 5.8. The oligosaccharides mixture was fermented for 30 hours at temperature of 26 0 C with intermittent agitation. The samples were analyzed on-line by HPLC to follow the sugar components. The content of glucose GI was 0%, the maltose G2 was 3.10 %, and the content of oligosaccharides was 93.35 %.

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  • Engineering & Computer Science (AREA)
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  • Chemical Kinetics & Catalysis (AREA)
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  • General Chemical & Material Sciences (AREA)
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  • Health & Medical Sciences (AREA)
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  • Bioinformatics & Cheminformatics (AREA)
  • General Engineering & Computer Science (AREA)
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  • Coloring Foods And Improving Nutritive Qualities (AREA)
  • Preparation Of Compounds By Using Micro-Organisms (AREA)

Abstract

A method for removal of the monosaccharide in oligosaccharides production which includes the step of culturing the yeast. A further step involves mixing 8%- 12% (W/W) of yeast based on the weight of oligosaccharides and 0.1%-0.5% (W/W) of carbamide as nitrogen source with raw oligosaccharide syrup, and then adjusting the pH value to 4.5 - 6.0. A further step involves culturing the above oligosaccharides syrup at 23°C - 26°C for 20 -30 hours with intermittent agitation.

Description

TITLE OF THE INVENTION;
A Method for the Removal of Monosaccharide in Oligosaccharides Production.
FIELD OF THE INVENTION The present invention relates to a method for the removal of monosaccharide in oligosaccharides production. The method is used to remove monosaccharide from oligosaccharides by yeast fermentation reaction.
BACKGROUND OF THE INVENTION
The oligosaccharides are a new generation of functional food or health food ingredient with special physiological effects which can promote the proliferation of colonic Liacteria of genus Bifidobacterium to balance the microbial ecology of the microflora in gastrointestinal tract of human being, suppress the growth of undesirable bacteria and function as an anti-dental caries. Oligosaccharides are a type of sweetener that is not absorbed or digested in the small intestine of man. Oligosaccharides are low in calories and can be used as conventional diet sweeteners such as those used by middle-age and older people who are on special diets due to diabetes.
Oligosaccharides are carbohydrates consisting of 3 to 5 monosaccharides linked together. There are two main methods to produce oligosaccharides. One method involves the application of retrosynthetic reaction of amylase with which the monosaccharides (glucose) are condensed to oligosaccharides. Normally the content of G3 to G5 in the final product is 20% - 30% with some other complicated components. G3 and G5 refer to Glucose units. By way of example, G3 refers to a sugar which is comprised of three glucose units linked together as one component. The other way to make oligosaccharides is the enzymatic hydrolysis method in which the starch is hydrolyzed to polysaccharides first by α-amylases, and then the polysaccharides are further hydrolyzed to oligosaccharides by glucosidase or other enzymes with transglucosylation function. Currently, the enzymatic hydrolysis method is the main process. It is based on starch as raw material. The process comprises two steps. The first step is to get the maltose syrup through starch hydrolysis with α-amylases. The second step is to get the target product through transglucosylation with the co-reaction of two or three kinds of enzymes, and then the routine filtration, decolouration, desalting and concentration processes are applied to get the final product.
Currently, the normal content of oligosaccharides is about 50% - 60%. The other main components are glucose and maltose which make about 50% of the final product. The glucose and maltose can disturb the two main health benefits of oligosaccharides product. One is the proliferation of beneficial microbiota Bifidobacteria species in the gastrointestinal tract of humans, and the other is the anti-dental caries benefit. As a result, the health benefits and commercial value of the oligosaccharides product are significantly reduced.
Normally, oligosaccharides with high purity can be obtained by a separation process from the raw oligosaccharides product.
One of separation methods is the membrane separation process. The membrane separation process removes the monosaccharides and disaccharide from the product and keeps the other sugars components with bigger molecular weights, so that the content of oligosaccharides is increased to about 80%. There are problems with this process including the high cost of expensive equipment, low efficiency and difficulties in commercial production. The other method is the adsorption separation process. The absorption separation process involves removing the monosaccharide and disaccharide by ion exchange columns. The content of oligosaccharides can be increased to 60% - 70% by one recycle operation. The disadvantage of this method is that capacity of the columns is low for the single recycle so that multiple recycle adsorption processes are needed to get the high purity oligosaccharides product.
SUMMARY OF THE INVENTION
What is required is a method for the removal of monosaccharide in oligosaccharides production to enhance the health benefits of the resulting product.
According to the present invention there is provided a method for removal of the monosaccharide in oligosaccharides production. The method includes the step of culturing the yeast. A further step involves mixing 8%- 12% (WAV) of yeast based on the weight of oligosaccharides and 0.1%-O.5% (WAV) of carbamide as nitrogen source with raw oligosaccharide syrup, and then adjusting the pH value to 4.5 - 6.0. A further step involves culturing the above oligosaccharides syrup at 230C - 26°C for 20 -30 hours with intermittent agitation.
The method removes the monosaccharide and disaccharide from raw oligosaccharides by microbial metabolism technology so that the purity and the content of G3 to G5 in oligosaccharides are significantly increased. Oligosaccharides with high purity are thereby obtained at a low cost in terms of equipment and operation. The method can utilize the raw material economically and simplify the commercial process to produce oligosaccharides with high purity. DETAILED DESCRIPTION OF THE PREFERRED EMBODIMENT
The present invention provides a method for removal of the monosaccharide in oligosaccharides production with selectively microbial metabolism by yeast, with which the purity and the content of G3 to G5 in oligosaccharides is significantly increased. The oligosaccharides with high purity can be obtained at a low cost in terms of equipment and operation. The method economically utilizes the raw material and simplifies the industrial process to produce oligosaccharides with high purity.
The method for removal of the monosaccharide in oligosaccharides production involves the step of activating the yeast with malt extract medium, and then culturing the yeast with glucose growth medium. A further step involves mixing 8% - 12% of the yeast
(WAV) based on the weight of oligosaccharides and 0.1 % 0.5% of carbamide as nitrogen source with raw oligosaccharides liquid, and then adjusting the pH to 4.5 - 6.0.
Another step involves fermenting the oligosaccharides mixture for 20 to 30 hours at temperature of between 23 0C - 26 °C with intermittent agitation.
With the method described above , the yeast is As 2.109 Yeast. The oligosaccharide is the isomaltooligosaccharides with 75% of solid content and the chemical used for pH adjustment is hydrogen chloride.
The method described above, removes the monosaccharide and disaccharide from raw oligosaccharides by microbial metabolism technology so that the purity and the content of G3 to G5 in oligosaccharides are significantly increased. Oligosaccharides with high purity are obtained with low costs in terms of equipment and operation. The technology economically utilizes the raw material and simplifies the process to commercially produce oligosaccharides with high purity. DESCRIPTION OF EXAMPLES
Application Example 1:
Based on the weight of oligosaccharides with content of 75%, As 2.109 yeast was first activated with malt extract medium, and then the yeast was cultured with glucose growth medium. Then 10% (Vyeast /Monosaccharides) of the yeast was added to the raw oligosaccharides liquid, followed by 0.2% (WCarbmide/WoiigOs∞ciiarides) of carbamide as nitrogen source was mixed with this oligosaccharides liquid. Hydrogen chloride was used to adjust the pH to 5.2. The oligosaccharides mixture was fermented for 22 hours at temperature of 230C with intermittent agitation. The samples were analyzed on-line by
HPLC to follow the sugar components. The content of glucose GI was 0%, the maltose
G2 was 4.2%, and the content of oligosaccharides was 92.56%.
Application Example 2: Based on the weight of oligosaccharides with content of 75%, As 2.109 yeast was first activated with malt extract medium, and then the yeast was cultured with glucose growth medium. Then 11% (Vyeast/Noiigosaccharides) of the yeast was added to the raw oligosaccharides liquid, and followed 0.3 % (WcarbamideAVoiigosacchaπdes ) °f carbamide as nitrogen source was mixed with this oligosaccharides liquid. Hydrogen chloride was used to adjust the pH to 4.8. The oligosaccharides mixture was fermented for 25 hours at temperature of 25 °C with intermittent agitation. The samples were analyzed on-line by HPLC to follow the sugar components. The content of glucose GI was 0%, the maltose G2 was 5.3 %, and the content of oligosaccharides was 94.5 %.
Application Example 3 :
Based on the weight of oligosaccharides with content of 75%, As 2.109 yeast was first activated with malt extract medium, and then the yeast was cultured with glucose growth medium. Then 9.0 % (VyeastA/Oiigosacchaπdes) of the yeast was added into the raw oligosaccharides liquid, and followed by 0.5% (Wcarbamide/Woiigosacohaπdes ) of carbamide as nitrogen source was mixed with this oligosaccharides liquid. Hydrogen chloride was used to adjust the pH to 5.8. The oligosaccharides mixture was fermented for 30 hours at temperature of 260C with intermittent agitation. The samples were analyzed on-line by HPLC to follow the sugar components. The content of glucose GI was 0%, the maltose G2 was 3.10 %, and the content of oligosaccharides was 93.35 %.
In this patent document, the word "comprising" is used in its non-limiting sense to mean that items following the word are included, but items not specifically mentioned are not excluded. A reference to an element by the indefinite article "a" does not exclude the possibility that more than one of the element is present, unless the context clearly requires that there be one and only one of the elements.
It will be apparent to one skilled in the art that modifications may be made to the illustrated embodiment without departing from the spirit and scope of the invention as hereinafter defined in the Claims.

Claims

THE EMBODIMENTS OF THE INVENTION IN WHICH AN EXCLUSIVE PROPERTY OR PRIVBLEGE IS CLAIMED ARE DEFINED AS FOLLOWS:
1. A method for removal of monosaccharide in oligosaccharides production, the method comprising:
(1). Activating the yeast with malt extract medium, and then culturing the yeast with glucose growth medium;
(2). Mixing 8% - 12% of the yeast (W/W) based on the weight of oligosaccarides and 0.1 % -0.5% of carbamide as nitrogen source with raw oligosaccharides, and then adjusting the pH to 4.5 - 6.0;
(3). Fermenting the above oligosaccharides mixture for 20 - 30 hours at temperature of 23°C 26 °C with intermittent agitation.
2. The method according to claim 1 wherein said yeast is As 2.109 Yeast.
3. The method according to claim 1 and claim 2 wherein the oligosaccharide is the isomaltooligosaccharides with 75% of solid content.
4. The method according to claim 1 and claim 2 wherein the chemical used for pH adjusting is hydrogen chloride.
5. The method according to claim 3 wherein the chemical used for pH adjusting is hydrogen chloride.
PCT/CA2005/001023 2005-06-30 2005-06-30 A method of the removal of monosaccharide in oligosaccharides production WO2007003027A1 (en)

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Citations (3)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
JPH09143191A (en) * 1995-11-22 1997-06-03 Nichiden Kagaku Kk Decomposed starch and its production
CN1231289A (en) * 1998-04-07 1999-10-13 孟松林 Process for producing isomalt oligosaccharide
CN1557956A (en) * 2004-01-15 2004-12-29 华南理工大学 Method for dispelling monosaccharide component from oligosaccharide

Patent Citations (5)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
JPH09143191A (en) * 1995-11-22 1997-06-03 Nichiden Kagaku Kk Decomposed starch and its production
CN1231289A (en) * 1998-04-07 1999-10-13 孟松林 Process for producing isomalt oligosaccharide
CN1557956A (en) * 2004-01-15 2004-12-29 华南理工大学 Method for dispelling monosaccharide component from oligosaccharide
CA2474999A1 (en) * 2004-01-15 2005-07-15 Bioneutra Inc. A method for the removal of monosaccharide in oligosaccharides production
US20050181486A1 (en) * 2004-01-15 2005-08-18 Zhensheng Zhong Method for the removal of monosaccharide in oligosaccharides production

Non-Patent Citations (1)

* Cited by examiner, † Cited by third party
Title
ZHONG Z. ET AL.: "Screening of yeast strain for purifying isomalto-oligosaccharide and its fermentation condition", WUXI QINGGONG DAXUE XUEBAO BIANJIBU, vol. 23, no. 2, March 2004 (2004-03-01), pages 45 - 48, XP008074801 *

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