CA2117472C - Process for isomerization of compound of aldose structure into compound of ketose structure, and isomerization agent or accelerator used therein - Google Patents
Process for isomerization of compound of aldose structure into compound of ketose structure, and isomerization agent or accelerator used therein Download PDFInfo
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Abstract
The present invention provides a process which comprises isomerizing a compound having an aldose structure into a compound having a ketose structure, by the use of or in the presence of an organogermanium compound having a structural portion represented by formula (I) and m isomerization agent or accelerator effective for the isomerization of a compound having an aldose structure in a compound having a ketose structure, which agent or accelerator comprises, as an active component an organogermanium compound having a structural portion represented by formula (I). Owing to the use or presence of the above organogermanium compound, said process is free from the problems of prior art and capable of isomerizing a compomd having an aldose structure into a compound having a ketose structure at a high isomerization ratio without requiring any special apparatus or any complicated operation.
Description
CA2 i i 7472 DESCRIPTION
Process for Isomerization of Compound of Aldose Structure into Compound of Ketose Structure, and Isomerization Agent or Accelerator Used Therein Technical Field The present invention relates to a process for isomerizing a compound having an aldose structure into a compound having a ketose structure, as well as to an isomerization agent or accelerator used in said process.
Background Art Carbohydrates are organic compounds which are very important to living things as their energy sources, etc. and which are present most abundantly on the earth.
They are composed mainly of monosaccharides. These monosaccharides have typical structures in which 3 to 8 carbon atoms are bonded in a ring and the structures are largely classified into two types.
That is, said structures are classified into al-dose (an aldehyde-containing monosaccharide) and ketose (a ketone-containing monosaccharide). Both aldose and ketose are further classified into respective trioses, tetroses, pentoses and hexoses depending upon the carbon atom number of aldose or ketose.
Various reactions using monosaccharides are known. As such a reaction which is used industrially, CA2ii7472 there is a reaction which comprises isomerizing glucose (grape sugar) (an aldohexose) into fructose (fruit sugar) (a corresponding ketohexose) to produce a high-fructose syrup.
Said high-fructose syrup is a mixture of glucose and fructose, obtained by isomerizing glucose partially.
Owing to the partial isomerization of glucose (having low sweetness) into fructose (having high sweetness), the high-fructose syrup has sweetness similar to that of sucrose.
About 70~ of the high-fructose syrup is used in cooling drinks and other drinks because fructose con-tained therein has higher sweetness at lower tempera-tures, and other portion is used in general foodstuffs as a sweetener. The yearly production of high-fructose syrup in the world is estimated about 8,000,000 kg.
Both glucose and fructose are hexoses similar in structure. Chemical and enzymatic processes have hith-erto been proposed for isomerization of glucose into fructose, and it is currently conducted in industry to isomerize glucose into fructose using an isomerization enzyme, namely, glucose isomerase to produce a high-fructose syrup.
That is, starch, for example, corn starch is liquefied; the resulting liquid is subjected to sacchar-ification using glucoamylase to obtain a starch syrup;
and passing the starch syrup continuously through an im-mobilized enzyme obtained by immobilizing, using one of CAZi various methods, a glucose isomerase produced by, a mi-croorganism of, for example, Streptomyces genus, to iso-merize the glucose contained in said solution into fruc-tose.
The above isomerization reaction is an equilib-rium reaction whose equilibrium point is 1 or there-abouts. At the equilibrium point, about 50% of glucose can be isomerized into fructose at a reaction tempera-ture of about 60°C. In order to allow the isomerization to proceed to such a level, however, a considerable length of time is required, the reaction mixture is col-ored owing to the heating for such a long time, and a high cost is incurred for the purification and condensa-tion steps required for product marketing. Hence, the reaction is terminated when the isomerization has pro-ceeded to a fructose content of about 42%.
As described above, the high-fructose syrup is produced in order to allow glucose of mass production and low cost to have sweetness similar to that of su-crose. However, when the sweetness of sucrose is arbi-trarily taken as 100, the above-mentioned high-fructose syrup containing about 42% of fructose (this fructose syrup is hereinafter referred to as 42%-fructose syrup, in some cases) has a sweetness of 95-100 which is slightly insufficient. Therefore, in the above isomer-~ ization reaction alone, it is impossible to directly ob-tain a high-fructose syrup having the same sweetness as sucrose.
Process for Isomerization of Compound of Aldose Structure into Compound of Ketose Structure, and Isomerization Agent or Accelerator Used Therein Technical Field The present invention relates to a process for isomerizing a compound having an aldose structure into a compound having a ketose structure, as well as to an isomerization agent or accelerator used in said process.
Background Art Carbohydrates are organic compounds which are very important to living things as their energy sources, etc. and which are present most abundantly on the earth.
They are composed mainly of monosaccharides. These monosaccharides have typical structures in which 3 to 8 carbon atoms are bonded in a ring and the structures are largely classified into two types.
That is, said structures are classified into al-dose (an aldehyde-containing monosaccharide) and ketose (a ketone-containing monosaccharide). Both aldose and ketose are further classified into respective trioses, tetroses, pentoses and hexoses depending upon the carbon atom number of aldose or ketose.
Various reactions using monosaccharides are known. As such a reaction which is used industrially, CA2ii7472 there is a reaction which comprises isomerizing glucose (grape sugar) (an aldohexose) into fructose (fruit sugar) (a corresponding ketohexose) to produce a high-fructose syrup.
Said high-fructose syrup is a mixture of glucose and fructose, obtained by isomerizing glucose partially.
Owing to the partial isomerization of glucose (having low sweetness) into fructose (having high sweetness), the high-fructose syrup has sweetness similar to that of sucrose.
About 70~ of the high-fructose syrup is used in cooling drinks and other drinks because fructose con-tained therein has higher sweetness at lower tempera-tures, and other portion is used in general foodstuffs as a sweetener. The yearly production of high-fructose syrup in the world is estimated about 8,000,000 kg.
Both glucose and fructose are hexoses similar in structure. Chemical and enzymatic processes have hith-erto been proposed for isomerization of glucose into fructose, and it is currently conducted in industry to isomerize glucose into fructose using an isomerization enzyme, namely, glucose isomerase to produce a high-fructose syrup.
That is, starch, for example, corn starch is liquefied; the resulting liquid is subjected to sacchar-ification using glucoamylase to obtain a starch syrup;
and passing the starch syrup continuously through an im-mobilized enzyme obtained by immobilizing, using one of CAZi various methods, a glucose isomerase produced by, a mi-croorganism of, for example, Streptomyces genus, to iso-merize the glucose contained in said solution into fruc-tose.
The above isomerization reaction is an equilib-rium reaction whose equilibrium point is 1 or there-abouts. At the equilibrium point, about 50% of glucose can be isomerized into fructose at a reaction tempera-ture of about 60°C. In order to allow the isomerization to proceed to such a level, however, a considerable length of time is required, the reaction mixture is col-ored owing to the heating for such a long time, and a high cost is incurred for the purification and condensa-tion steps required for product marketing. Hence, the reaction is terminated when the isomerization has pro-ceeded to a fructose content of about 42%.
As described above, the high-fructose syrup is produced in order to allow glucose of mass production and low cost to have sweetness similar to that of su-crose. However, when the sweetness of sucrose is arbi-trarily taken as 100, the above-mentioned high-fructose syrup containing about 42% of fructose (this fructose syrup is hereinafter referred to as 42%-fructose syrup, in some cases) has a sweetness of 95-100 which is slightly insufficient. Therefore, in the above isomer-~ ization reaction alone, it is impossible to directly ob-tain a high-fructose syrup having the same sweetness as sucrose.
CA2ii7472 Hence, there is currently produced in industry a 55%-fructose syrup having a sweetness of 100-110 by in-creasing the fructose content in the 42%-fructose syrup to 55%.
In order to produce a 55%-fructose syrup from the 42%-fructose syrup, however, a large apparatus such as a reactor packed with a cation exchange resin is re-quired; moreover, a complicated operation must be con-ducted, that is, continuous sugar separation is con-ducted using said reactor to obtain a fructose syrup containing about 95% of fructose and then this fructose is mixed with the 42%-fructose syrup.
Meanwhile, as the isomerization of other com-pound having an aldose structure into a compound having a ketose structure, there can be mentioned, for example, isomerization of lactose (a dissacharide) into lactu-lose. In this isomerization, however, unlike the above isomerization of glucose into fructose, no enzyme effec-tive for isomerization of lactose into lactulose has not yet been found; therefore, the isomerization is cur-rently conducted by adding, to lactose, sodium hydroxide of a concentration not exceeding a given level and then heating the mixture at 70°C or higher to isomerize lac-tose into lactulose (Japanese Patent Publication No.
2984/1977). This process, however, gives a low isomer-ization ratio, i.e. a low lactulose yield of 20% or less (this is lower than the fructose yield). In order to WO 94!14826 PCT/JP93/01896 CA2ii7472 obtain a high-lactulose syrup, the process has a problem that the lactulose syrup obtained must be condensed.
An object of the present invention is to provide a process which is free from the above-mentioned prob-lems of prior art and which can isomerize a compound having an aldose structure into a compound having a ke-tose structure at a high isomerization ratio.
Another object of the present invention is to provide a process which can isomerize a compound having an aldose structure into a compound having a ketose structure without requiring any special apparatus or any complicated operation.
Still another object of the present invention is to provide a process which can isomerize a compound hav-ing an aldose structure into a compound having a ketose structure, using an isomerization enzyme or without us-ing any isomerization enzyme.
Still another object of the present invention is to provide a process which can isomerize a compound hav-ing an aldose structure into a compound having a ketose structure without employing the condition of heating in alkalinity (this condition is sometimes disadvantageous for isomerization ratio) even when there has been found no enzyme effective for said isomerization.
Still another object of the present invention is to provide an isomerization agent or accelerator effec-tive in the above process.
WO 94!14826 PCT/JP93/01896 CA2ii7472 Disclosure of the Invention According to the present invention there is pro-vided a process which comprises isomerizing a compound having an aldose structure into a compound having a ke-tose structure, by the use of or in the presence of an organogermanium compound having a structural portion represented by the following formula (I).
O1/z-Ge- ( I ) O1/z According to the present invention there is fur-ther provided an isomerization agent or accelerator ef-fective for the isomerization of a compound having an aldose structure into a compound having a ketose struc-ture, which agent or accelerator comprises, as an active component, an organogermanium compound having a struc-tural portion represented by the following formula (I).
O1/z-Ge- ( I ) O1/z Brief Description of the Drawing CA2ii7472 Fig. 1 is a graph showing a relation between re-action time and isomerization ratio.
A case where an organogermanium compound (23) was used as the present isomerization agent.
A case where an organogermanium compound (18) was used as the present isomerization agent.
A case where an organogermanium compound (1) was used as the present isomerization agent.
A blank Best Mode for Carrying Out the Invention The present invention is hereinafter described in detail.
In the present invention, the isomerization of a compound having an aldose structure into a compound hav-ing a ketose structure is conducted by the use of or in the presence of an organogermanium compound having a structural portion represented by the above-mentioned formula (I) with the remaining structure being a chain or cyclic hydrocarbon, a substitution product or deriva-tive thereof, or other organic group. Hence, descrip-tion is made first on the organogermanium compound hav-ing such a structure.
The organogermanium compound can be exemplified by a compound represented by formula (II) CA2ii7472 Oi/z R1 R3 O~/2-Ge- ( C ) n-CH-COX1 ( Ol/z R2 [Rl, R2 and R3, which may be the same or different, in-dependently represent a hydrogen atom, a lower alkyl group, a substituted or unsubstituted phenyl group, a carboxyl group, a carboxyalkyl group or an amino group which is unsubstituted or substituted with appropriate group(s); X1 represents a hydroxyl group, an O-lower alkyl group, an amino group or a salt represented by OY1 (Y1 represents a metal or a basic group-containing com-pound); and n represents an integer of 1 or more), which contains, as a basic skeleton, a germylcarboxylic acid derivative formed by bonding between a germanium atom and a carboxylic acid derivative having three sub-stituents R1, RZ and R3 and an oxygen-containing func-tional group OX1, with the germanium atom in the basic skeleton bonding to oxygen atoms at an atomic ratio of 2 (germanium) : 3 (oxygen).
The substituents R1, RZ and R3, which may be the same or different, independently represent a hydrogen atom; a lower alkyl group such as methyl, ethyl, propyl, butyl or the like; a substituted or unsubstituted phenyl group; a carboxyl group; a carboxyalkyl group; or an amino group which is unprotected or protected with a protective group such as acetyl or the like. The sub-WO 94!14826 PCT/JP93/01896 CA2ii7472 stituent X1 represents a hydroxyl group, an O-lower alkyl group, an amino group or a salt represented by OY1 (Y1 represents a metal such as sodium, potassium or the like (the metal need not be monovalent), or a basic com-pound typified by lysozyme or a basic amino acid such as lysine].
The substituents R1 and R2 bond to each carbon of the carbon chain represented by (C)n (n is an integer of 1 or more) present at the a-position of the germanium atom. Accordingly, when n is 1, 2, ...n, R1 becomes R11. R12. -~~Rln. and R2n becomes R21, R22. ...R2n. The substituent R3 bonds to the methylene group present be-tween said carbon chain and the oxygen-containing func-tional group.
The organogermanium compound used in the present invention can therefore be exemplified by those shown in the following Tables 1-5.
CA2ii7472 Table 1 Compound I
(C) n R3 X 1 No. I
CH
CH
I
C H OH
I
CH
CH
CH
CH2 H ONa CA2ii7472 Table 2 RI
Compound I
(C) n R3 X I
No. I
CH
CH
I
I
CH
CH
CA2ii7472 Table 3 Compound (C) n R3 X1 No. I
CH
I
I
CH
I
I
CH
CH
26 CH2 NH2 ONa CA2ii7472 Table 4 Compound I
(C) n R3 X1 No. I
2$ I NHCOCH3 OH
CH
I
I
CH
I
I
CH
CH
35 ~ CH2 NHCOCH3 ONa CA2ii7472 Table 5 R, Compound I
( C ) n R 3 X , No. I
Rz CBHS
CHCHZ
43 CHZCHz NHCOCH3 OH
CHZCHCHz CBHS
CHCHZCHZ
49 CHZ (CH2) ZCHZ H OH
CH (CHZ) ZCH2 1 CHZ (C H2) 3CH2 H OH
CA2ii7472 Of the compounds shown in Tables 1-5, those shown in Tables 1-4 represented by the following formula (III) are preferable from the availability standpoint:
Oi~a-Ge-C-CH-COR2 ( III ) O1/zR5 wherein R4, R5 and R6, which may be the same or differ-ent, independently represent, similarly to R1, R2 and R3, a hydrogen atom, a lower alkyl group, a substituted or unsubstituted phenyl group, a carboxyl group, a car-boxyalkyl group or an amino group which is unsubstituted or substituted with appropriate group(s); and X2 repre-sents, similarly to X1, a hydroxyl group, an O-lower alkyl group, an amino group or a salt represented by OY2 (Y2 represents a metal or a basic group-containing com-pound).
The organogermanium compound having the above structure can be produced by various methods (for exam-ple, Japanese Patent Publication No. 40159/1984, Japanese Patent Kokai (Laid-open) No. 86890/1991 and Japanese Patent Kokai (Laid-open) No. 62885/1990).
Description is made on the production of organogermanium compounds represented by formula (III).
An organogermanium compound of formula (III) wherein X2 is a hydroxyl group, can be produced by, for CA2ii7472 example, hydrolyzing a trihalogermylpropionic acid (e. g., trichlorogermylpropionic acid) having sub-stituents R4 to R6, as shown in the following formula.
cisGe-c-cH-coox ~ (zl=) I
RS
An organogermanium compound of formula (III) wherein XZ is an O-lower alkyl group, can be produced by, for example, reacting the above trichlorogermylpro-pionic acid with thionyl chloride or the like to convert said acid into a corresponding acid halide, reacting said halide with an alcohol corresponding to said lower alkyl group, and hydrolyzing the reaction product. An organogermanium compound of formula (III) wherein X2 is an amino group, can be produced by, for example, react-ing said acid halide with ammonia and then hydrolyzing the reaction product.
An organogermanium compound of formula (iii) wherein XZ is a salt represented by OYZ and YZ is a metal, can be produced by reacting a compound of formula (III) wherein XZ is a hydroxyl group, with a hydroxide of Y2. An organogermanium compound of formula (III) wherein XZ is a salt represented by OYZ and YZ is a ba-sic group-containing compound, can be synthesized by a known acid-base reaction.
CA2ii7472 Organogermanium compounds of formula (III) wherein n is larger than 1, can be produced basically in accordance with the above-mentioned methods.
That the thus produced organogermanium compound is represented by the above-shown general formula (II) can be well supported by the results of instrumental analyses (e. g., NMR absorption spectrum, IR absorption spectrum) obtained for said compound.
The formulas (II) and (III) representing the organogermanium compound of the present invention, each represents said compound in its crystal state. It is known that the present compound, for example compound (II), takes a structure represented by the following formula (II'), in water.
OH-Ge- (C) n-CH-COX1 The organogermanium compounds (II) and (IZI) can be represented also by other structural formulas. For example, the compound (II) is the same as a compound represented by the following structural formula (II" ).
Ge-(C)n-CH-COX1 CA2ii7472 In the present invention, the organogermanium compound which is represented by at least one of above formulas cari be used, regardless of their crystal struc-tures.
The organogermanium compound used in the present invention has very low toxicity. For example, a com-pound (II) wherein n=1, R1=RZ=R3=A and X1=OH [compound No. 1, this compound is hereinafter referred to as organogermanium compound (1) in some cases], shows a LDSp of 6 g/kg or more when orally administered to mice and 10 g/kg or more when orally administered to rats.
In the present invention, as described previ-ously, a compound having an aldose structure is isomer-ized into a compound having a ketose structure by the use of or in the presence of an organogermanium compound having a structural portion represented by the above formula (I). The compound to be isomerized may be any compound which has, in the molecule, the following al-dose structure represented by Fischer's projection for-mula O
I I
C-H
I
(OH)H-C-OH(H) I
(OH)H-C-OH(H) la CA2ii7472 and which can be isomerized into a compound having the following ketose structure represented by Fischer's pro-jection formula I
C=O
I
(OH)H-C-OH(H) via an interim stage of formation of a cis-ene-diol structure as shown below.
O
II H \C/OH CHz_pH
I H ~ ~C~ ~ C=O
I
As the compound having the above aldose struc-ture, monosaccharides and their derivatives such as shown below at the left side can be mentioned. They are isomerized into compounds shown below at the right side glyceraldehyde ~ dihydroxyacetone erythrose, threose -~ erythrulose ribose, arabinose -~ ribulose xylose, lyxose ~ xylulose allose, altrose -~ psicose glucose, mannose ~ fructose ~~~i7472 gulose, idose -> sorbose galactose, talose -~ tagatose As the compound having the aldose structure, re-ducing disaccharides and their derivatives such as shown below at the left side can also be mentioned. They are isomerized into compounds shown below at the right side.
maltose -~ maltulose lactose --> lactulose Trisaccharides and higher, and also polysaccha-rides and their derivatives can be isomerized. In that case, they must have an aldose structure at the molecu-lar end. Incidentally, for some (e. g. maltose and lac-tose) of the above compounds which can be isomerized, there has been found no enzyme capable of isomerizing them into corresponding compounds each having a ketose structure.
Of the compounds of ketose structure, lactulose is clinically used for the improvement of psychoneurosis associated with hyperammonemia, tremors of hands and fingers, etc.
In the isomerization of a compound having an al-dose structure according to the present invention, an isomerization enzyme may or may not be used. when no isomerization enzyme ,is used, the isomerization may be conducted under the same conditions as employed in the conventional isomerization of glucose into fructose us-ing an isomerization enzyme, for example, at room tem-perature to 60-90°C in the presence of an alkali such as CA2ii7472 sodium hydroxide, calcium hydroxide or the like. In the isomerization using no enzyme, it is also possible to use the alkaline portion of the electrolytic water ob-tained by the polarization of water using a particular apparatus therefor.
The concentration of the organogermanium com-pound used in the isomerization are not particularly re-stricted because it is determined depending upon isomer-ization time, desired isomerization ratio, etc.
However, as an example, 1~ by weight or more of the organogermanium compound is added to a 10~ by weight to solution of the compound having an aldose structure.
In the isomerization of the present process, the isomerization ratio increases generally with an increase in the reaction time. Therefore, the isomerization ra-tio is controlled by controlling the reaction time, whereby a desired isomerization ratio is obtained.
In the isomerization process according to the present invention, an isomerization enzyme may be used as in the conventional isomerization of glucose into fructose using an isomerization enzyme.
Description is made on a case of isomerization of glucose into fructose using an isomerization enzyme.
First, starch (e.g. corn starch) is liquefied using a-amylase produced by, for example, Bacillus genus; the resulting liquid is subjected to saccharification using glucoamylase produced by, for example, Aspergillus niger, to obtain a starch syrup. Incidentally, this CA~ii7-472 starch syrup contains about 93-95% of glucose. In the saccharification, there may be used, in combination, pullulanase which is an enzyme for cleavage of a-1,6-glycoside linkage of starch; in this case, the glucose content in the resulting starch syrup is about 96%.
The starch syrup is purified and condensed as necessary; then, there is added, as necessary, a metal ion of magnesium, manganese or cobalt required by glu-cose isomerase used in the subsequent isomerization step. From the standpoint of food safety, magnesium ion is preferred as the metal ion.
The resulting starch syrup is subjected to an isomerization step. Glucose isomerase used in this step maybe any as long as it can isomerize glucose into fruc-tose. Examples of glucose isomerase are those enzymes produced by microorganisms belonging to Streptomyces genus, Bacillus genus, Arthrobacter genus, Microbacterium genus, etc. Specific examples of the en-zyme are as follows.
Lactobacillus brevis Bacillus coagulans Brevibacterium pentosoaminoacidium Arthrobactor sp.
Actinoplanes missouriensis Streptomyces phaeochromogenus Streptomyces rubiginosus Streptomyces albus NRRL-5778 Streptomyces griseofuscus CA2ii7472 The above-mentioned glucose isomerase is allowed to act on the above-mentioned starch syrup in the pres-ence of the above-mentioned organogermanium compound to isomerize glucose in the syrup into fructose. This step may be conducted in a mixture of the starch syrup, the organogermanium compound and the glucose isomerase; how-ever, it is also possible that the glucose isomerase be immobilized according to one of conventional methods to prepare an immobilized enzyme and the starch syrup con-taining the organogermanium compound be continuously passed through the immobilized enzyme. Incidentally, in the present invention, a microbial cell preparation whose proteins other than glucose isomerase have been inactivated, may be used in place of the isomerization enzyme.
The conditions employed for the isomerization of glucose into fructose according to the present inven-tion, can be the same as used in the conventional known isomerization processes. That is, the isomerization may be conducted, for example, in neutrality to weak alka-linity at 60-90°C.
In the isomerization of glucose into fructose according to the present invention, the isomerization ratio increases with the lapse of the reaction time, as shown in Examples given later. Therefore, it is possi-ble to control the reaction time to control the isomer-ization ratio and thereby obtain a desired isomerization CA2'~ ~ 772 ratio, for example, a ratio of isomerization to fructose of about 55~ or more.
In the present invention, the amount of the organogermanium compound used can be determined depend-ing upon the intended isomerization ratio, etc. The organogermanium compound can be used in a concentration range of, for example, 1/100 M or more.
The present invention is hereinafter described in more detail with reference to Examples.
Example 1 (1) Synthesis of organogermanium compounds Trichlorogermane (Cl3GeH) was added to acrylic acid (CH2CHCOOH) to obtain trichlorogermylpropionic acid (Cl3GeCH2CH2COOH). It was hydrolyzed to synthesize an organogermanium compound (1). In the same manner were synthesized organogermanium compounds (2) to (51).
(2) Preparation of substrate solutions A solution containing 40~ glucose and 1.2 M
organogermanium compound was prepared according to the following procedure. 0.8 g of anhydrous glucose was dissolved in 0.8 ml of deionized water. To the solution was added, in small portions, 0.407 g of the organoger-uranium compound (1) as an isomerization accelerator of the present invention [a compound represented by formula (II) wherein n=1, R1=R2=R3 and X1=OH] while the pH of the solution was maintained at very weak alkalinity, to completely dissolve the compound in the solution.
CA2ii7472 Thereto was added 4.9 mg of magnesium sulfate, and the pH of the resulting mixture was adjusted to 8Ø Then, deionized water was added to make the total volume 2.0 ml, whereby a substrate solution was prepared.
Two other substrate solutions containing the organogermanium compounds (18) [a compound represented by formula (II) wherein n=1, R1=R2=H, R3=NH2 and X1=OH]
and (23) [a compound represented by formula (II) wherein n=1, R1=H, R2=C6H5, R3=NH2 and X1=OH], respectively, were prepared in the same manner as above except that the organogermanium compounds (18) and (23) were used in amounts of 0.443 g and 0.638 g, respectively (these amounts corresponded to 1.2 M of germanium).
(3) Preparation of enzyme An isomerization enzyme (glucose isomerase) ex-tracted from the cells of Streptomyces griseofuscus S-41 was purified according to a known method using an ion exchange column, a gel filtration column or the like, until a single band was obtained electrophoretically.
The resulting purified enzyme was used as a standard en-zyme.
(4) Enzymatic isomerization reaction In a small test tube were placed 0.7 ml of the above substrate solution, 0.1 ml of a 200 mM MOPS buffer solution (pH 8.0) and 0.2 ml of a solution containing the above-prepared standard enzyme (5.69 mg/ml). The test tube was placed in a water bath of 60°C and the mixture in the test tube was subjected to a reaction.
CA2ii7472 Each 50 ul of the reaction mixture was taken and added, at regular intervals, to 50 pl of 0.5 N perchloric acid placed in a microvial, to terminate the reaction. The amount of formed fructose in the microvial was deter-mined by high-performance liquid chromatography using a column [LC7A, SCR-101 (N) manufactured by Shimadzu Corp.] to examine the change with time, of ratio of iso-merization of glucose into fructose.
In order to produce a 55%-fructose syrup from the 42%-fructose syrup, however, a large apparatus such as a reactor packed with a cation exchange resin is re-quired; moreover, a complicated operation must be con-ducted, that is, continuous sugar separation is con-ducted using said reactor to obtain a fructose syrup containing about 95% of fructose and then this fructose is mixed with the 42%-fructose syrup.
Meanwhile, as the isomerization of other com-pound having an aldose structure into a compound having a ketose structure, there can be mentioned, for example, isomerization of lactose (a dissacharide) into lactu-lose. In this isomerization, however, unlike the above isomerization of glucose into fructose, no enzyme effec-tive for isomerization of lactose into lactulose has not yet been found; therefore, the isomerization is cur-rently conducted by adding, to lactose, sodium hydroxide of a concentration not exceeding a given level and then heating the mixture at 70°C or higher to isomerize lac-tose into lactulose (Japanese Patent Publication No.
2984/1977). This process, however, gives a low isomer-ization ratio, i.e. a low lactulose yield of 20% or less (this is lower than the fructose yield). In order to WO 94!14826 PCT/JP93/01896 CA2ii7472 obtain a high-lactulose syrup, the process has a problem that the lactulose syrup obtained must be condensed.
An object of the present invention is to provide a process which is free from the above-mentioned prob-lems of prior art and which can isomerize a compound having an aldose structure into a compound having a ke-tose structure at a high isomerization ratio.
Another object of the present invention is to provide a process which can isomerize a compound having an aldose structure into a compound having a ketose structure without requiring any special apparatus or any complicated operation.
Still another object of the present invention is to provide a process which can isomerize a compound hav-ing an aldose structure into a compound having a ketose structure, using an isomerization enzyme or without us-ing any isomerization enzyme.
Still another object of the present invention is to provide a process which can isomerize a compound hav-ing an aldose structure into a compound having a ketose structure without employing the condition of heating in alkalinity (this condition is sometimes disadvantageous for isomerization ratio) even when there has been found no enzyme effective for said isomerization.
Still another object of the present invention is to provide an isomerization agent or accelerator effec-tive in the above process.
WO 94!14826 PCT/JP93/01896 CA2ii7472 Disclosure of the Invention According to the present invention there is pro-vided a process which comprises isomerizing a compound having an aldose structure into a compound having a ke-tose structure, by the use of or in the presence of an organogermanium compound having a structural portion represented by the following formula (I).
O1/z-Ge- ( I ) O1/z According to the present invention there is fur-ther provided an isomerization agent or accelerator ef-fective for the isomerization of a compound having an aldose structure into a compound having a ketose struc-ture, which agent or accelerator comprises, as an active component, an organogermanium compound having a struc-tural portion represented by the following formula (I).
O1/z-Ge- ( I ) O1/z Brief Description of the Drawing CA2ii7472 Fig. 1 is a graph showing a relation between re-action time and isomerization ratio.
A case where an organogermanium compound (23) was used as the present isomerization agent.
A case where an organogermanium compound (18) was used as the present isomerization agent.
A case where an organogermanium compound (1) was used as the present isomerization agent.
A blank Best Mode for Carrying Out the Invention The present invention is hereinafter described in detail.
In the present invention, the isomerization of a compound having an aldose structure into a compound hav-ing a ketose structure is conducted by the use of or in the presence of an organogermanium compound having a structural portion represented by the above-mentioned formula (I) with the remaining structure being a chain or cyclic hydrocarbon, a substitution product or deriva-tive thereof, or other organic group. Hence, descrip-tion is made first on the organogermanium compound hav-ing such a structure.
The organogermanium compound can be exemplified by a compound represented by formula (II) CA2ii7472 Oi/z R1 R3 O~/2-Ge- ( C ) n-CH-COX1 ( Ol/z R2 [Rl, R2 and R3, which may be the same or different, in-dependently represent a hydrogen atom, a lower alkyl group, a substituted or unsubstituted phenyl group, a carboxyl group, a carboxyalkyl group or an amino group which is unsubstituted or substituted with appropriate group(s); X1 represents a hydroxyl group, an O-lower alkyl group, an amino group or a salt represented by OY1 (Y1 represents a metal or a basic group-containing com-pound); and n represents an integer of 1 or more), which contains, as a basic skeleton, a germylcarboxylic acid derivative formed by bonding between a germanium atom and a carboxylic acid derivative having three sub-stituents R1, RZ and R3 and an oxygen-containing func-tional group OX1, with the germanium atom in the basic skeleton bonding to oxygen atoms at an atomic ratio of 2 (germanium) : 3 (oxygen).
The substituents R1, RZ and R3, which may be the same or different, independently represent a hydrogen atom; a lower alkyl group such as methyl, ethyl, propyl, butyl or the like; a substituted or unsubstituted phenyl group; a carboxyl group; a carboxyalkyl group; or an amino group which is unprotected or protected with a protective group such as acetyl or the like. The sub-WO 94!14826 PCT/JP93/01896 CA2ii7472 stituent X1 represents a hydroxyl group, an O-lower alkyl group, an amino group or a salt represented by OY1 (Y1 represents a metal such as sodium, potassium or the like (the metal need not be monovalent), or a basic com-pound typified by lysozyme or a basic amino acid such as lysine].
The substituents R1 and R2 bond to each carbon of the carbon chain represented by (C)n (n is an integer of 1 or more) present at the a-position of the germanium atom. Accordingly, when n is 1, 2, ...n, R1 becomes R11. R12. -~~Rln. and R2n becomes R21, R22. ...R2n. The substituent R3 bonds to the methylene group present be-tween said carbon chain and the oxygen-containing func-tional group.
The organogermanium compound used in the present invention can therefore be exemplified by those shown in the following Tables 1-5.
CA2ii7472 Table 1 Compound I
(C) n R3 X 1 No. I
CH
CH
I
C H OH
I
CH
CH
CH
CH2 H ONa CA2ii7472 Table 2 RI
Compound I
(C) n R3 X I
No. I
CH
CH
I
I
CH
CH
CA2ii7472 Table 3 Compound (C) n R3 X1 No. I
CH
I
I
CH
I
I
CH
CH
26 CH2 NH2 ONa CA2ii7472 Table 4 Compound I
(C) n R3 X1 No. I
2$ I NHCOCH3 OH
CH
I
I
CH
I
I
CH
CH
35 ~ CH2 NHCOCH3 ONa CA2ii7472 Table 5 R, Compound I
( C ) n R 3 X , No. I
Rz CBHS
CHCHZ
43 CHZCHz NHCOCH3 OH
CHZCHCHz CBHS
CHCHZCHZ
49 CHZ (CH2) ZCHZ H OH
CH (CHZ) ZCH2 1 CHZ (C H2) 3CH2 H OH
CA2ii7472 Of the compounds shown in Tables 1-5, those shown in Tables 1-4 represented by the following formula (III) are preferable from the availability standpoint:
Oi~a-Ge-C-CH-COR2 ( III ) O1/zR5 wherein R4, R5 and R6, which may be the same or differ-ent, independently represent, similarly to R1, R2 and R3, a hydrogen atom, a lower alkyl group, a substituted or unsubstituted phenyl group, a carboxyl group, a car-boxyalkyl group or an amino group which is unsubstituted or substituted with appropriate group(s); and X2 repre-sents, similarly to X1, a hydroxyl group, an O-lower alkyl group, an amino group or a salt represented by OY2 (Y2 represents a metal or a basic group-containing com-pound).
The organogermanium compound having the above structure can be produced by various methods (for exam-ple, Japanese Patent Publication No. 40159/1984, Japanese Patent Kokai (Laid-open) No. 86890/1991 and Japanese Patent Kokai (Laid-open) No. 62885/1990).
Description is made on the production of organogermanium compounds represented by formula (III).
An organogermanium compound of formula (III) wherein X2 is a hydroxyl group, can be produced by, for CA2ii7472 example, hydrolyzing a trihalogermylpropionic acid (e. g., trichlorogermylpropionic acid) having sub-stituents R4 to R6, as shown in the following formula.
cisGe-c-cH-coox ~ (zl=) I
RS
An organogermanium compound of formula (III) wherein XZ is an O-lower alkyl group, can be produced by, for example, reacting the above trichlorogermylpro-pionic acid with thionyl chloride or the like to convert said acid into a corresponding acid halide, reacting said halide with an alcohol corresponding to said lower alkyl group, and hydrolyzing the reaction product. An organogermanium compound of formula (III) wherein X2 is an amino group, can be produced by, for example, react-ing said acid halide with ammonia and then hydrolyzing the reaction product.
An organogermanium compound of formula (iii) wherein XZ is a salt represented by OYZ and YZ is a metal, can be produced by reacting a compound of formula (III) wherein XZ is a hydroxyl group, with a hydroxide of Y2. An organogermanium compound of formula (III) wherein XZ is a salt represented by OYZ and YZ is a ba-sic group-containing compound, can be synthesized by a known acid-base reaction.
CA2ii7472 Organogermanium compounds of formula (III) wherein n is larger than 1, can be produced basically in accordance with the above-mentioned methods.
That the thus produced organogermanium compound is represented by the above-shown general formula (II) can be well supported by the results of instrumental analyses (e. g., NMR absorption spectrum, IR absorption spectrum) obtained for said compound.
The formulas (II) and (III) representing the organogermanium compound of the present invention, each represents said compound in its crystal state. It is known that the present compound, for example compound (II), takes a structure represented by the following formula (II'), in water.
OH-Ge- (C) n-CH-COX1 The organogermanium compounds (II) and (IZI) can be represented also by other structural formulas. For example, the compound (II) is the same as a compound represented by the following structural formula (II" ).
Ge-(C)n-CH-COX1 CA2ii7472 In the present invention, the organogermanium compound which is represented by at least one of above formulas cari be used, regardless of their crystal struc-tures.
The organogermanium compound used in the present invention has very low toxicity. For example, a com-pound (II) wherein n=1, R1=RZ=R3=A and X1=OH [compound No. 1, this compound is hereinafter referred to as organogermanium compound (1) in some cases], shows a LDSp of 6 g/kg or more when orally administered to mice and 10 g/kg or more when orally administered to rats.
In the present invention, as described previ-ously, a compound having an aldose structure is isomer-ized into a compound having a ketose structure by the use of or in the presence of an organogermanium compound having a structural portion represented by the above formula (I). The compound to be isomerized may be any compound which has, in the molecule, the following al-dose structure represented by Fischer's projection for-mula O
I I
C-H
I
(OH)H-C-OH(H) I
(OH)H-C-OH(H) la CA2ii7472 and which can be isomerized into a compound having the following ketose structure represented by Fischer's pro-jection formula I
C=O
I
(OH)H-C-OH(H) via an interim stage of formation of a cis-ene-diol structure as shown below.
O
II H \C/OH CHz_pH
I H ~ ~C~ ~ C=O
I
As the compound having the above aldose struc-ture, monosaccharides and their derivatives such as shown below at the left side can be mentioned. They are isomerized into compounds shown below at the right side glyceraldehyde ~ dihydroxyacetone erythrose, threose -~ erythrulose ribose, arabinose -~ ribulose xylose, lyxose ~ xylulose allose, altrose -~ psicose glucose, mannose ~ fructose ~~~i7472 gulose, idose -> sorbose galactose, talose -~ tagatose As the compound having the aldose structure, re-ducing disaccharides and their derivatives such as shown below at the left side can also be mentioned. They are isomerized into compounds shown below at the right side.
maltose -~ maltulose lactose --> lactulose Trisaccharides and higher, and also polysaccha-rides and their derivatives can be isomerized. In that case, they must have an aldose structure at the molecu-lar end. Incidentally, for some (e. g. maltose and lac-tose) of the above compounds which can be isomerized, there has been found no enzyme capable of isomerizing them into corresponding compounds each having a ketose structure.
Of the compounds of ketose structure, lactulose is clinically used for the improvement of psychoneurosis associated with hyperammonemia, tremors of hands and fingers, etc.
In the isomerization of a compound having an al-dose structure according to the present invention, an isomerization enzyme may or may not be used. when no isomerization enzyme ,is used, the isomerization may be conducted under the same conditions as employed in the conventional isomerization of glucose into fructose us-ing an isomerization enzyme, for example, at room tem-perature to 60-90°C in the presence of an alkali such as CA2ii7472 sodium hydroxide, calcium hydroxide or the like. In the isomerization using no enzyme, it is also possible to use the alkaline portion of the electrolytic water ob-tained by the polarization of water using a particular apparatus therefor.
The concentration of the organogermanium com-pound used in the isomerization are not particularly re-stricted because it is determined depending upon isomer-ization time, desired isomerization ratio, etc.
However, as an example, 1~ by weight or more of the organogermanium compound is added to a 10~ by weight to solution of the compound having an aldose structure.
In the isomerization of the present process, the isomerization ratio increases generally with an increase in the reaction time. Therefore, the isomerization ra-tio is controlled by controlling the reaction time, whereby a desired isomerization ratio is obtained.
In the isomerization process according to the present invention, an isomerization enzyme may be used as in the conventional isomerization of glucose into fructose using an isomerization enzyme.
Description is made on a case of isomerization of glucose into fructose using an isomerization enzyme.
First, starch (e.g. corn starch) is liquefied using a-amylase produced by, for example, Bacillus genus; the resulting liquid is subjected to saccharification using glucoamylase produced by, for example, Aspergillus niger, to obtain a starch syrup. Incidentally, this CA~ii7-472 starch syrup contains about 93-95% of glucose. In the saccharification, there may be used, in combination, pullulanase which is an enzyme for cleavage of a-1,6-glycoside linkage of starch; in this case, the glucose content in the resulting starch syrup is about 96%.
The starch syrup is purified and condensed as necessary; then, there is added, as necessary, a metal ion of magnesium, manganese or cobalt required by glu-cose isomerase used in the subsequent isomerization step. From the standpoint of food safety, magnesium ion is preferred as the metal ion.
The resulting starch syrup is subjected to an isomerization step. Glucose isomerase used in this step maybe any as long as it can isomerize glucose into fruc-tose. Examples of glucose isomerase are those enzymes produced by microorganisms belonging to Streptomyces genus, Bacillus genus, Arthrobacter genus, Microbacterium genus, etc. Specific examples of the en-zyme are as follows.
Lactobacillus brevis Bacillus coagulans Brevibacterium pentosoaminoacidium Arthrobactor sp.
Actinoplanes missouriensis Streptomyces phaeochromogenus Streptomyces rubiginosus Streptomyces albus NRRL-5778 Streptomyces griseofuscus CA2ii7472 The above-mentioned glucose isomerase is allowed to act on the above-mentioned starch syrup in the pres-ence of the above-mentioned organogermanium compound to isomerize glucose in the syrup into fructose. This step may be conducted in a mixture of the starch syrup, the organogermanium compound and the glucose isomerase; how-ever, it is also possible that the glucose isomerase be immobilized according to one of conventional methods to prepare an immobilized enzyme and the starch syrup con-taining the organogermanium compound be continuously passed through the immobilized enzyme. Incidentally, in the present invention, a microbial cell preparation whose proteins other than glucose isomerase have been inactivated, may be used in place of the isomerization enzyme.
The conditions employed for the isomerization of glucose into fructose according to the present inven-tion, can be the same as used in the conventional known isomerization processes. That is, the isomerization may be conducted, for example, in neutrality to weak alka-linity at 60-90°C.
In the isomerization of glucose into fructose according to the present invention, the isomerization ratio increases with the lapse of the reaction time, as shown in Examples given later. Therefore, it is possi-ble to control the reaction time to control the isomer-ization ratio and thereby obtain a desired isomerization CA2'~ ~ 772 ratio, for example, a ratio of isomerization to fructose of about 55~ or more.
In the present invention, the amount of the organogermanium compound used can be determined depend-ing upon the intended isomerization ratio, etc. The organogermanium compound can be used in a concentration range of, for example, 1/100 M or more.
The present invention is hereinafter described in more detail with reference to Examples.
Example 1 (1) Synthesis of organogermanium compounds Trichlorogermane (Cl3GeH) was added to acrylic acid (CH2CHCOOH) to obtain trichlorogermylpropionic acid (Cl3GeCH2CH2COOH). It was hydrolyzed to synthesize an organogermanium compound (1). In the same manner were synthesized organogermanium compounds (2) to (51).
(2) Preparation of substrate solutions A solution containing 40~ glucose and 1.2 M
organogermanium compound was prepared according to the following procedure. 0.8 g of anhydrous glucose was dissolved in 0.8 ml of deionized water. To the solution was added, in small portions, 0.407 g of the organoger-uranium compound (1) as an isomerization accelerator of the present invention [a compound represented by formula (II) wherein n=1, R1=R2=R3 and X1=OH] while the pH of the solution was maintained at very weak alkalinity, to completely dissolve the compound in the solution.
CA2ii7472 Thereto was added 4.9 mg of magnesium sulfate, and the pH of the resulting mixture was adjusted to 8Ø Then, deionized water was added to make the total volume 2.0 ml, whereby a substrate solution was prepared.
Two other substrate solutions containing the organogermanium compounds (18) [a compound represented by formula (II) wherein n=1, R1=R2=H, R3=NH2 and X1=OH]
and (23) [a compound represented by formula (II) wherein n=1, R1=H, R2=C6H5, R3=NH2 and X1=OH], respectively, were prepared in the same manner as above except that the organogermanium compounds (18) and (23) were used in amounts of 0.443 g and 0.638 g, respectively (these amounts corresponded to 1.2 M of germanium).
(3) Preparation of enzyme An isomerization enzyme (glucose isomerase) ex-tracted from the cells of Streptomyces griseofuscus S-41 was purified according to a known method using an ion exchange column, a gel filtration column or the like, until a single band was obtained electrophoretically.
The resulting purified enzyme was used as a standard en-zyme.
(4) Enzymatic isomerization reaction In a small test tube were placed 0.7 ml of the above substrate solution, 0.1 ml of a 200 mM MOPS buffer solution (pH 8.0) and 0.2 ml of a solution containing the above-prepared standard enzyme (5.69 mg/ml). The test tube was placed in a water bath of 60°C and the mixture in the test tube was subjected to a reaction.
CA2ii7472 Each 50 ul of the reaction mixture was taken and added, at regular intervals, to 50 pl of 0.5 N perchloric acid placed in a microvial, to terminate the reaction. The amount of formed fructose in the microvial was deter-mined by high-performance liquid chromatography using a column [LC7A, SCR-101 (N) manufactured by Shimadzu Corp.] to examine the change with time, of ratio of iso-merization of glucose into fructose.
(5) Results As shown in Fig. 1, in the blank using no organogermanium compound, the reaction reached an equi-librium in about 6 hours and the isomerization ratio was as low as 50~. When the organogermanium compound of the present invention was added as an isomerization acceler-ator, both the initial reaction rate and the isomeriza-tion ratio in equilibrium were superior to those of the blank. That is, the initial reaction rate was 40-50~
higher than that of the blank, in all cases and there was substantially no difference in initial reaction rate between different organogermanium compounds. Meanwhile, the isomerization ratio in equilibrium varied depending upon the kinds of organogermanium compounds used; and the compound (23) gave an isomerization ratio of 99~, the compound (18) gave an isomerization ratio of 80$, and the compound (1) gave an isomerization ratio of 75~.
Example 2 (1) Preparation of weakly alkaline electrolytic water by electrolysis Water was passed through an apparatus for elec-trolysis [e.g. Microcluster* manufactured by Asahi Glass Co., Ltd.]. The alkaline portion of the re-sulting electrolytic water was taken to use as a weakly alkaline electrolytic water.
(2) Preparation of glucose solutions 14 g or 28 g of anhydrous glucose was dissolved in about 80 ml of the weakly alkaline electrolytic water prepared above. The same electrolytic water was further added to make the total volume 100 ml, whereby a 14 %
glucose solution and a 28% glucose solution were pre-pared. The 14% glucose solution had pH 9.l and the 28%
glucose solution had pH 8.61, right after the prepara-tion.
(3) Preparation of organogermanium compound solutions 1.847 g of the organogermanium compound (18) was weighed and added to about 2 ml of deionized water. The mixture was made weakly alkaline (pH 8.00 or 8.53) with a small amount of sodium hydroxide. The same deionized water was further added to make the total volume of 3 ml. The final concentration of the compound (18) in the solution was 1.67 M.
(4) Isomerization 200 N1 of the 14% or 28% glucose solution and 200~r1 of the organogermanium compound solution (pH 8.00 or 8.53) were placed in a small test tube. Also, 200 ul *Trade-mark C-A2 i 17472 of the 14% or 28% glucose solution and 200 N1 of the weakly alkaline electrolytic water were placed in a small test tube. Each test tube was thoroughly shaken and then placed in a water bath of 80°C to give rise to a reaction. 1-3 hours later, 50 ul of the reaction mix-ture was added to 50 ul of 0.5 N HC104 to terminate the reaction. Thereafter, the mixture was diluted 100-fold with deionized water to determine the amount of formed fructose and the amount of residual glucose by high-per-formance liquid chromatography using 7A (a column) manu-factured by Shimadzu Corp.
The results are shown in Table 6.
Table 6 Run Glucose pH of reaction Isomerization No. mixture ratio (%1 concentration I%1 1 (Ge)14 7.17 48.0 2 14 8.75 2.1 3 (Ge)7 7.52 73:1 4 7 9.03 3.1 (Ge)14 7.81 65.0 6 14 8.74 2.0 7 (Ge)7 8.15 94.7 8 7 9.03 3.5 9 (Na,Ge) 14 8.61 98.9 14 10.62 32.3 (Na) CA2ii7472 As is clear from Table 6, the isomerization ra-tios of glucose were 2.0 to 3.5% when a glucose solution was dissolved in a weakly alkaline electrolytic water alone. Meanwhile, when an organogermanium compound so-lution was further added, the isomerization ratios of glucose were 48.0 to 94.7%. Further, the isomerization ratio of glucose was 32.3% when sodium hydroxide was added to a glucose solution, while the isomerization ra-do of glucose was 98.9% when an organogermanium com-pound solution was further added.
Incidentally, in Table 6, (Ge) shows cases in which an organogermanium compound solution was added;
(Na) shows a case using sodium hydroxide and deionized water; in other cases, isomerization was conducted using weakly alkaline electrolytic water alone and without us-ing any of (Ge) and (rla).
Example 3 Other compounds represented by formula (I) were subjected to 3-hour isomerization in the same manner as in Example 2. The results are shown in Table 7.
Incidentally, compounds other than those shown in Table 7 showed substantially the same isomerization ratios.
CA2ii7472 U
~~ NC t~N V O .Hu7sY O O 07 Mtp M! M t0 GOO t~t~N M ..nOf WIff ?!~ < M M N It7M 0p t~
M
x t~< t~N M
V ! Y Of 00 t~ N ~t0 A Ml' M 1p ~ pf M W tp M 1A M n~
z ~.~ ~ ~ .o~ M ~o~o ~ a .~ <M
M!~ Ost~ N M o0OIN O 00 n op WM W t~ I'N .-~Oun .~ M O OCO
N~f N .~ t0 C' CO W N.~
x MM ~ C a0tp .~N a M N t~. Ot N O00 ! v0 0pM p C~O t~ N ID Nt~
z nto n to ton inr n n r .c cv ~~ tDN t0O .rM C M T ID t~ tD TIp OIt~ I~t~ b o0 10O N OI t~ u7 N.~
N Q
N
,xT'x MM tAM M N 47OIN 1~ p .r b OO ! N O M N OI.r Op pf pp Nd.
z MN N N N M .~ M N M N
"~ <CO C M t0M t0M N n < !' t0M
MN t~O Op.~ M < N O pu Op .-n.~
a M.w .-r.r .~ n N O < N
a ~"'IF' x na0 O M t0.-nN M u7 tp t0 1t7 pp~
O
!~.r O tD t~O .w0 O t~ N 0p NOp ,Z <V M M M C ~p? C M M M N.~
IG.r N O < < Iwp M O I~ N NV
O O f~ M M !~OIN 10 N t0 IDID
_N .w ~i a M M N
'IF x ICM N M COV eJN tp M N M %O
b NO W y~ t~C' O M O OI ~ .r nN
'~."NN .~ N .~N N .-n N ..n a .-nC~ M ID t~a M t0N Oo N M NO
.-nOoO O W N O O .~ M N 0poD
D
.rN a < V V
N
iF ~x MtD M < ~ Op O ~ .H Ip M a7. Qn N QN .~N O N OIC~e7.V M C~ OIp ,Z, NN N N N N .-~N N N N N
a '_~,t~m N Ic M ao ..N a c M .. ma VIIIt0t~ N M OWf700 V' OD N tpN
~ aa ooc~ I~m toa o. a~ m op mn iF ~x QI07 M < < 00 .yO a0 7 1f7t0 NI~
N 00(~ tptp M sT I~I~t~ tp N N M01 z o,of a a a m m a o, o~ o, of mI
~ -.N M a I mo opo n N a ., inlc N N M MM
U
z xx ~ ~ ~
A
C7 U t7 Ur V UYC~ V V p fJC7 CA2ii7472 Example 4 The same isomerization test as in Example 2 was conducted with slight modifications.
That is, 200 N1 of one of various saccharide so-lutions and 200 ul of one of various organogermanium compound solutions were placed in a small test tube.
The mixture was adjusted to pH 10 with an aqueous sodium hydroxide solution, after which the tube was placed in a water bath of 80°C for a reaction. 3 hours later, the reaction was terminated and the amount of each saccha-ride isomerized was determined by high-performance liq-uid chromatography using 7A (a column) manufactured by Shimadzu Corp.
The results are shown in Table 8.
Table 8 Organogermanium Isomerization (%) compound Galactose Ribose MaltoseArabinose Xvlose Mannose 1 38.67 27.76 78.91 20.87 40.66 37.23 8 40.60 29.60 80.41 22.22 33.26 39.18 17 16.38 27.06 53.84 7.96 25.88 16.53 22 19.72 57.98 49.26 11.49 31.24 38.20 Blank 7.60 2.89 12.59 2.75 5.59 12.48 Industrial Applicability C~2~3~4~2 As is shown from the foregoing Examples, the present isomerization process is free from the problems of prior art and can isomerize a compound having an al-dose structure into a compound having a ketose structure without requiring any special apparatus or any compli-cated operation.
This implies that an isomerized saccharose of desired concentration can be supplied, in a desired amount, to a processed food plant, for example, a plant for production of cold drink using an isomerized saccha-rose, by installing therein a small isomerization unit utilizing the technique of the present invention.
Further, when said isomerization unit is incorporated into a processed food production line, costs associated with transportation, storage and feeding of raw materi-als can be reduced significantly.
Further, the present process can isomerize a compound having an aldose structure into a compound hav-ing a ketose structure in the presence or absence of an isomerization enzyme. Even when no effective isomeriza-tion enzyme is found to exist for a particular compound of aldose structure to be isomerized into a correspond-ing ketose structure, the present process can isomerize such a compound into a compound having a ketose struc-ture by not resorting to the condition of heating under alkalinity (this condition is sometimes disadvantageous in isomerization ratio).
CA2ii7472 Furthermore, the present isomerization agent or accelerator effective for and used in carrying out the present process is very safe and highly stable.
higher than that of the blank, in all cases and there was substantially no difference in initial reaction rate between different organogermanium compounds. Meanwhile, the isomerization ratio in equilibrium varied depending upon the kinds of organogermanium compounds used; and the compound (23) gave an isomerization ratio of 99~, the compound (18) gave an isomerization ratio of 80$, and the compound (1) gave an isomerization ratio of 75~.
Example 2 (1) Preparation of weakly alkaline electrolytic water by electrolysis Water was passed through an apparatus for elec-trolysis [e.g. Microcluster* manufactured by Asahi Glass Co., Ltd.]. The alkaline portion of the re-sulting electrolytic water was taken to use as a weakly alkaline electrolytic water.
(2) Preparation of glucose solutions 14 g or 28 g of anhydrous glucose was dissolved in about 80 ml of the weakly alkaline electrolytic water prepared above. The same electrolytic water was further added to make the total volume 100 ml, whereby a 14 %
glucose solution and a 28% glucose solution were pre-pared. The 14% glucose solution had pH 9.l and the 28%
glucose solution had pH 8.61, right after the prepara-tion.
(3) Preparation of organogermanium compound solutions 1.847 g of the organogermanium compound (18) was weighed and added to about 2 ml of deionized water. The mixture was made weakly alkaline (pH 8.00 or 8.53) with a small amount of sodium hydroxide. The same deionized water was further added to make the total volume of 3 ml. The final concentration of the compound (18) in the solution was 1.67 M.
(4) Isomerization 200 N1 of the 14% or 28% glucose solution and 200~r1 of the organogermanium compound solution (pH 8.00 or 8.53) were placed in a small test tube. Also, 200 ul *Trade-mark C-A2 i 17472 of the 14% or 28% glucose solution and 200 N1 of the weakly alkaline electrolytic water were placed in a small test tube. Each test tube was thoroughly shaken and then placed in a water bath of 80°C to give rise to a reaction. 1-3 hours later, 50 ul of the reaction mix-ture was added to 50 ul of 0.5 N HC104 to terminate the reaction. Thereafter, the mixture was diluted 100-fold with deionized water to determine the amount of formed fructose and the amount of residual glucose by high-per-formance liquid chromatography using 7A (a column) manu-factured by Shimadzu Corp.
The results are shown in Table 6.
Table 6 Run Glucose pH of reaction Isomerization No. mixture ratio (%1 concentration I%1 1 (Ge)14 7.17 48.0 2 14 8.75 2.1 3 (Ge)7 7.52 73:1 4 7 9.03 3.1 (Ge)14 7.81 65.0 6 14 8.74 2.0 7 (Ge)7 8.15 94.7 8 7 9.03 3.5 9 (Na,Ge) 14 8.61 98.9 14 10.62 32.3 (Na) CA2ii7472 As is clear from Table 6, the isomerization ra-tios of glucose were 2.0 to 3.5% when a glucose solution was dissolved in a weakly alkaline electrolytic water alone. Meanwhile, when an organogermanium compound so-lution was further added, the isomerization ratios of glucose were 48.0 to 94.7%. Further, the isomerization ratio of glucose was 32.3% when sodium hydroxide was added to a glucose solution, while the isomerization ra-do of glucose was 98.9% when an organogermanium com-pound solution was further added.
Incidentally, in Table 6, (Ge) shows cases in which an organogermanium compound solution was added;
(Na) shows a case using sodium hydroxide and deionized water; in other cases, isomerization was conducted using weakly alkaline electrolytic water alone and without us-ing any of (Ge) and (rla).
Example 3 Other compounds represented by formula (I) were subjected to 3-hour isomerization in the same manner as in Example 2. The results are shown in Table 7.
Incidentally, compounds other than those shown in Table 7 showed substantially the same isomerization ratios.
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C7 U t7 Ur V UYC~ V V p fJC7 CA2ii7472 Example 4 The same isomerization test as in Example 2 was conducted with slight modifications.
That is, 200 N1 of one of various saccharide so-lutions and 200 ul of one of various organogermanium compound solutions were placed in a small test tube.
The mixture was adjusted to pH 10 with an aqueous sodium hydroxide solution, after which the tube was placed in a water bath of 80°C for a reaction. 3 hours later, the reaction was terminated and the amount of each saccha-ride isomerized was determined by high-performance liq-uid chromatography using 7A (a column) manufactured by Shimadzu Corp.
The results are shown in Table 8.
Table 8 Organogermanium Isomerization (%) compound Galactose Ribose MaltoseArabinose Xvlose Mannose 1 38.67 27.76 78.91 20.87 40.66 37.23 8 40.60 29.60 80.41 22.22 33.26 39.18 17 16.38 27.06 53.84 7.96 25.88 16.53 22 19.72 57.98 49.26 11.49 31.24 38.20 Blank 7.60 2.89 12.59 2.75 5.59 12.48 Industrial Applicability C~2~3~4~2 As is shown from the foregoing Examples, the present isomerization process is free from the problems of prior art and can isomerize a compound having an al-dose structure into a compound having a ketose structure without requiring any special apparatus or any compli-cated operation.
This implies that an isomerized saccharose of desired concentration can be supplied, in a desired amount, to a processed food plant, for example, a plant for production of cold drink using an isomerized saccha-rose, by installing therein a small isomerization unit utilizing the technique of the present invention.
Further, when said isomerization unit is incorporated into a processed food production line, costs associated with transportation, storage and feeding of raw materi-als can be reduced significantly.
Further, the present process can isomerize a compound having an aldose structure into a compound hav-ing a ketose structure in the presence or absence of an isomerization enzyme. Even when no effective isomeriza-tion enzyme is found to exist for a particular compound of aldose structure to be isomerized into a correspond-ing ketose structure, the present process can isomerize such a compound into a compound having a ketose struc-ture by not resorting to the condition of heating under alkalinity (this condition is sometimes disadvantageous in isomerization ratio).
CA2ii7472 Furthermore, the present isomerization agent or accelerator effective for and used in carrying out the present process is very safe and highly stable.
Claims (20)
1. ~A process which comprises isomerizing a compound having an aldose structure into a compound having a ketose structure, in the presence of an organogermanium compound represented by formula (II):
wherein R1, R2 and R3, which may be the same or different, independently represent a hydrogen atom, a lower alkyl group, a substituted or unsubstituted phenyl group, a carboxyl group, a carboxyalkyl group or an amino group which is unsubstituted or substituted with appropriate group(s); X1 represents a hydroxyl group, an O-lower alkyl group, an amino group or a salt represented by OY1 (Y1 represents a metal or a basic group-containing compound); and n represents an integer of 1 or more.
wherein R1, R2 and R3, which may be the same or different, independently represent a hydrogen atom, a lower alkyl group, a substituted or unsubstituted phenyl group, a carboxyl group, a carboxyalkyl group or an amino group which is unsubstituted or substituted with appropriate group(s); X1 represents a hydroxyl group, an O-lower alkyl group, an amino group or a salt represented by OY1 (Y1 represents a metal or a basic group-containing compound); and n represents an integer of 1 or more.
2. ~The process according to claim 1, wherein the organogermanium compound is represented by formula (II'):
in an aqueous solution, or formula (II"):
in crystal state, wherein R1, R2, R3, X1 and n are defined as in claim 1.
in an aqueous solution, or formula (II"):
in crystal state, wherein R1, R2, R3, X1 and n are defined as in claim 1.
3. ~The process according to claim 1, wherein the organogermanium compound is represented by formula (III):
wherein R4, R5 and R6, which may be the same or different, independently represent a hydrogen atom, a lower alkyl group, a substituted or unsubstituted phenyl group, a~
carboxyl group, a carboxyalkyl group or an amino group which is unsubstituted or substituted with appropriate group(s);
and X2 represents a hydroxyl group, an O-lower alkyl group, an amino group or a salt represented by OY2 (Y2 represents a metal or a basic group-containing compound).
wherein R4, R5 and R6, which may be the same or different, independently represent a hydrogen atom, a lower alkyl group, a substituted or unsubstituted phenyl group, a~
carboxyl group, a carboxyalkyl group or an amino group which is unsubstituted or substituted with appropriate group(s);
and X2 represents a hydroxyl group, an O-lower alkyl group, an amino group or a salt represented by OY2 (Y2 represents a metal or a basic group-containing compound).
4. ~The process according to any one of claims 1 to 3, wherein the isomerization is conducted without using any enzyme effective for that particular isomerization.
5. ~The process according to any one of claims 1 to 3, wherein the isomerization is conducted in the co-presence of an enzyme effective for that particular isomerization.
6. ~The process according to any one of claims 1 to 5, wherein the isomerization is conducted in neutrality to alkalinity.
7. ~The process according to any one of claims 1 to 6, wherein the isomerization is conducted in a weakly alkaline water obtained by electrolysis.
8. ~The process according to any one of claims 1 to 7, wherein the isomerization is conducted via an interim stage in which a cis-ene-diol structure is formed.
9. ~The process according to any one of claims 1 to 8, wherein the compound having an aldose structure is a monosaccharide.
10. ~The process according to any one of claims 1 to 3, wherein the compound having an aldose structure is glucose and is isomerized into fructose.
11. ~The process according to claim 10, wherein the isomerization of glucose into fructose is conducted in the co-presence of an isomerization enzyme.
12. ~The process according to claim 11, wherein the isomerization of glucose into fructose is conducted in the co-presence of a metal ion required by the isomerization enzyme.
13. ~The process according to any one of claims 10 to 12, wherein the isomerization of glucose into fructose is conducted in neutrality to alkalinity at a temperature of 60-90°C.
14. ~The process according to any one of claims 10 to 13, wherein the isomerization of glucose into fructose is conducted while controlling an isomerization reaction time to control an isomerization ratio.
15. ~The process according to any one of claims 10 to 14, wherein the isomerization of glucose into fructose is conducted until an isomerization degree into fructose reaches at least about 55%.
16. ~The process according to claim 10, wherein the isomerization of glucose into fructose is conducted in a solution which is a mixture of (1) a glucose-containing solution, (2) the organogermanium compound and (3) an isomerization enzyme.
17. ~The process according to claim 16, wherein the glucose-containing solution is a syrup obtained by liquefying starch and subjecting the resulting liquid to saccharification.
18. ~The process according to any one of claims 1 to 8, wherein the compound having an aldose structure is a disaccharide.
19. ~The process according to claim 18, wherein the compound having an aldose structure is lactose and is isomerized into lactulose.
20. ~The process according to any one of claims 1 to 8, wherein the compound having an aldose structure is an oligosaccharide or a polysaccharide.
Applications Claiming Priority (5)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| JP4360343A JPH06315391A (en) | 1992-12-28 | 1992-12-28 | Method for isomerizing glucose and isomerization promotor |
| JP4/360343 | 1992-12-28 | ||
| JP5188877A JPH0717991A (en) | 1993-06-30 | 1993-06-30 | Method for isomerizing aldose structure-having compound into ketose structure-having compound, isomerization and accelerating agent thereof |
| JP5/188877 | 1993-06-30 | ||
| PCT/JP1993/001896 WO1994014826A1 (en) | 1992-12-28 | 1993-12-27 | Process for isomerization of compound of aldose structure into compound of ketose structure, and isomerization agent or accelerator used therein |
Publications (2)
| Publication Number | Publication Date |
|---|---|
| CA2117472A1 CA2117472A1 (en) | 1994-07-07 |
| CA2117472C true CA2117472C (en) | 2006-06-13 |
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ID=36587328
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| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| CA002117472A Expired - Fee Related CA2117472C (en) | 1992-12-28 | 1993-12-27 | Process for isomerization of compound of aldose structure into compound of ketose structure, and isomerization agent or accelerator used therein |
Country Status (1)
| Country | Link |
|---|---|
| CA (1) | CA2117472C (en) |
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| Publication number | Publication date |
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| CA2117472A1 (en) | 1994-07-07 |
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