JP2993724B2 - Stabilized yellow dye - Google Patents

Stabilized yellow dye

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Publication number
JP2993724B2
JP2993724B2 JP2275284A JP27528490A JP2993724B2 JP 2993724 B2 JP2993724 B2 JP 2993724B2 JP 2275284 A JP2275284 A JP 2275284A JP 27528490 A JP27528490 A JP 27528490A JP 2993724 B2 JP2993724 B2 JP 2993724B2
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JP
Japan
Prior art keywords
dye
pigment
present
crocin
glycoside
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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JP2275284A
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Japanese (ja)
Other versions
JPH04153271A (en
Inventor
正宏 中尾
祐子 福井
茂昭 藤川
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Suntory Ltd
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Suntory Ltd
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Description

【発明の詳細な説明】 〔産業上の利用分野〕 本発明は天然黄色系色素及びその製造方法並びにその
用途に関する。The present invention relates to a natural yellow pigment, a method for producing the same, and uses thereof.

〔従来の技術〕[Conventional technology]

カロチノイド系色素の配糖体、特にクチナシ黄色色素
は、耐光性、耐酸性に劣り、その使用範囲は限定されて
いた。例えば、クロシンは、使用する食品、飲料などに
含まれる酵素β−グルコシダーゼ、酸、アルカリの作用
によってその糖質であるゲンチオビオースがはずれクロ
セチンとなり、水での溶解性が著しく低下するという問
題が指摘されていた。Glycosides of carotenoid pigments, especially gardenia yellow pigments, are inferior in light resistance and acid resistance, and their use range is limited. For example, it has been pointed out that crocin loses gentiobiose, which is a saccharide thereof, due to the action of an enzyme β-glucosidase, an acid, or an alkali contained in foods and beverages to be used, becomes crocetin, and significantly reduces the solubility in water. I was

この色素の安定性の向上の目的で、サイクロデキスト
リンを加える方法(特開昭54−117536号公報)、アスコ
ルビン酸、ポリリン酸を加える方法(特公昭51−37336
号公報)、茶類の抽出物を加える方法(特開昭62−1269
53号公報)が知られている。For the purpose of improving the stability of the dye, a method of adding cyclodextrin (JP-A-54-117536), a method of adding ascorbic acid and polyphosphoric acid (JP-B-51-37336).
JP-A-62-1269), and a method of adding an extract of teas
No. 53) is known.

しかしこれらの方法では、一定の安定性の向上は認め
られるものの実用に耐えるほどの向上でなかったり、本
来の色素成分以外のものを添加するため、その添加物の
作用により、例えば溶解性の低下、酸味もしくは苦味の
増強、および色調変化などの難点が生起する可能性があ
るとの指摘がある。さらに上記の方法ではクロセチンへ
の分解を阻害する効果は認められない。また、配糖体を
持つ色素の安定性向上の方法としてアントシアニン系色
素の配糖体に酵素サイクロデキストリングルカノトラン
スフェラーゼを用いて、サイクロデキストリン、デキス
トリンなどの糖を転移反応させる方法も知られている
(特開昭63−43959号公報)が、アントシアニン以外の
色素の配糖体への糖転移色素はいまだ知られていない。However, in these methods, although a certain improvement in stability is observed, the improvement is not enough to endure practical use, or because other than the original dye component is added, the action of the additive causes a decrease in solubility, for example. It is pointed out that difficulties such as enhancement of acidity or bitterness and color tone change may occur. Furthermore, the above method has no effect of inhibiting the decomposition into crocetin. In addition, as a method for improving the stability of a pigment having a glycoside, there is also known a method in which a sugar such as cyclodextrin or dextrin is subjected to a transfer reaction using an enzyme cyclodextrin glucanotransferase in a glycoside of an anthocyanin-based pigment. (Japanese Unexamined Patent Publication (Kokai) No. 63-43959), a glycosyl transfer dye to a glycoside of a dye other than anthocyanin has not yet been known.

〔発明が解決しようとする課題〕[Problems to be solved by the invention]

本発明は新規なカロチノイド系色素、特にクチナシの
実から得たクロシンを主成分とする黄色色素に転移酵素
を用いて各種の糖を転移縮合させた色素を提供し、従来
技術に包含される課題、特に色素の安定性の向上を図る
ことを目的とする。The present invention provides a novel carotenoid pigment, particularly a pigment obtained by transfer-condensation of various sugars using a transferase to a yellow pigment containing crocin as a main component obtained from gardenia fruits, and the problems involved in the prior art are provided. In particular, it is intended to improve the stability of the dye.

〔課題を解決するための手段〕[Means for solving the problem]

本発明者らは、上記課題を解決すべく鋭意研究を重ね
た結果、クチナシの実から得られるクロシンを主成分と
する黄色色素に各種の糖、例えば澱粉、グリコーゲン、
サイクロデキストリン、デキストリン、その他のオリゴ
糖、例えば、乳糖、砂糖、キシロオリゴ糖等のいずれか
を単独でまたはそれらの2種以上を加え、それぞれに対
応する転移酵素の存在下でクロシンを主成分とする黄色
色素を処理することにより各種糖質が縮合した新規な色
素が得られ、かつこの色素は従来知られているクチナシ
黄色系色素に比べて低いpHでの熱安定性が良く、光に安
定であり、さらにβ−グルコシダーゼに対する安定性が
増すことを見いだし本発明を完成した。The present inventors have conducted intensive studies to solve the above-mentioned problems, and as a result, various sugars, such as starch, glycogen, and the like, in a yellow pigment mainly containing crocin obtained from gardenia fruits.
Cyclodextrin, dextrin, and other oligosaccharides, for example, lactose, sugar, xylo-oligosaccharides, etc., alone or in combination of two or more thereof, with crosin as the main component in the presence of the corresponding transferase By treating the yellow pigment, a novel pigment in which various carbohydrates are condensed can be obtained, and this pigment has better heat stability at a lower pH than conventional known gardenia yellow pigment, and is stable to light. In addition, the inventors have found that the stability to β-glucosidase is increased, and completed the present invention.

従って、本発明によれば、カロチノイド系色素の配糖
体の水酸基に糖質が縮合した新規カロチノイド系色素が
提供され、さらにそれらの製造方法および用途が提供さ
れる。Therefore, according to the present invention, there is provided a novel carotenoid pigment in which a carbohydrate is condensed to a hydroxyl group of a glycoside of a carotenoid pigment, and a method for producing the carotenoid pigment and a use thereof are provided.

以下、本発明を具体的に説明する。 Hereinafter, the present invention will be described specifically.

本発明のカロチノイド系色素には、その製造に用いる
出発原料色素および新たな糖鎖を供与する糖質(「供与
体糖質」と称する)の種類に応じて多種多様な糖質縮合
体が包含される。このようなカロチノイド系色素として
は、詳細については後述するような本発明の酵素転移反
応を利用して製造できるものであればその起源を問わな
いが、特にクチナシ黄色色素、すなわちクロシンの配糖
体の水酸基に前述の各種糖が縮合したものを挙げること
ができ、より具体的には第1−a図と第2図、第4図と
第5図、第6図と第7図、および第9図によってそれぞ
れ特定されるような色素混合物、ならびにその各構成色
素を挙げることができる。本発明にいう「縮合」したと
は、クロシンの糖鎖(ゲンチオビース由来)部分の水酸
基に供与体糖質の水酸基が対応する糖転移酵素の作用に
より脱水縮合したものをいう。この縮合は、使用する酵
素により異なるが、サイクロデキストリングルカノトラ
ンスフェラーゼの場合、前記糖鎖の4位の水酸基にグル
コースが1〜6(主に6)個、α−1,4結合を介して結
合し、α−グルコシダーゼの場合は、前記糖鎖の6位の
水酸基にグルコースがα−1,6結合し、β−ガラクトシ
ダーゼの場合は、前記糖鎖の4位の水酸基にガラクトー
スがβ−1,4結合した物が主であると推定される。従っ
て、本発明の色素類は用いる供与体糖質、転移酵素およ
び/または反応時間によって様々な糖鎖の縮合したクロ
シン色素類が提供される。The carotenoid pigment of the present invention includes a wide variety of carbohydrate condensates depending on the type of the starting material pigment used for the production and the kind of carbohydrate donating a new sugar chain (referred to as “donor carbohydrate”). Is done. Such a carotenoid pigment may be of any origin as long as it can be produced by utilizing the enzymatic transfer reaction of the present invention as described in detail later, but particularly the gardenia yellow pigment, that is, the glycoside of crocin 1-a and FIG. 2, FIG. 4 and FIG. 5, FIG. 6 and FIG. 7, and FIG. Dye mixtures as specified by FIG. 9 as well as their constituent dyes can be mentioned. The term “condensed” as used in the present invention refers to a product obtained by dehydrating and condensing a hydroxyl group of a donor saccharide by a corresponding glycosyltransferase to a hydroxyl group of a sugar chain (derived from gentiobiose) of crocin. This condensation differs depending on the enzyme used. In the case of cyclodextrin glucanotransferase, 1 to 6 (mainly 6) glucoses are bonded to the hydroxyl group at the 4-position of the sugar chain via α-1,4 bonds. However, in the case of α-glucosidase, glucose is α-1,6 bonded to the hydroxyl group at position 6 of the sugar chain, and in the case of β-galactosidase, galactose is β-1 ,, at the hydroxyl group at position 4 of the sugar chain. It is presumed that the one with four bonds is the main. Therefore, the dyes of the present invention provide crocin dyes in which various sugar chains are condensed depending on the donor saccharide, transferase and / or reaction time used.

これらの色素類は、より具体的にはもう一つの本発明
である、カロチノイド系色素の配糖体および糖質の存在
下で糖転移酵素を用いて転移反応を起こすことにより前
記配糖体の水酸基に前記糖質を縮合させることを特徴と
する方法によって製造することができる。本発明で用い
る各種糖転移酵素は、用いる供与体糖質によって適切な
組み合わせが存在するので、縮合させる糖質に応じて酵
素の種類を選んで用いることが好ましい。すなわち、ク
チナシ黄色色素であるクロシンにデキストリン、澱粉ま
たはマルトオリゴ糖等の糖質を縮合させる場合には、サ
イクロデキストリン・グルカノトランスフェラーゼ(CG
Tase E.C.2.4.1.19)、好ましくはバチラス属菌由来のC
GTaseを作用させることにより本発明の色素類を製造す
ることができる。また同様に糖質として乳糖、ガラクト
オリゴ糖を用いる場合にはβ−ガラクトシダーゼを、砂
糖を用いる場合にはインベルターゼ、あるいはシュクラ
ーゼを、キシラン、キシロオリゴ糖を用いる場合にはキ
シラナーゼを作用させることにより本発明の色素類を製
造することができる。使用する酵素により異なるが、CG
Taseの反応に際し、クロシンを主成分とする黄色色素0.
1〜8%(望ましくは0.5〜4%)、デキストリン0.5〜4
0%(望ましくは5〜20%)CGTase5ユニット/gデキスト
リン以上(望ましくは10ユニット/gデキストリン以上)
を用いる。使用する緩衝液とその濃度は酵素反応を阻害
しないものであれば、自由に選択することが出来る。例
えば50mMリン酸緩衝液が挙げられる。そのpHは5〜8
(望ましくは6)が適当であり、反応温度は35〜50℃が
適当であり、適宜液体クロマトグラフィーにより反応混
合物の組成を確認し反応の終了とすればよい。These pigments are more specifically another invention of the present invention, in which a glycosyltransferase of the carotenoid pigment and a glycosyltransferase are used to cause a transfer reaction in the presence of a carbohydrate to thereby form the glycoside. It can be produced by a method characterized by condensing the saccharide with a hydroxyl group. Since various types of glycosyltransferases used in the present invention have an appropriate combination depending on the donor saccharide used, it is preferable to select and use the type of enzyme according to the saccharide to be condensed. That is, when saccharide such as dextrin, starch or maltooligosaccharide is condensed with crocin, a gardenia yellow pigment, cyclodextrin-glucanotransferase (CG
Tase EC2.4.1.19), preferably C from Bacillus sp.
The dyes of the present invention can be produced by allowing GTase to act. Similarly, lactose as a saccharide, β-galactosidase when using galactooligosaccharides, invertase or sucralase when using sugar, xylan, and xylanase when using xylo-oligosaccharides act on the xylanase of the present invention. Pigments can be produced. Depending on the enzyme used, CG
In the reaction of Tase, yellow pigment mainly composed of crocin
1-8% (preferably 0.5-4%), dextrin 0.5-4
0% (preferably 5 to 20%) CGTase 5 units / g dextrin or more (preferably 10 units / g dextrin or more)
Is used. The buffer used and its concentration can be freely selected as long as they do not inhibit the enzyme reaction. For example, a 50 mM phosphate buffer may be mentioned. Its pH is 5-8
(Preferably 6) is appropriate, the reaction temperature is suitably 35 to 50 ° C., and the composition of the reaction mixture may be appropriately confirmed by liquid chromatography to terminate the reaction.

反応生成物は常法、すなわち、吸着樹脂あるいは限外
濾過その他の方法を用いて分離精製すればよく、精製を
終わった色素液は濃縮または凍結乾燥などにより目的と
する本発明の安定化黄色色素を単品または混合物として
得ることができる。The reaction product may be separated and purified by a conventional method, that is, by using an adsorption resin or ultrafiltration or another method.The purified dye solution may be concentrated or freeze-dried to obtain the stabilized yellow dye of the present invention. Can be obtained individually or as a mixture.

使用にあたっては、上記の方法で得られた溶液のま
ま、もしくは適当に希釈または濃縮して使用しても良
く、あるいは所望により乾燥して粉末状態で使用しても
良い。さらに、使用目的に応じてそのまま、または他の
色素と組み合わせて使用することができる。Upon use, the solution obtained by the above method may be used as it is, or may be used after being appropriately diluted or concentrated, or may be dried and used in a powdered state if desired. Further, they can be used as they are or in combination with other dyes depending on the purpose of use.

〔実施例〕〔Example〕

以下、実施例に従って本発明を更に詳しく説明する
が、本発明は実施例に限定されるものではない。Hereinafter, the present invention will be described in more detail with reference to examples, but the present invention is not limited to the examples.

実施例1 クチナシ黄色色素(色価▲E10W% 1cm▼=2000)0.5
g、デキストリン5gを50mMリン酸緩衝液(pH6)100mに
溶解し、酵素CGTase(天野製薬(株)コンチザイム)を
25ユニット加え、45℃で24時間反応させた。得られた本
発明の色素類混合物は、第1図のクロマトグラムで示さ
れる組成と、第2図の紫外部および可視部の吸収スペク
トルを示す。Example 1 Gardenia yellow pigment (color value ▲ E 10W% 1cm ▼ = 2000) 0.5
g and 5 g of dextrin are dissolved in 100 mM of 50 mM phosphate buffer (pH 6), and the enzyme CGTase (Antano Pharmaceutical Co., Ltd. Contizyme) is dissolved.
25 units were added and reacted at 45 ° C. for 24 hours. The obtained dye mixture of the present invention shows the composition shown in the chromatogram in FIG. 1 and the absorption spectrum in the ultraviolet and visible regions in FIG.

色調の安定性 本色素およびコントロールとして原料のクロシンを主
成分とする黄色色素をそれぞれ、pH3もしくは6のマッ
クルベイン緩衝液中で調製時および12,000ルクス蛍光燈
20時間照射後の吸光度、100℃で1時間、37℃で4日、
7日保持した後の吸光度を第1表に示す。Color Tone Stability This dye and a yellow dye mainly composed of crocin as a control were prepared in McClubane buffer at pH 3 or 6, respectively.
Absorbance after irradiation for 20 hours, 1 hour at 100 ° C, 4 days at 37 ° C,
Table 1 shows the absorbance after holding for 7 days.

以上の結果から、本色素は原料色素自体より特に低pH
領域で著しい安定性を示すことが明らかになった。 From the above results, this dye has a particularly low pH than the raw material dye itself.
It was found to show significant stability in the region.

酵素安定性 本色素にβ−グルコシダーゼ(スミチームAC)を83ユ
ニット/g色素を加え、50℃で2時間反応させた。反応前
および反応後のHPLCクロマトグラムをそれぞれ第3−a
図および第3−b図に示す。また原料のクロシンを主成
分とする黄色色素を同様にβ−グルコシダーゼ処理し、
反応前および反応後のHPLCクロマトグラムをそれぞれ第
3−c図および第3−d図に示す。このように、本色素
は上記酵素処理によってもクロシンおよびクロセチンに
分解されにくく、優れた酵素安定性を示す。Enzyme stability β-glucosidase (Sumizyme AC) was added to the present dye at 83 units / g, and reacted at 50 ° C for 2 hours. The HPLC chromatograms before and after the reaction were respectively expressed as 3-a
This is shown in the figure and FIG. 3-b. Similarly, a yellow pigment mainly containing crocin as a raw material is similarly treated with β-glucosidase,
The HPLC chromatograms before and after the reaction are shown in FIGS. 3-c and 3-d, respectively. As described above, the present dye is hardly decomposed into crocin and crocetin even by the above-mentioned enzyme treatment, and exhibits excellent enzyme stability.

実施例2 クチナシ黄色色素(色価▲E10W% 1cm▼=2000)0.01
g、乳糖0.5gを100mMリン酸緩衝液(pH7.2)10mに溶解
し、β−ガラクトシダーゼを0.75ユニット加え、50℃で
6時間反応させた。得られた本発明の色素類混合物は、
第4図のクロマトグラムで示される組成と、第5図の紫
外部および可視部の吸収スペクトルを示す。Example 2 Gardenia yellow pigment (color value ▲ E 10W% 1cm ▼ = 2000) 0.01
g and lactose (0.5 g) were dissolved in 10 mM 100 mM phosphate buffer (pH 7.2), and β-galactosidase (0.75 units) was added, followed by reaction at 50 ° C. for 6 hours. The obtained pigment mixture of the present invention is
4 shows the composition shown in the chromatogram in FIG. 4 and the absorption spectrum in the ultraviolet and visible regions in FIG.

色調の安定性 本色素を、pH3もしくは6のマックルベイン緩衝液中
で調製時及び12,000ルクス蛍光燈20時間照射後の吸光
度、100℃で1時間、37℃で4日、7日保持した後の吸
光度を第2表に示す。Color Tone Stability The absorbance of this dye at pH 3 or 6 in McClubane buffer at the time of preparation and after irradiation for 20 hours at 12,000 lux fluorescent lamp, after 1 hour at 100 ° C, 4 days at 37 ° C and 7 days The absorbance is shown in Table 2.

実施例3 クチナシ黄色色素(色価▲E10W% 1cm▼=2000)0.01
g、デキストリン0.5gを50mMリン酸緩衝液(pH6)10m
に溶解し、α−グルコシダーゼ10ユニットを加え、50℃
で2時間反応させた。得られた本発明の色素類混合物は
第6図のクロマトグラムで示される組成と、第7図の紫
外部および可視部の吸収スペクトルを示す。 Example 3 Gardenia yellow pigment (color value ▲ E 10W% 1cm ▼ = 2000) 0.01
g, dextrin 0.5g, 50mM phosphate buffer (pH6) 10m
And add 10 units of α-glucosidase,
For 2 hours. The obtained dye mixture of the present invention has the composition shown in the chromatogram in FIG. 6 and the absorption spectrum in the ultraviolet and visible regions in FIG.

色調の安定性 pH3もしくは6のマックルベイン緩衝液での調製時及
び12,000ルクス蛍光燈20時間照射後の吸光度、100℃で
1時間、37℃で4日、7日保持した後の吸光度を第3表
に示す。Color tone stability The absorbance after preparation with McClubane buffer of pH 3 or 6 and after irradiation with 12,000 lux fluorescent lamp for 20 hours, and after holding at 100 ° C for 1 hour, 37 ° C for 4 days and 7 days, were measured as the third values. It is shown in the table.

尚、本発明の安定化黄色系色素に対するクロマトグラ
ムは高圧液体クロマトグラフィー(HPLC)(山村化学研
究所製YMC ODS A−312、直径:0.6cm、長さ:15cm、溶媒:
50%メタノール、1m/分、検出:分光光度計、440n
m、レコーダー:島津製作所製CR−3A)にて分析した結
果を示した。 The chromatogram for the stabilized yellow dye of the present invention was obtained by high pressure liquid chromatography (HPLC) (YMC ODS A-312 manufactured by Yamamura Chemical Laboratory, diameter: 0.6 cm, length: 15 cm, solvent:
50% methanol, 1m / min, detection: spectrophotometer, 440n
m, Recorder: The results of analysis with a Shimadzu CR-3A) are shown.

実施例4 安定化黄色色素の精製−1 実施例1で得られた色素を吸着樹脂(ダイヤイオンHP
−20三菱化成製)に吸着させ、十分水洗した後、80%メ
タノール水溶液で色素を溶出させ濃縮凍結乾燥を行い1.
85gの安定化黄色色素粉末が得られた。Example 4 Purification of Stabilized Yellow Dye-1 The dye obtained in Example 1 was adsorbed on an adsorption resin (Diaion HP
-20 (manufactured by Mitsubishi Kasei), washed thoroughly with water, and then eluted the dye with an 80% methanol aqueous solution.
85 g of stabilized yellow pigment powder were obtained.

実施例5 安定化黄色色素の精製−2 実施例4で得られた安定化黄色色素粉末0.1gををゲル
濾過樹脂(セファデックスLH−20ファルマシア製)2.8c
mφ×140cmのカラムに負荷し50%アセトンで溶出させた
ところ190〜300mの間に糖修飾(縮合)色素が溶出し
た。そのクロマトグラムを第8図に示す。Example 5 Purification of stabilized yellow pigment-2 0.1 g of the stabilized yellow pigment powder obtained in Example 4 was subjected to gel filtration resin (Sephadex LH-20 Pharmacia) 2.8c.
When loaded onto a column of mφ × 140 cm and eluted with 50% acetone, the sugar-modified (condensed) dye eluted between 190 and 300 m. The chromatogram is shown in FIG.

実施例6 発酵法によるクロシンの糖修飾を以下の方法で行っ
た。即ち、バチルス・マセランス(Bacillus maceran
s)(IF03490)をクロシン0.1%、コーンスティープリ
カー1.0%、可溶性澱粉5.0%、硫酸アンモニウム0.5
%、炭酸カルシウム1.0%を含む液体培地で30℃、3日
間培養しクロシンを糖修飾した。培養3日目の培養液の
HLPCによるクロマトグラムを第9図に示す。Example 6 The sugar modification of crocin by the fermentation method was performed by the following method. That is, Bacillus maceran
s) (IF03490) crocin 0.1%, corn steep liquor 1.0%, soluble starch 5.0%, ammonium sulfate 0.5
% And calcium carbonate at 1.0%, and cultured at 30 ° C. for 3 days to modify crocin with sugar. On the 3rd day of culture
The chromatogram by HLPC is shown in FIG.

上記配合を用いて常法に従い中華麺を製造した。 Chinese noodles were produced according to a conventional method using the above blends.

(結果)クロシン配糖体含有の本実施例のものは色調、
香味、耐熱性、耐光性の面で比較例のものより優れてい
た。(Results) The color tone of this example containing crocin glycoside was
The flavor, heat resistance and light resistance were superior to those of the comparative example.

上記配合を用いて、常法に従いシロップ50Lを調製し
た。そのシロップ50mを炭酸水にて希釈し瓶詰充填し
全容200mとした。 Using the above composition, 50 L of syrup was prepared according to a conventional method. 50 m of the syrup was diluted with carbonated water and filled into a bottle to make a total volume of 200 m.

(結果)本実施例のものは比較例に比べ耐光性、耐熱
性、色調、香味の点で優れており褐変もみられなかっ
た。(Results) This example was superior to the comparative example in light resistance, heat resistance, color tone and flavor, and did not show browning.

〔発明の効果〕〔The invention's effect〕

以上の方法により製造された本発明の黄色系色素は上
記実施例1に示すとおり、前記従来技術の黄色系色素に
比べて、低いpHにおける熱、光安定性が良く、酵素によ
る加水分解に対する安定性も高い。したがって、酒類、
食品、飲料、化粧品、医薬品、麺類、かまぼこなどの加
工タンパク製品の着色剤としても優れている。As shown in Example 1 above, the yellow dye of the present invention produced by the above method has better heat and light stability at a low pH than the above-mentioned conventional yellow dye, and is more stable to hydrolysis by enzymes. The nature is also high. Therefore, liquor,
It is also excellent as a coloring agent for processed protein products such as foods, beverages, cosmetics, pharmaceuticals, noodles, and kamaboko.

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

第1−a図、第4図、第6図および第9図は、それぞれ
実施例1、同2、同3および同6で製造した色素混合物
のHPLCによるクロマトグラムであり、第1−b図は原料
クチナシ黄色色素の同様なクロマトグラムを表わし、 第2図、第5図および第7図は、それぞれ上記混合物の
紫外部および可視部における吸収スペクトルを表わし、 第3−a図は、実施例で得られた安定化色素のβ−グル
コシダーゼ処理前、第3−b図は同処理後、第3−c図
は原料色素の処理前、第3−d図は同処理後のHPLCクロ
マトグラムを表わし、そして 第8図は、実施例2の混合物をゲル濾過クロマト処理し
たクロマトグラムを表わす。 なお、第1−a図、第1−b図、第3図の各クロマトグ
ラム、第4図、第6図及び第9図のX軸の単位は、それ
ぞれ保持時間(分)を表わし、そして第2図、第5図及
び第7図のX軸の単位は、それぞれ波長(nm)を表わ
し、そしてY軸の単位は、それぞれ吸光度を表わす。FIG. 1-a, FIG. 4, FIG. 6 and FIG. 9 are chromatograms by HPLC of the dye mixtures produced in Examples 1, 2, 3 and 6, respectively, and FIG. 1-b. Represents the same chromatogram of the raw gardenia yellow pigment, FIGS. 2, 5 and 7 show the absorption spectra of the above mixture in the ultraviolet and visible parts, respectively. FIG. Before the β-glucosidase treatment of the stabilized dye obtained in the above, FIG. 3-b shows the HPLC chromatogram after the treatment, FIG. 3-c shows the HPLC chromatogram before the treatment of the raw material dye, and FIG. FIG. 8 shows a chromatogram of the mixture of Example 2 after gel filtration chromatography. The units on the X-axis in FIGS. 1-a, 1-b and 3 and the units on the X-axis in FIGS. 4, 6 and 9 respectively represent the retention time (minutes), and The units on the X-axis in FIGS. 2, 5 and 7 each represent wavelength (nm), and the units on the Y-axis each represent absorbance.

───────────────────────────────────────────────────── フロントページの続き (58)調査した分野(Int.Cl.6,DB名) C09B 61/00 C12P 19/18 A23L 1/275 ──────────────────────────────────────────────────続 き Continued on front page (58) Field surveyed (Int. Cl. 6 , DB name) C09B 61/00 C12P 19/18 A23L 1/275

Claims (4)

(57)【特許請求の範囲】(57) [Claims] 【請求項1】カロチノイド系色素の配糖体の水酸基に糖
質が縮合した新規カロチノイド系色素。1. A novel carotenoid pigment in which a saccharide is condensed with a hydroxyl group of a glycoside of a carotenoid pigment. 【請求項2】カロチノイド系色素の配糖体および糖質の
存在下で糖転移酵素を用いて転移反応を起こすことによ
り前記配糖体の水酸基に前記糖質を縮合させることを特
徴とする請求項1記載の色素の製造方法。2. The method according to claim 1, wherein the carbohydrate is condensed with a hydroxyl group of the glycoside by causing a transfer reaction using a glycosyltransferase in the presence of the carotenoid pigment glycoside and carbohydrate. Item 10. A method for producing the dye according to Item 1. 【請求項3】請求項1記載の色素を含んでなる食品。3. A food comprising the pigment according to claim 1. 【請求項4】請求項1記載の色素を含んでなる着色剤。4. A coloring agent comprising the coloring matter according to claim 1.
JP2275284A 1990-10-16 1990-10-16 Stabilized yellow dye Expired - Lifetime JP2993724B2 (en)

Priority Applications (1)

Application Number Priority Date Filing Date Title
JP2275284A JP2993724B2 (en) 1990-10-16 1990-10-16 Stabilized yellow dye

Applications Claiming Priority (1)

Application Number Priority Date Filing Date Title
JP2275284A JP2993724B2 (en) 1990-10-16 1990-10-16 Stabilized yellow dye

Publications (2)

Publication Number Publication Date
JPH04153271A JPH04153271A (en) 1992-05-26
JP2993724B2 true JP2993724B2 (en) 1999-12-27

Family

ID=17553282

Family Applications (1)

Application Number Title Priority Date Filing Date
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Country Status (1)

Country Link
JP (1) JP2993724B2 (en)

Families Citing this family (8)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
JPH05254483A (en) * 1992-03-12 1993-10-05 Koyo Eng Kk Method and device for preventing rolling of ship and off-shore floating structure
JPH06248193A (en) * 1993-02-25 1994-09-06 Ensuiko Sugar Refining Co Ltd Crocetin-containing pigment
ES2317786B1 (en) * 2007-07-31 2010-02-16 Consejo Superior De Investigaciones Cientificas ADDED OR SOLUBLE CAROTENOID MOLECULAR COMPLEX, PROCEDURE OF OBTAINING AND ITS APPLICATIONS.
CN102344692B (en) * 2011-08-10 2013-11-13 浙江工业大学 Method for extracting gardenia yellow pigment from gardeniae longicarpae fruit
CN102311660B (en) * 2011-09-14 2013-09-11 河南中大生物工程有限公司 Production method of gardenia yellow pigment
CN102936424B (en) * 2012-11-09 2014-10-08 苏州衷中医药科技有限公司 Method for preparing gardenia yellow pigment with high color value
CN106701640B (en) * 2017-02-17 2020-02-21 新疆农业科学院微生物应用研究所(中国新疆-亚美尼亚生物工程研究开发中心) New strain of natural yellow pigment producing strain XJ2, and preparation and application thereof
KR102025140B1 (en) * 2017-11-16 2019-09-25 대한민국(농촌진흥청장) Black rice flour improved in antioxidant activity and UVB decomposition stability and production method thereof

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