JP3043888B2 - Colorectal cancer prophylactic agent containing glucomannan partial hydrolyzate as active ingredient - Google Patents

Colorectal cancer prophylactic agent containing glucomannan partial hydrolyzate as active ingredient

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Publication number
JP3043888B2
JP3043888B2 JP4069364A JP6936492A JP3043888B2 JP 3043888 B2 JP3043888 B2 JP 3043888B2 JP 4069364 A JP4069364 A JP 4069364A JP 6936492 A JP6936492 A JP 6936492A JP 3043888 B2 JP3043888 B2 JP 3043888B2
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JP
Japan
Prior art keywords
glucomannan
partial hydrolyzate
molecular weight
average molecular
colorectal cancer
Prior art date
Legal status (The legal status 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 status listed.)
Expired - Lifetime
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JP4069364A
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Japanese (ja)
Other versions
JPH05246860A (en
Inventor
守 冨田
誠一 島村
康夫 福渡
和美 難波
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Morinaga Milk Industry Co Ltd
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Morinaga Milk Industry Co Ltd
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Application filed by Morinaga Milk Industry Co Ltd filed Critical Morinaga Milk Industry Co Ltd
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Publication of JP3043888B2 publication Critical patent/JP3043888B2/en
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  • Pharmaceuticals Containing Other Organic And Inorganic Compounds (AREA)
  • Polysaccharides And Polysaccharide Derivatives (AREA)

Description

【発明の詳細な説明】DETAILED DESCRIPTION OF THE INVENTION

【0001】[0001]

【産業上の利用分野】本発明は、平均分子量が2,00
0乃至5,000であるコンンニャク由来のグルコマン
ナンの部分加水分解物(以下、加水分解物と記載するこ
とがある)を有効成分とす大腸ガンの予防剤に関す
る。BACKGROUND OF THE INVENTION The present invention relates to an acetylene compound having an average molecular weight of 2,000.
0 to partial hydrolyzate of glucomannan derived Kon'n'nyaku 5,000 (hereinafter sometimes referred to as a hydrolyzate) on prevention agent for colon cancer shall be the active ingredient.

【0002】本明細書において百分率は、特に断りのな
い限り重量による値である。[0002] In the present specification, percentages are values by weight unless otherwise specified.

【0003】[0003]

【従来の技術】コンニャク粉は難消化性(左右田徳郎監
修、江上不二夫編集、「多糖類化学」第280頁、共立
出版、1955年)であり、水溶性多糖類であるグルコ
マンナンを約80%の濃度で含有するために水溶性食物
繊維、又は天然の低エネルギー食品及び医薬品原料とし
て使用されている。コンニャク粉は、それを人が摂取し
た場合には食物繊維として有益な効果を発現する反面、
(1)加工工程において水溶液が高粘度化すること、
(2)異臭を伴う好ましくない風味のために用途及び利
用形態が制限されること、(3)人の栄養上必要なミネ
ラルを吸着する性質がある等の欠点を有し、該コンニャ
ク粉を人が他の食品と同時に、又、該コンニャク粉を添
加した食品を摂取した場合、食品中のカルシウムを吸着
し、このためカルシウムの吸収が阻害され、生体のカル
シウム出納が負になり骨組織灰分の減少を惹起し、骨軟
化症の原因となる[ジャーナル・オブ・ニュートリショ
ン(Journal of Nutrition)、第
112巻、第410頁、1982年]等の問題を有す
る。2. Description of the Related Art Konjac flour is indigestible (edited by Tokuro Soda and edited by Fujio Egami, "Polysaccharide Chemistry", p. 280, Kyoritsu Shuppan, 1955), and contains about 80% of glucomannan, a water-soluble polysaccharide. It is used as a water-soluble dietary fiber, or as a natural low-energy food and pharmaceutical raw material because of its content. Konjac flour has a beneficial effect as dietary fiber when consumed by humans,
(1) The viscosity of the aqueous solution increases in the processing step;
The konjac flour is disadvantageous in that (2) its use and form of use are limited due to an unpleasant flavor accompanied by an off-flavor, and (3) it has the property of adsorbing minerals necessary for human nutrition. However, when ingesting a food to which the konjac flour is added at the same time as other foods, it absorbs calcium in the food, thereby inhibiting the absorption of calcium, negatively affecting the calcium balance of the living body, and reducing bone tissue ash content. It causes a decrease and causes problems such as osteomalacia [Journal of Nutrition, vol. 112, p. 410, 1982].

【0004】コンニャクのグルコマンナンを人が摂取し
た場合には人の消化酵素で消化されず、食餌又は胆汁酸
に由来するコレステロール及び胆汁中の胆汁酸を吸着し
て排泄することにより、血中コレステロール低下作用を
示す[ジャーナル・オブ・ニュートリション(Jour
nal of Nutrition)、第97巻、第3
82頁、1968年]ことが知られているが、このコレ
ステロール低下作用には食物繊維の高分子構造が不可欠
の条件である(印南敏・桐山修八編、「食物繊維」、第
145頁、第一出版、1982年)ことが報告されてい
る。従って、セルラーゼ又は酸で加水分解を行ったグル
コマンナンの血中コレステロール低下作用が消失する
[ジャーナル・オブ・ニュートリション(Journa
l ofNutrition)、第102巻、第168
9頁、1972年。アグリカルチュラル・アンド・バイ
オロジカル・ケミストリー(Agricultural
and Biological Chemistr
y)、第34巻、第641頁、1970年]ことが知ら
れている。When konjac glucomannan is ingested by humans, it is not digested by human digestive enzymes, and adsorbs and excretes cholesterol derived from the diet or bile acids and bile acids in bile, resulting in blood cholesterol. [Journal of Nutrition (Jour
nal of Nutrition), Vol. 97, No. 3
82, 1968], but the polymer structure of dietary fiber is an essential condition for this cholesterol-lowering effect (Satoshi Innan and Shuhei Kiriyama, "Dietary Fiber", p. 145, 1st publishing, 1982). Therefore, the blood cholesterol lowering effect of glucomannan hydrolyzed with cellulase or acid disappears [Journa of Nutrition (Journa).
l of Nutrition), Vol. 102, 168
9 pages, 1972. Agricultural and biological chemistry
and Biological Chemistr
y), 34, 641, 1970].

【0005】本発明者らは、先にカルシウム等の有用な
ミネラルの吸収を阻害せず、過量摂取しても下痢を誘発
しない、平均分子量が2,000乃至15,000のコ
ンニャク粉に含まれる多糖類の分解物からなる飲食品用
の水溶性食物繊維を発明し、出願した(特開平2−22
2659号公報。以下先願と記載する)。[0005] The present inventors have previously found that konjac flour having an average molecular weight of 2,000 to 15,000 does not inhibit the absorption of useful minerals such as calcium and does not induce diarrhea even when overdosed. Invented and filed a water-soluble dietary fiber for foods and drinks comprising a decomposed product of polysaccharide (Japanese Patent Laid-Open No. 22-22 / 1990).
No. 2659. Hereinafter referred to as the earlier application).

【0006】[0006]

【発明が解決しようとする課題】本発明者らは、先願を
出願した後、先願のコンニャク由来のグルコマンナンの
部分加水分解物の薬理作用について鋭意研究を行った。
その結果、高分子構造を有しない平均分子量が2,00
乃至5,000である特定のグルコマンナン部分加水
分解物が血中コレステロール低下作用を有するという従
来未知の新規な事実を発見した。After filing the prior application, the present inventors conducted intensive research on the pharmacological action of the partial hydrolyzate of glucomannan derived from konjac of the prior application.
As a result, the average molecular weight having no polymer structure is 2,000.
The present inventors have discovered a novel fact that a specific glucomannan partial hydrolyzate of 0 to 5,000 has a blood cholesterol lowering effect.

【0007】さらに本発明者らは、前記平均分子量が
2,000乃至5,000である特定のグルコマンナン
部分加水分解物が、血中コレステロール低下作用に加え
て、大腸ガンのプロモーター又は変異原物質として知ら
れている二次胆汁酸のデオキシコール酸及びリトコール
酸(光岡知足編、「腸内フローラの代謝」、第140
頁、学会出版センター、1988年)の生成を抑制する
作用を有するという、従来未知の更なる新規な事実を発
見した。Further, the present inventors have found that the average molecular weight is
The specific glucomannan partial hydrolyzate of from 2,000 to 5,000, in addition to its blood cholesterol-lowering effect, also has a secondary bile acid deoxycholic acid, which is known as a colorectal cancer promoter or mutagen, and Lithocholic acid (Toshimitsu Mitsuoka, “Metabolism of intestinal flora”, No. 140
Page, Academic Publishing Center, 1988).

【0008】本発明は、上述した新規発見事実に基づい
て完成されたものである。[0008] The present invention has been completed based on the above-described novel findings.

【0009】本発明は、コンニャク粉にみられる上述し
た欠点及び問題点が全くなく、血中コレステロール低下
作用を発揮しながら大腸ガン予防作用を発揮するグルコ
マンナン部分加水分解物を提供することを目的とする。It is an object of the present invention to provide a glucomannan partial hydrolyzate which does not have any of the above-mentioned drawbacks and problems found in konjac flour and has a blood cholesterol lowering effect and a colorectal cancer preventive effect. And

【0010】本発明の他の目的は、血中コレステロール
低下作用を発揮する平均分子量が2,000乃至5,0
00であるグルコマンナン部分加水分解物を提供するこ
とにある。Another object of the present invention is to provide a blood cholesterol lowering agent having an average molecular weight of 2,000 to 50,000.
It is to provide a glucomannan partial hydrolyzate which is 00.

【0011】本発明の他の目的は、血中コレステロール
低下作用を発揮するとともに大腸ガン予防作用を発揮す
る平均分子量が2,000乃至5,000であるグルコ
マンナン部分加水分解物を提供することにある。Another object of the present invention is to provide a glucomannan partial hydrolyzate having an average molecular weight of 2,000 to 5,000, which has a blood cholesterol lowering effect and a colorectal cancer preventing effect. is there.

【0012】本発明の他の目的は、平均分子量が2,0
00乃至5,000であるグルコマンナン部分加水分解
物を有効成分とする大腸ガン予防剤を提供することにあ
る。Another object of the present invention is to provide a polymer having an average molecular weight of 2,0.
It is an object of the present invention to provide a colorectal cancer preventive agent comprising a glucomannan partial hydrolyzate of from 00 to 5,000 as an active ingredient.

【0013】[0013]

【課題を解決するための手段】本発明の上記課題(即
ち、目的)は、平均分子量が2,000乃至5,000
であるコンニャク由来のグルコマンナンの特定の部分加
水分解物(以下単に、平均分子量が2,000乃至5,
000のグルコマンナン部分加水分解物という。)を使
用することにより達成される。SUMMARY OF THE INVENTION The object (namely, object) of the present invention is that the average molecular weight is from 2,000 to 5,000.
Is a specific partial hydrolyzate of glucomannan derived from konjac (hereinafter simply having an average molecular weight of 2,000 to 5,
000 glucomannan partial hydrolyzate. ) Is achieved.

【0014】以下、本発明について詳述する。本発明に
おける平均分子量が2,000乃至5,000のグルコ
マンナン部分加水分解物は、次のようにして製造され
る。Hereinafter, the present invention will be described in detail. The glucomannan partial hydrolyzate having an average molecular weight of 2,000 to 5,000 in the present invention is produced as follows.

【0015】即ち、市販の精粉、中粉、荒粉等のコンニ
ャク粉、コンニャク粉から分離したグルコマンナン、又
はアルコールで脱色、脱臭したコンニャク粉等を出発原
料として使用する。これらの出発原料の部分加水分解
(低分子化)は、公知の酸加水分解法又は酵素分解法に
より行うことができる。前記酸加水分解は多糖類の側鎖
が主鎖よりも早く分解されてしまう(特開昭63−26
9993号公報)ので、分解度を調整するためには、酵
素分解が望ましい。当該酵素分解に用いる酵素は、グル
コマンナンを加水分解する機能を有する市販の酵素が使
用できる。こうした酵素として、例えばアスペルギルス
・ニガー(Aspergillus niger)、ト
リコデルマ・ビリデ(Trichoderma vir
ide)、ペニシリウム・ノターツム(Penicil
lium notatum)、ストレプトマイセス属に
属する微生物(Streptomyces sp.)、
リゾプス・ニベウス(Rizopus niveus
u)、バシラス・サーキュランス(Bacillus
circulans)、コンニャク塊茎のマンナナーゼ
(mannanase)等を挙げることができる。これ
らのうち、グルコマンナンの分子内β−グルコシド結合
を加水分解するエンド型酵素、特にアスペルギルス属に
属する微生物に由来するセルラーゼが望ましい。That is, commercially available konjac flour such as refined, medium and coarse flour, glucomannan separated from konjac flour, or konjac flour decolorized and deodorized with alcohol are used as starting materials. Partial hydrolysis (low molecular weight) of these starting materials can be performed by a known acid hydrolysis method or enzymatic decomposition method. In the acid hydrolysis, the side chain of the polysaccharide is degraded faster than the main chain (Japanese Patent Application Laid-Open (JP-A) No. 63-26).
In order to adjust the degree of decomposition, enzymatic decomposition is desirable. A commercially available enzyme having a function of hydrolyzing glucomannan can be used as the enzyme used for the enzymatic decomposition. Such enzymes include, for example, Aspergillus
Niger (Aspergillus niger), Trichoderma virido ( Trichoderma vir)
ide), Penicillium notatum (Penicil)
ium notatum), a microorganism belonging to the genus Streptomyces (Streptomyces sp.),
Rizopus niveus
u), Bacillus
circulans), mannanase of konjac tubers, and the like. Of these, endo-type enzymes that hydrolyze intramolecular β-glucoside bonds of glucomannan, particularly cellulases derived from microorganisms belonging to the genus Aspergillus, are desirable.

【0016】上記酵素分解の際のpH及び反応時間は生
成物の分子量に大きな影響を及ぼす。即ち、市販酵素製
剤はエンド型及びエキソ型酵素の混合物であるため、酵
素中に含まれるエキソ型酵素の活性を低下させる条件で
酵素反応を行わせ、単糖の遊離量を最少に抑制する反応
液のpH及び反応時間を予め実験により決定する必要が
ある。例示すれば、後述する実施例1〜3のように、反
応条件を40〜60℃で4〜16時間保持するようにす
る。次いで反応液のpHを2〜5に調整し、加熱して酵
素を失活させると同時に蛋白質を除去し、上澄液を集
め、活性炭、合成吸着剤、又はイオン交換樹脂により、
不純物を除去する。又、必要に応じて更にUF膜、ルー
ズRO膜、セファデックスを用いたゲル濾過により、単
糖の除去又は所望の分子量分画を採取し、濃縮し、乾燥
して粉末化することもできる。The pH and reaction time during the enzymatic decomposition have a great influence on the molecular weight of the product. That is, since a commercially available enzyme preparation is a mixture of an endo-type enzyme and an exo-type enzyme, an enzyme reaction is carried out under conditions that reduce the activity of the exo-type enzyme contained in the enzyme, and a reaction that minimizes the amount of released monosaccharides. The pH of the solution and the reaction time must be determined in advance by experiments. For example, as in Examples 1 to 3 described below, the reaction conditions are maintained at 40 to 60 ° C. for 4 to 16 hours. Next, the pH of the reaction solution was adjusted to 2 to 5, and the protein was removed at the same time as heating to inactivate the enzyme, the supernatant was collected, and activated carbon, a synthetic adsorbent, or an ion exchange resin was used.
Remove impurities. Further, if necessary, a monosaccharide can be removed or a desired molecular weight fraction can be collected by gel filtration using a UF membrane, a loose RO membrane, or Sephadex, concentrated, dried and powdered.

【0017】本発明による平均分子量が2,000乃至
5,000のグルコマンナン部分加水分解物は、そのま
ま直接経口的に摂取することができる。この場合、本発
明による平均分子量が2,000乃至5,000のグル
コマンナン部分加水分解物を賦形剤と混合して製剤とす
ることもでき、他の血中コレステロール低下剤、又は大
腸ガン予防剤等と併用して製剤とすることもできる。
又、該グルコマンナン部分加水分解物は、種々の食品に
それらの特性を変化させること無くして添加することも
できる。後者の場合、例えば冷菓、パン、ゼリー等の固
形状の食品ばかりでなく牛乳、果汁等の液状食品にも安
定的に添加することが可能である。The partially hydrolyzed glucomannan having an average molecular weight of 2,000 to 5,000 according to the present invention can be directly orally ingested as it is. In this case, a partial hydrolyzate of glucomannan having an average molecular weight of 2,000 to 5,000 according to the present invention may be mixed with an excipient to prepare a formulation, and other blood cholesterol lowering agents or colorectal cancer prevention It can also be used as a preparation in combination with an agent.
Also, the glucomannan partial hydrolyzate can be added to various foods without changing their properties. In the latter case, it can be stably added not only to solid foods such as frozen desserts, breads and jellies, but also to liquid foods such as milk and fruit juice.

【0018】次に試験例を示して本発明を詳述する。Next, the present invention will be described in detail with reference to test examples.

【0019】(試験例1)この試験は、加水分解物の作
用を調べるために行った。(Test Example 1) This test was conducted to examine the action of the hydrolyzate.

【0020】(1)試料の調製 表1に示す成分の飼料を用いた。基礎飼料は、常法にお
ける標準的な飼料であるが、試験飼料は、基礎飼料にお
けるショ糖のうちの5%を、後述の実施例1(平均分子
量:2,000)、後述の実施例2(平均分子量:3,
000)、後述の実施例3(平均分子量:5,00
0)、後述の比較例1(平均分子量:600)、後述の
比較例2(平均分子量:15,000)及び後述の比較
例3(平均分子量:7,000)と同一の方法により調
製した加水分解物で置換した試験飼料である。(1) Preparation of samples Feeds having the components shown in Table 1 were used. The basal feed is a standard feed in a conventional method, but the test feed contains 5% of the sucrose in the basal feed as described in Example 1 described below (average molecular weight: 2,000) and Example 2 described later. (Average molecular weight: 3,
000) and Example 3 described below (average molecular weight: 5,000).
0), a water prepared by the same method as Comparative Example 1 (average molecular weight: 600), Comparative Example 2 (average molecular weight: 15,000) described later, and Comparative Example 3 (average molecular weight: 7,000) described later. This is a test feed that has been replaced with a degradation product.

【0021】[0021]

【表1】 *:各実施例及び比較例で得られたグルコマンナン部分
加水分解物[Table 1] *: Glucomannan partial hydrolyzate obtained in each of Examples and Comparative Examples

【0022】(2)試験方法 SD系ラット8匹を1群とする7群の試験動物群に、表
1に示す成分の試験飼料、基礎飼料を21日間給飼を行
った。7日間の間隔で尾静脈より採血を行い、抗凝固剤
のヘパリンを加えた後、この血液を3,000rpm、
15分間遠心分離し、血漿を得た。(2) Test Method Seven test animal groups, each group consisting of eight SD rats, were fed a test feed having the components shown in Table 1 and a basic feed for 21 days. Blood was collected from the tail vein at 7-day intervals, and heparin, an anticoagulant, was added.
Centrifugation was performed for 15 minutes to obtain plasma.

【0023】血漿コレステロール値は、総コレステロー
ル測定キット(共和メディクス社製、デタミナーTC5
55)を用い、比色定量した。The plasma cholesterol level was measured using a total cholesterol measurement kit (Kyowa Medix, Determiner TC5).
55) and colorimetrically determined.

【0024】さらに飼育最終日に新鮮糞便を集め、凍結
乾燥を行った後、常法により胆汁酸の抽出を行った。胆
汁酸は逆相カラムクロマトグラフを用いたHPLCによ
り、3α−hydroxysteroid dehyd
rogenaseによる酵素ポストラベル法によって分
析を行った。Further, on the last day of breeding, fresh feces were collected, freeze-dried, and bile acids were extracted by a conventional method. Bile acid was analyzed by HPLC using reverse-phase column chromatography to obtain 3α-hydroxysteroid dehydrogen.
The analysis was performed by the enzyme post-labeling method using R. genase.

【0025】(3)試験結果 この試験結果は、図1及び表2に示すとおりである。図
の縦軸及び横軸は、それぞれ血中コレステロール及び日
数を表し、図中−●−は基礎飼料投与群、−○−は実施
例1の部分加水分解物を用いた5%投与群、−◇−は実
施例2の部分加水分解物を用いた5%投与群、−◆−は
実施例3の部分加水分解物を用いた5%投与群、−□−
は比較例1の部分加水分解物を用いた5%投与群、−△
−は比較例2の部分加水分解物を用いた5%投与群、−
▲−は比較例3の部分加水分解物を用いた5%投与群を
それぞれ示す。(3) Test Results The test results are as shown in FIG. 1 and Table 2. The vertical and horizontal axes in the figure represent blood cholesterol and the number of days, respectively. In the figure,-●-is a basal feed administration group,-○-is a 5% administration group using the partial hydrolyzate of Example 1,- ◇-is a 5% administration group using the partial hydrolyzate of Example 2,-◆-is a 5% administration group using the partial hydrolyzate of Example 3,-□-
Is a 5% administration group using the partial hydrolyzate of Comparative Example 1,-△
-Is a 5% administration group using the partial hydrolyzate of Comparative Example 2,-
−- indicates a 5% administration group using the partial hydrolyzate of Comparative Example 3, respectively.

【0026】図1から明らかなように本発明の加水分解
物を投与した群では、投与開始7日間はその効果が認め
られなかったが、7日以降は顕著な血中コレステロール
低下が認められた。しかしながら、平均分子量600、
平均分子量7,000及び平均分子量15,000の加
水分解物ではその作用は認められなかった。As is clear from FIG. 1, in the group to which the hydrolyzate of the present invention was administered, no effect was observed for 7 days after the administration, but a marked decrease in blood cholesterol was observed after 7 days. . However, average molecular weight 600,
No effect was observed in the hydrolyzate having an average molecular weight of 7,000 and an average molecular weight of 15,000.

【0027】表2に二次胆汁酸であるデオキシコール酸
及びリトコール酸の生成量を示した。Table 2 shows the amounts of secondary bile acids deoxycholic acid and lithocholic acid produced.

【0028】表2の結果から次のことがわかった。即
ち、後述の実施例1、2及び3のグルコマンナン部分加
水分解物投与群は、基礎飼料投与群、後述の比較例1、
2及び3のグルコマンナン部分加水分解物投与群と比較
して二次胆汁酸量が低下した。尚、他の方法で調整した
グルコマンナン加水分解物を使用した場合もほぼ同等の
結果が得られた。From the results in Table 2, the following was found. That is, the glucomannan partial hydrolyzate administration group of Examples 1, 2 and 3 described below is a basal feed administration group, Comparative Example 1 described below,
The amount of secondary bile acids was reduced as compared with the glucomannan partial hydrolyzate administration groups 2 and 3. In addition, when the glucomannan hydrolyzate prepared by another method was used, almost the same results were obtained.

【0029】[0029]

【表2】 [Table 2]

【0030】[0030]

【比較例1】セルラーゼによる酵素反応の時間を24時
間としたこと、及び加熱時のpHを2.0に調整したこ
と以外は、下記の実施例1と同様の方法により、グルコ
マンナン部分加水分解物約2,500gを得た。この部
分加水分解物の平均分子量は600であった。Comparative Example 1 Glucomannan partial hydrolysis was carried out in the same manner as in Example 1 below, except that the time of the enzyme reaction with cellulase was set to 24 hours and the pH during heating was adjusted to 2.0. About 2,500 g of the product was obtained. The average molecular weight of this partial hydrolyzate was 600.

【0031】[0031]

【比較例2】セルラーゼによる酵素反応の時間を3.5
時間としたこと以外は、下記の実施例3と同様の方法に
より、精製したグルコマンナン部分加水分解物約4,3
00gを得た。この部分加水分解物の平均分子量は1
5,000であった。[Comparative Example 2] The enzymatic reaction time by cellulase was 3.5.
A glucomannan partial hydrolyzate purified by the same method as in Example 3 described below except that
00 g were obtained. The average molecular weight of this partial hydrolyzate is 1
It was 5,000.

【0032】[0032]

【比較例3】セルラーゼによる酵素反応の時間を8時間
としたこと、及び加熱時のpHを3.0に調整したこと
以外は、下記の実施例1と同様の方法により、グルコマ
ンナン部分加水分解物約980gを得た。この部分加水
分解物の平均分子量は7,000であった。Comparative Example 3 Glucomannan partial hydrolysis was carried out in the same manner as in Example 1 below, except that the time of the enzyme reaction with cellulase was set to 8 hours and the pH during heating was adjusted to 3.0. About 980 g of the product was obtained. The average molecular weight of this partial hydrolyzate was 7,000.

【0033】次に実施例を示して本発明を更に詳述する
が、本発明は以下の実施例に限定されるものではない。Next, the present invention will be described in more detail by way of examples, but the present invention is not limited to the following examples.

【0034】[0034]

【実施例1】燐酸緩衝液(pH6.5)40lに市販の
セルラーゼアマノ(天野製薬製、繊維素糖化力15,0
00U/g)120gを添加し、50℃に加温しながら
市販のコンニャク粉4.0kgを撹拌溶解し、50℃に
16時間保持し、のち塩酸でpH4.5に調整し、95
℃で10分間加熱した。この反応液を珪藻土濾過により
残渣を分離し、上澄液を活性炭500ml、陽イオン交
換樹脂ダウエックス50W×8(H+)1,000ml
及び陰イオン交換樹脂ダウエックス1×8(OH-
4,000mlに順次通液して脱塩精製し、濃縮し、噴
霧乾燥し、グルコマンナン部分加水分解物約2,550
gを得た。この部分加水分解物の平均分子量は2,00
0であった。Example 1 A commercially available cellulase Amano (manufactured by Amano Pharmaceutical Co., Ltd., fibrous saccharifying power 15.0) was added to 40 l of a phosphate buffer (pH 6.5).
(00 U / g), and 120 kg of commercially available konjac flour was stirred and dissolved while heating to 50 ° C., kept at 50 ° C. for 16 hours, and then adjusted to pH 4.5 with hydrochloric acid.
Heated at ° C for 10 minutes. The residue was separated from the reaction solution by diatomaceous earth filtration, and the supernatant was used for activated carbon (500 ml) and cation exchange resin Dowex (50 W × 8 (H + ), 1,000 ml).
And anion exchange resin Dowex 1 × 8 (OH -)
The mixture was passed through 4,000 ml in order to purify, desalted, concentrated, spray-dried, and partially hydrolyzed with glucomannan of about 2,550.
g was obtained. The average molecular weight of this partial hydrolyzate is 2,000
It was 0.

【0035】[0035]

【実施例2】セルラーゼによる酵素反応の時間を12時
間としたこと、及び加熱時のpHを5.0に調整したこ
と以外は、実施例1と同様の方法により、グルコマンナ
ン部分加水分解物約2,540gを得た。この部分加水
分解物の平均分子量は3,000であった。Example 2 A glucomannan partial hydrolyzate was prepared in the same manner as in Example 1 except that the time of the enzyme reaction with cellulase was set to 12 hours, and the pH during heating was adjusted to 5.0. 2,540 g were obtained. The average molecular weight of this partial hydrolyzate was 3,000.

【0036】[0036]

【実施例3】酢酸緩衝液(pH4.5)90lに市販の
セルレースナガセ(ナガセ生化学工業製、繊維素糖化力
1,000U/g)60gを添加し、60℃に加温しな
がら市販のコンニャク粉10.0kgを撹拌溶解し、6
0℃に5時間保持し、のち塩酸でpH4.5に調整し、
95℃で10分間加熱した。この反応液を珪藻土濾過に
より残渣を分離し、上澄液を活性炭2,000ml、陽
イオン交換樹脂ダウエックス50W×8(H+)2,5
00ml及び陰イオン交換樹脂ダウエックス1×8(O
-)6,000mlに順次通液して脱塩精製し、濃縮
し、噴霧乾燥し、グルコマンナン部分加水分解物約5,
130gを得た。この部分加水分解物の平均分子量は
5,000であった。Example 3 60 g of commercially available cellulase Nagase (manufactured by Nagase Seikagaku Kogyo Co., Ltd., with a saccharifying power of 1,000 U / g) was added to 90 l of an acetate buffer (pH 4.5), and the mixture was heated to 60 ° C. and marketed Dissolve 10.0 kg of konjac flour with stirring.
Hold at 0 ° C. for 5 hours, then adjust to pH 4.5 with hydrochloric acid,
Heated at 95 ° C. for 10 minutes. The residue was separated from the reaction mixture by diatomaceous earth filtration, and the supernatant was separated from activated carbon (2,000 ml) and a cation exchange resin Dowex 50W × 8 (H + ) 2.5.
00 ml and anion exchange resin Dowex 1 × 8 (O
H ) was sequentially passed through 6,000 ml, desalted and purified, concentrated, spray-dried, and partially hydrolyzed with glucomannan partially
130 g were obtained. The average molecular weight of this partial hydrolyzate was 5,000.

【0037】[0037]

【発明の効果】本発明によって奉せられる効果は次のと
おりである。The effects provided by the present invention are as follows.

【0038】(1)本発明の平均分子量が2,000乃
至5,000のグルコマンナン部分加水分解物は、血中
コレステロール低下作用を有する。(1) The glucomannan partial hydrolyzate of the present invention having an average molecular weight of 2,000 to 5,000 has a blood cholesterol lowering effect.

【0039】(2)本発明の平均分子量が2,000乃
至5,000のグルコマンナン部分加水分解物は、二次
胆汁酸生成抑制作用を有するので、大腸ガンの予防に有
効である。(2) The glucomannan partial hydrolyzate of the present invention having an average molecular weight of 2,000 to 5,000 has an inhibitory effect on secondary bile acid production, and is therefore effective in preventing colon cancer.

【0040】(3)本発明の平均分子量が2,000乃
至5,000のグルコマンナン部分加水分解物は、これ
を食品に加えても、食品の官能的特性に影響を与えな
い。(3) The partial hydrolyzate of glucomannan having an average molecular weight of 2,000 to 5,000 according to the present invention does not affect the sensory characteristics of food even when it is added to food.

【図面の簡単な説明】[Brief description of the drawings]

【図1】図は飼育日数と血中コレステロールの関係を示
す。FIG. 1 shows the relationship between the days of breeding and blood cholesterol.

───────────────────────────────────────────────────── フロントページの続き (56)参考文献 特開 平2−222659(JP,A) (58)調査した分野(Int.Cl.7,DB名) A61K 31/715 C08B 37/00 ──────────────────────────────────────────────────続 き Continuation of the front page (56) References JP-A-2-22659 (JP, A) (58) Fields investigated (Int. Cl. 7 , DB name) A61K 31/715 C08B 37/00

Claims (1)

(57)【特許請求の範囲】(57) [Claims] 【請求項1】 コンンニャク由来のグルコマンナンを酵
素分解し、精製して得られる平均分子量が2,000乃
至5,000であるグルコマンナン部分加水分解物を有
効成分とする大腸ガン予防剤。An agent for preventing colorectal cancer comprising as an active ingredient a partially hydrolyzed glucomannan having an average molecular weight of 2,000 to 5,000, which is obtained by enzymatically decomposing and purifying konjac-derived glucomannan.
JP4069364A 1992-02-20 1992-02-20 Colorectal cancer prophylactic agent containing glucomannan partial hydrolyzate as active ingredient Expired - Lifetime JP3043888B2 (en)

Priority Applications (1)

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JP4069364A JP3043888B2 (en) 1992-02-20 1992-02-20 Colorectal cancer prophylactic agent containing glucomannan partial hydrolyzate as active ingredient

Applications Claiming Priority (1)

Application Number Priority Date Filing Date Title
JP4069364A JP3043888B2 (en) 1992-02-20 1992-02-20 Colorectal cancer prophylactic agent containing glucomannan partial hydrolyzate as active ingredient

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JP3043888B2 true JP3043888B2 (en) 2000-05-22

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* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
AUPM322393A0 (en) * 1993-12-24 1994-01-27 Austin Research Institute, The Mucin carbohydrate compounds and their use in immunotherapy
US8021667B2 (en) 1994-11-16 2011-09-20 Macfarlane Burnet Institute For Medical Research And Public Health Ltd Compositions for immunotherapy and uses thereof
US6548643B1 (en) 1994-11-16 2003-04-15 Austin Research Institute Antigen carbohydrate compounds and their use in immunotherapy
ES2322212T3 (en) 1997-09-29 2009-06-17 The Macfarlane Burnet Institute For Medical Research And Public Health Ltd COMPOSITION OF ANTIGEN AND CELL LINE THAT CARRIES THE HANDY RECEIVER.
US7408057B2 (en) 2000-07-03 2008-08-05 Marine Bioproducts Intenational Clarified hydrocolloids of undiminished properties and method of producing same
JP2002262827A (en) * 2001-03-13 2002-09-17 Ajinomoto General Foods Inc Serum lipid improving composition containing mannooligosaccharide
JP4115183B2 (en) * 2002-07-16 2008-07-09 ユニチカ株式会社 Feed additive, feed and egg to which it is added
JP4728572B2 (en) * 2003-11-11 2011-07-20 国立大学法人広島大学 Allergy improvement agent
JP4488852B2 (en) * 2004-09-17 2010-06-23 味の素ゼネラルフーヅ株式会社 Composition having body fat reducing action
JP4673753B2 (en) * 2006-01-16 2011-04-20 味の素ゼネラルフーヅ株式会社 Serum lipid improving agent containing mannooligosaccharide
JP2009275047A (en) * 2009-06-30 2009-11-26 Ajinomoto General Foods Inc Composition having body fat reducing action and food and drink containing the same
JP6894789B2 (en) * 2016-07-22 2021-06-30 新一郎 石橋 Bile acid adsorbent, its manufacturing method, and beverages containing bile acid adsorbent
CN107936135B (en) * 2017-12-14 2020-05-26 宁波拜尔玛生物科技有限公司 Preparation method and application of high-purity mannan

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