JP7037162B2 - VEGF gene expression promoter and FGF7 gene expression promoter - Google Patents
VEGF gene expression promoter and FGF7 gene expression promoter Download PDFInfo
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- JP7037162B2 JP7037162B2 JP2016228476A JP2016228476A JP7037162B2 JP 7037162 B2 JP7037162 B2 JP 7037162B2 JP 2016228476 A JP2016228476 A JP 2016228476A JP 2016228476 A JP2016228476 A JP 2016228476A JP 7037162 B2 JP7037162 B2 JP 7037162B2
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Description
本発明は、新規なVEGF遺伝子発現促進剤及びFGF7遺伝子発現促進剤に関するものである。 The present invention relates to a novel VEGF gene expression promoter and an FGF7 gene expression promoter.
毛髪は、成長期、退行期及び休止期からなる周期的なヘアサイクル(毛周期)に従って成長及び脱落を繰り返している。このヘアサイクルのうち、休止期から成長期にかけての新たな毛包が形成されるステージが、発毛に最も重要であると考えられており、このステージにおける毛包上皮系細胞の増殖・分化に重要な役割を果たしているのが、毛乳頭細胞であると考えられている。毛乳頭細胞は、毛根近傍にある外毛根鞘細胞とマトリックス細胞とからなる毛包上皮系細胞の内側にあって、基底膜に包まれている毛根の根幹部分に位置する細胞であり、毛包上皮系細胞に働きかけてその増殖を促進する等、毛包上皮系細胞の増殖・分化及び毛髪の形成において重要な役割を担っている(非特許文献1参照)。 Hair repeats growth and shedding according to a periodic hair cycle (hair cycle) consisting of a growth phase, a catagen phase, and a resting phase. Of this hair cycle, the stage where new hair follicles are formed from the resting phase to the growing phase is considered to be the most important for hair growth, and it is responsible for the proliferation and differentiation of hair follicle epithelial cells at this stage. It is believed that telogen cells play an important role. Hair follicle cells are cells located inside the hair follicle epithelial cells consisting of outer root sheath cells and matrix cells near the hair root, and are located in the root of the hair follicle surrounded by the basal membrane. It plays an important role in the proliferation and differentiation of hair follicle epithelial cells and the formation of hair, such as acting on epithelial cells to promote their proliferation (see Non-Patent Document 1).
このように、毛乳頭細胞は、毛包上皮系細胞の増殖・分化及び毛髪の形成において最も重要な役割を果たしており、従来、培養毛乳頭細胞に対象物質を接触させて、その細胞の増殖活性の有無及び/又は強弱を特定することで、その対象物質の育毛効果を検定する方法が提案されている(特許文献1参照)。 As described above, the hair papilla cells play the most important role in the proliferation and differentiation of hair follicle epithelial cells and the formation of hair. Conventionally, the cultured hair papilla cells are brought into contact with the target substance to carry out the proliferative activity of the cells. A method for testing the hair-growth effect of the target substance by specifying the presence / absence and / or the strength of the substance has been proposed (see Patent Document 1).
線維芽細胞増殖因子-7(FGF-7)は、線維芽細胞増殖因子(FGF)のファミリーのうちの1つであり、KGF(keratinocytegrowth factor)とも呼ばれる。FGFには、20種類以上のファミリーが存在することが知られている。FGFは、中胚葉と神経外胚葉から発生した幅広い細胞の増殖を促進する因子であり、例えば、線維芽細胞、血管内皮細胞、筋芽細胞、軟骨細胞、グリア細胞、骨芽細胞等の分裂・成長を誘導する。FGFは、血管新生作用、コラーゲンやフィブロネクチンの合成抑制作用等を有することや、ヘパリンに対して強い親和性を有することが知られている。 Fibroblast growth factor-7 (FGF-7) is one of the family of fibroblast growth factor (FGF) and is also called KGF (keratinoxytegrawth factor). It is known that there are more than 20 families of FGF. FGF is a factor that promotes the proliferation of a wide range of cells generated from the mesoderm and the neuroexternal embryo. For example, division of fibroblasts, vascular endothelial cells, myoblasts, chondrocytes, glia cells, osteoblasts, etc. Induces growth. It is known that FGF has an angiogenic action, an action of suppressing the synthesis of collagen and fibronectin, and has a strong affinity for heparin.
また、毛包の毛乳頭細胞において、FGF-7が発現していることが示され(例えば、非特許文献2参照)、FGF-7が毛根の活発化を介した育毛効果を有することが明らかになった。また、ノックアウトマウスを用いた研究により、FGF-7は、毛の伸びる方向に関与することが示唆されている。これまでに、FGF-7産生の促進作用を有する植物エキスとして、クララ等が知られている(非特許文献3参照)。
さらには歯周組織においてこれらの成長因子の産生を促進することにより、歯周組織の再生が可能になり、歯周組織再生促進剤として有効である。(特許文献2参照)
In addition, it was shown that FGF-7 was expressed in the dermal papilla cells of hair follicles (see, for example, Non-Patent Document 2), and it was clarified that FGF-7 has a hair growth effect through activation of hair roots. Became. In addition, studies using knockout mice suggest that FGF-7 is involved in the direction of hair growth. So far, Clara and the like have been known as plant extracts having an action of promoting FGF-7 production (see Non-Patent Document 3).
Furthermore, by promoting the production of these growth factors in the periodontal tissue, the periodontal tissue can be regenerated, which is effective as a periodontal tissue regeneration promoting agent. (See Patent Document 2)
一方、血管内皮増殖因子(VEGF、vascular endothelial growth factor)は、下垂体星状濾胞細胞の培養液より単離された、血管内皮細胞に特異的に作用する増殖因子である。そして、VEGFは、毛乳頭をはじめとして下垂体星状濾胞細胞、マクロファージ、平滑筋細胞、胚線維芽細胞等の多様な細胞に発現をしている。 On the other hand, vascular endothelial growth factor (VEGF) is a growth factor that acts specifically on vascular endothelial cells, isolated from the culture medium of pituitary stellate follicular cells. VEGF is expressed in various cells such as dermal papilla, pituitary stellate follicular cells, macrophages, smooth muscle cells, and germ fibroblasts.
VEGFの動きを阻害する特異抗体をマウス腹腔に注射すると、成長期が遅れるとともに毛包のサイズが小さくなり、毛包の発達や再生に血管新生が重要であることが報告されている。反対に、外毛根鞘でのVEGF合成量を増加させた場合、毛包のサイズが増大し、作られる毛の直径も太くなることが報告されている。更に、毛乳頭細胞から産生されるVEGFは発毛を促進することや、医薬品の育毛剤に用いられているミノキシジルの作用に関与すること等が知られている。 It has been reported that when a specific antibody that inhibits the movement of VEGF is injected into the abdominal cavity of a mouse, the growth phase is delayed and the size of the hair follicle is reduced, and angiogenesis is important for the development and regeneration of the hair follicle. On the contrary, it has been reported that when the amount of VEGF synthesized in the outer root sheath is increased, the size of the hair follicle is increased and the diameter of the hair produced is also increased. Further, it is known that VEGF produced from dermal papilla cells promotes hair growth and is involved in the action of minoxidil used as a hair restorer in pharmaceutical products.
以上のことから、脱毛や薄毛といった症状の予防・改善のために、優れたFGF7並びにVEGFの産生促進が誘導される発毛促進剤の開発が期待されており、これら作用を有する育毛剤に対する需要は極めて高い。
また、VEGFの産生促進は末梢動脈疾患の治療又は予防を行う。(特許文献3参照)
From the above, it is expected to develop a hair growth-promoting agent that induces the production promotion of excellent FGF7 and VEGF for the prevention and improvement of symptoms such as hair loss and thinning hair, and there is a demand for a hair-growth agent having these actions. Is extremely expensive.
In addition, promotion of VEGF production treats or prevents peripheral arterial diseases. (See Patent Document 3)
イシゲ(Ishige okamurae)は、主に潮間帯中部の岩上に生息し、本州太平洋側では茨城以南、日本海沿岸から南部、瀬戸内海、九州、朝鮮半島、中国と幅広く分布している。 Ishige okamurae mainly inhabits rocks in the central intertidal zone, and is widely distributed south of Ibaraki on the Pacific side of Honshu, from the coast of the Sea of Japan to the south, the Seto Inland Sea, Kyushu, the Korean Peninsula, and China.
イシゲには、デンドライト伸長抑制作用(特許文献4参照)や皮膚バリアの強化作用(特許文献5参照)が、見出されているがFGF7やVEGFを対象とした有効な発毛促進作用については知られていなかった。 Although dendrite elongation inhibitory action (see Patent Document 4) and skin barrier strengthening action (see Patent Document 5) have been found in Ishige, we are aware of the effective hair growth promoting action for FGF7 and VEGF. It wasn't done.
VEGF及びFGF7遺伝子の発現を促進し、発毛促進剤を得ること、さらには歯周組織再生促進剤や末梢動脈疾患の治療又は予防に有効な製剤を得ることを目的とする。 It is an object of the present invention to promote the expression of VEGF and FGF7 genes, to obtain a hair growth-promoting agent, and to obtain a periodontal tissue regeneration-promoting agent and a preparation effective for the treatment or prevention of peripheral arterial diseases.
このような背景の下、鋭意検討した結果、イシゲ抽出物において有効なFGF7遺伝子の発現を促進する作用を見出し、本発明を完成させた。
イシゲの抽出効率を考え、細切、乾燥、粉砕等の処理を行った後に抽出を行うことが好ましい。乾燥は天日で行ってもよいし、通常使用される乾燥機を用いて行ってもよい。前記抽出に用いる溶媒としては、水若しくは親水性有機溶媒又はこれらの混合液を用いる。
前記抽出溶媒として使用し得る水としては、例えば、純水、水道水、井戸水、鉱泉水、鉱水、温泉水、湧水、淡水等の他、これらに各種処理を施したものが含まれる。水に施す処理としては、例えば、精製、加熱、殺菌、ろ過、イオン交換、浸透圧の調整、緩衝化等が含まれる。従って、本発明において抽出溶媒として使用し得る水には、精製水、熱水、イオン交換水、生理食塩水、リン酸緩衝液、リン酸緩衝生理食塩水等も含まれる。
前記親水性有機溶媒としては、例えば、メタノール、エタノール、プロピルアルコール、イソプロピルアルコール等の炭素数1~5の低級アルコール;アセトン、メチルエチルケトン等の低級脂肪族ケトン;1,3-ブチレングリコール、プロピレングリコール、グリセリン等の炭素数2~5の多価アルコールなどが挙げられ、これら親水性有機溶媒と水との混合溶媒などを用いることができる。
なお、前記水と親水性有機溶媒との混合溶媒を使用する場合には、低級アルコールの場合は水10質量部に対して1~20質量部、低級脂肪族ケトンの場合は水10質量部に対して1~15質量部添加することが好ましい。多価アルコールの場合は水10質量部に対して1~20質量部添加することが好ましい。
抽出に使用する有機溶媒の量は、原料となる植物(海藻)に対して望ましくは5~100倍量程度、さらに望ましくは10~50倍量程度が良い。さらに抽出効率を上げるため、抽出溶媒中で撹拌やホモジナイズしてもよい。抽出温度としては、5℃程度から抽出溶媒の沸点以下の温度とするのが適切である。抽出時間は抽出溶媒の種類や抽出温度によっても異なるが、1時間~14日間程度とするのが適切である。
尚、抽出操作は1回のみの操作に限定されるものではない。抽出後の残渣に再度新鮮な溶媒を添加し、抽出操作を施すこともできるし、抽出溶媒を複数回抽出原料に接触させることも可能である。必要ならば、その効果に影響のない範囲で更に脱臭、脱色等の精製処理を加えても良く、エバポレーターのような減圧濃縮装置や加熱による溶媒除去などにより、濃縮することができる。また、この抽出物を合成吸着剤(ダイアイオンHP20やセファビースSP825、アンバーライトXAD4、MCIgelCHP20P等)やデキストラン樹脂(セファデックスLH-20など)、限外濾過等を用いてさらに精製することも可能である。
Against this background, as a result of diligent studies, we have found an action that promotes the expression of an effective FGF7 gene in the Ishige extract, and completed the present invention.
Considering the extraction efficiency of Ishige, it is preferable to perform extraction after performing treatments such as shredding, drying and crushing. Drying may be carried out in the sun or by using a commonly used dryer. As the solvent used for the extraction, water, a hydrophilic organic solvent, or a mixed solution thereof is used.
The water that can be used as the extraction solvent includes, for example, pure water, tap water, well water, mineral spring water, mineral water, hot spring water, spring water, fresh water, and the like, as well as those subjected to various treatments. Treatments applied to water include, for example, purification, heating, sterilization, filtration, ion exchange, osmotic pressure adjustment, buffering and the like. Therefore, the water that can be used as the extraction solvent in the present invention includes purified water, hot water, ion-exchanged water, physiological saline, phosphate buffer, phosphate buffered saline and the like.
Examples of the hydrophilic organic solvent include lower alcohols having 1 to 5 carbon atoms such as methanol, ethanol, propyl alcohol and isopropyl alcohol; lower aliphatic ketones such as acetone and methyl ethyl ketone; 1,3-butylene glycol and propylene glycol. Examples thereof include polyhydric alcohols having 2 to 5 carbon atoms such as glycerin, and a mixed solvent of these hydrophilic organic solvents and water can be used.
When a mixed solvent of the water and a hydrophilic organic solvent is used, the amount of lower alcohol is 1 to 20 parts by mass with respect to 10 parts by mass of water, and the amount of lower aliphatic ketone is 10 parts by mass of water. On the other hand, it is preferable to add 1 to 15 parts by mass. In the case of polyhydric alcohol, it is preferable to add 1 to 20 parts by mass with respect to 10 parts by mass of water.
The amount of the organic solvent used for extraction is preferably about 5 to 100 times, more preferably about 10 to 50 times the amount of the plant (seaweed) as a raw material. In order to further increase the extraction efficiency, stirring or homogenization may be performed in the extraction solvent. It is appropriate that the extraction temperature is from about 5 ° C. to a temperature equal to or lower than the boiling point of the extraction solvent. The extraction time varies depending on the type of extraction solvent and the extraction temperature, but it is appropriate to set it to about 1 hour to 14 days.
The extraction operation is not limited to a one-time operation. A fresh solvent can be added again to the residue after extraction to perform an extraction operation, or the extraction solvent can be brought into contact with the extraction raw material multiple times. If necessary, further purification treatment such as deodorization and decolorization may be added within a range that does not affect the effect, and the concentration can be achieved by a vacuum concentrating device such as an evaporator or solvent removal by heating. Further, this extract can be further purified using a synthetic adsorbent (Diaion HP20, Sephadex SP825, Amberlite XAD4, MCIgelCHP20P, etc.), dextran resin (Sephadex LH-20, etc.), ultrafiltration, etc. be.
本発明の製剤は、経口、注射、外用のいずれでも薬効を発現するが、皮膚外用剤として用いるのが好ましい。皮膚外用剤には、皮膚化粧料、外用医薬部外品、医療用皮膚外用剤が含まれる。 Although the pharmaceutical product of the present invention exerts a medicinal effect by oral, injectable or external use, it is preferably used as a skin external preparation. External skin preparations include skin cosmetics, quasi-drugs for external use, and external external preparations for medical use.
また、本発明の製剤には、上記成分の他に医薬品や化粧品の各種製剤において使用されている界面活性剤、油性成分、保湿剤、高分子化合物、紫外線吸収剤、抗炎症剤、殺菌剤、酸化防止剤、金属イオン封鎖剤、防腐剤、ビタミン類、色素、香料、水等を配合することができる。 In addition to the above-mentioned ingredients, the formulations of the present invention include surfactants, oily ingredients, moisturizers, polymer compounds, ultraviolet absorbers, anti-inflammatory agents, and bactericidal agents used in various pharmaceutical and cosmetic formulations. Antioxidants, metal ion blockers, preservatives, vitamins, pigments, fragrances, water and the like can be blended.
上記界面活性剤としては、アニオン性、カチオン性、非イオン性、天然、合成のいずれの界面活性剤も使用できるが、皮膚に対する刺激性を考慮すると非イオン性のものを使用することが好ましい。非イオン性界面活性剤としては、例えばグリセリン脂肪酸エステル、プロピレングリコール脂肪酸エステル、ソルビタン脂肪酸エステル、ポリオキシエチレンソルビタン脂肪酸エステル、ポリオキシエチレンソルビット脂肪酸エステル、ポリオキシエチレンアルキルエーテル、ポリオキシエチレンポリオキシプロピレングリコール、ポリオキシエチレンポリオキシプロピレンアルキルエーテル、ポリエチレングリコール脂肪酸エステル、ポリオキシエチレンヒマシ油、ポリオキシエチレン硬化ヒマシ油、アルキルグリコシド等が挙げられる。 As the above-mentioned surfactant, any of anionic, cationic, nonionic, natural and synthetic surfactants can be used, but it is preferable to use nonionic surfactants in consideration of skin irritation. Examples of the nonionic surfactant include glycerin fatty acid ester, propylene glycol fatty acid ester, sorbitan fatty acid ester, polyoxyethylene sorbitan fatty acid ester, polyoxyethylene sorbit fatty acid ester, polyoxyethylene alkyl ether, and polyoxyethylene polyoxypropylene glycol. , Polyoxyethylene polyoxypropylene alkyl ether, polyethylene glycol fatty acid ester, polyoxyethylene castor oil, polyoxyethylene hydrogenated castor oil, alkyl glycoside and the like.
油性成分としては、油脂類、ロウ類、炭化水素類、高級脂肪酸類、高級アルコール類、エステル類、精油類、シリコーン油類などを挙げることができる。油脂類としては、例えば大豆油、ヌカ油、ホホバ油、アボガド油、アーモンド油、オリーブ油、カカオ油、ゴマ油、パーシック油、ヒマシ油、ヤシ油、ミンク油、牛脂、豚脂等の天然油脂、これらの天然油脂を水素添加して得られる硬化油及びミリスチン酸グリセリド、2-エチルヘキサン酸トリグリセリド等の合成トリグリセリド等が;ロウ類としては、例えばカルナバロウ、鯨ロウ、ミツロウ、ラノリン等が;炭化水素類としては、例えば流動パラフィン、ワセリン、パラフィンマイクロクリスタリンワックス、セレシン、スクワラン、ブリスタン等が;高級脂肪酸類としては、例えばラウリン酸、ミリスチン酸、パルミチン酸、ステアリン酸、ベヘニン酸、オレイン酸、リノール酸、リノレン酸、ラノリン酸、イソステアリン酸等が;高級アルコール類としては、例えばラウリルアルコール、セチルアルコール、ステアリルアルコール、オレイルアルコール、ラノリンアルコール、コレステロール、2-ヘキシルデカノール等が;エステル類としては、例えばオクタン酸セチル、オクタン酸トリグリセライド、乳酸ミリスチル、乳酸セチル、ミリスチン酸イソプロピル、ミリスチン酸ミリスチル、ミリスチン酸オクチルドデシル、パルミチン酸イソプロピル、アジピン酸イソプロピル、ステアリン酸ブチル、オレイン酸デシル、イソステアリン酸コレステロール、POEソルビット脂肪酸エステル等が;精油類としては、例えばハッカ油、ジャスミン油、ショウ脳油、ヒノキ油、トウヒ油、リュウ油、テレピン油、ケイ皮油、ベルガモット油、ミカン油、ショウブ油、パイン油、ラベンダー油、ベイ油、クローブ油、ヒバ油、バラ油、ユーカリ油、レモン油、タイム油、ペパーミント油、ローズ油、セージ油、メントール、シネオール、オイゲノール、シトラール、シトロネラール、ボルネオール、リナロール、ゲラニオール、カンファー、チモール、スピラントール、ピネン、リモネン、テルペン系化合物等が;シリコーン油類としては、例えばジメチルポリシロキサン等が挙げられる。これら上述の油性成分は一種又は二種以上を組み合わせて使用することができる。
本発明においては、このうち特にミリスチン酸グリセリド、2-エチルヘキサン酸トリグリセリド、ラノリン、流動パラフィン、ワセリン、パラフィンマイクロクリスタリンワックス、スクワラン、ラウリン酸、ミリスチン酸、パルミチン酸、リノール酸、リノレン酸、イソステアリン酸、セチルアルコール、ステアリルアルコール、オレイルアルコール、コレステロール、オクタン酸セチル、オクタン酸トリグリセライド、ミリスチレン酸イソプロピル、ミリスチン酸オクチルドデシル、イソステアリン酸コレステロール、POEソルビット脂肪酸エステル、ハッカ油、トウヒ油、ケイ皮油、ローズ油、メントール、シネオール、オイゲノール、シトラール、シトロネラール、ゲラニオール、ピネン、リモネン、ジメチルポリシロキサンを使用することが好ましい。
Examples of the oily component include fats and oils, waxes, hydrocarbons, higher fatty acids, higher alcohols, esters, essential oils, silicone oils and the like. Examples of oils and fats include soybean oil, nuka oil, jojoba oil, avocado oil, almond oil, olive oil, cacao oil, sesame oil, persic oil, castor oil, palm oil, minced oil, beef oil, pork oil and other natural oils and fats. Hardened oil obtained by hydrogenating natural fats and oils from Japan and synthetic triglycerides such as myristic acid glyceride and 2-ethylhexanoic acid triglyceride; Examples of waxes include carnauba wax, whale wax, beeswax, lanolin and the like; hydrocarbons. Examples include liquid paraffin, vaseline, paraffin microcrystalin wax, selecin, squalane, bristan, etc .; and higher fatty acids include, for example, lauric acid, myristic acid, palmitic acid, stearic acid, behenic acid, oleic acid, linoleic acid, etc. Linolenic acid, lanolinic acid, isostearic acid and the like; higher alcohols include, for example, lauryl alcohol, cetyl alcohol, stearyl alcohol, oleyl alcohol, lanolin alcohol, cholesterol, 2-hexyldecanol and the like; esters include, for example, cetyl octanate. , Octanoic acid triglyceride, myristyl lactate, cetyl lactate, isopropyl myristate, myristyl myristate, octyldodecyl myristate, isopropyl palmitate, isopropyl adipate, butyl stearate, decyl oleate, cholesterol isostearate, POE sorbit fatty acid ester, etc. The essential oils include, for example, peppermint oil, jasmine oil, show brain oil, hinoki oil, peppermint oil, ryu oil, terepine oil, calyx skin oil, bergamot oil, orange oil, shove oil, pine oil, lavender oil, and bay oil. , Clove oil, hiba oil, rose oil, eucalyptus oil, lemon oil, thyme oil, peppermint oil, rose oil, sage oil, menthol, cineole, eugenol, citral, citroneral, borneol, linalol, geraniol, camphor, timole, spirantol, Pinen, limonene, terpene-based compounds and the like; Examples of silicone oils include dimethylpolysiloxane and the like. These above-mentioned oily components can be used alone or in combination of two or more.
In the present invention, among these, myristic acid glyceride, 2-ethylhexanoic acid triglyceride, lanolin, liquid paraffin, vaseline, paraffin microcrystalin wax, squalane, lauric acid, myristic acid, palmitic acid, linoleic acid, linolenic acid, isostearic acid. , Cetyl alcohol, stearyl alcohol, oleyl alcohol, cholesterol, cetyl octanoate, triglyceride octanoate, isopropyl myristyrene, octyldodecyl myristate, cholesterol isostearate, POE sorbit fatty acid ester, peppermint oil, peppermint oil, calyx oil, rose It is preferable to use oil, menthol, cineol, eugenol, citral, citronellal, geraniol, pinen, limonene and dimethylpolysiloxane.
本発明の製剤には、さらに下記のような成分を配合することができるが、その成分もこれらに限定されるものではない。色素類;黄色4号、青色1号、黄色202号等の厚生省令に定められたタール色素別表I及びIIの色素、クロロフィル、リボフラビン、クロシン、紅花、アントラキノン等の食品添加物として認められている天然色素等。
ビタミン類;ビタミンA、ビタミンC、ビタミンD、ビタミンE等。その他;殺菌剤、防腐剤、その他製剤上必要な成分等。
The following components can be further added to the pharmaceutical product of the present invention, but the components are not limited thereto. Pigments; Tar dyes specified in the Ordinance of the Ministry of Health and Welfare such as Yellow No. 4, Blue No. 1, Yellow No. 202, etc. Approved as food additives such as pigments in Appendix I and II, chlorophyll, riboflavin, crocin, safflower, anthraquinone, etc. Natural pigments, etc.
Vitamins; Vitamin A, Vitamin C, Vitamin D, Vitamin E, etc. Others; bactericides, preservatives, other ingredients necessary for formulation, etc.
本発明の製剤は、前記必須成分に必要に応じて前記任意成分を加え、常法に従って製造することができ、クリーム、乳液、化粧水等の形態とすることができる。 The pharmaceutical product of the present invention can be produced according to a conventional method by adding the optional ingredient to the essential ingredient as necessary, and can be in the form of cream, milky lotion, lotion or the like.
次に実施例を挙げて本発明を詳細に説明する。 Next, the present invention will be described in detail with reference to examples.
実施例1
イシゲ50g(湿重量)に精製水500gを加え、ミキサーを用いてホモジナイズした。これを遠心分離し濾液を得た。この濾液に4倍量のエタノール2Lを加え、ときどき撹拌しながら、24時間後に濾過(No5C)し、これを凍結乾燥した。
Example 1
500 g of purified water was added to 50 g of Ishige (wet weight), and homogenized using a mixer. This was centrifuged to obtain a filtrate. 4 times the amount of ethanol was added to this filtrate, and the mixture was filtered (No5C) after 24 hours with occasional stirring, and this was lyophilized.
確認試験(FGF7およびVEGF遺伝子発現促進試験)
ヒト毛乳頭細胞(PromoCell)を6ウェルプレートに播種し、3日間培養した。3日後に、FBSを含まないDMEM培地へ、実施例にて製造したイシゲ抽出物を1mg/mLに調整したものを、先のヒト毛乳頭細胞へ添加し2時間培養した。培養後、以下の方法に従い、RNAを抽出しRT反応後、リアルタイムPCRを実施した。
Confirmation test (FGF7 and VEGF gene expression promotion test)
Human dermal papilla cells (PromoCell) were seeded on 6-well plates and cultured for 3 days. Three days later, the Ishige extract prepared in the example was adjusted to 1 mg / mL in DMEM medium containing no FBS, added to the above-mentioned human dermal papilla cells, and cultured for 2 hours. After culturing, RNA was extracted according to the following method, and after RT reaction, real-time PCR was performed.
RNAの抽出
細胞からのTotal RNAの抽出は、PureLink(登録商標)RNA Mini Kit(ライフテクノロジーズ・ジャパン)を用い、添付マニュアルに従い調整した。RNA濃度は、NanoDop1000(Thermo Fisher scientific)を用いて算出した。
Extraction of RNA Extraction of Total RNA from cells was adjusted using PureLink® RNA Mini Kit (Life Technologies Japan) according to the attached manual. RNA concentration was calculated using NanoDop1000 (Thermo Fisher scientific).
RT反応およびリアルタイムPCR
抽出したTotal RNAを使い、High-Capacity RNA-to-cDNA Kit(ライフテクノロジーズ・ジャパン)を用いて、添付マニュアルに従いRT反応を行った。
リアルタイムPCRは、7500 Real-Time PCR System(ライフテクノロジーズ・ジャパン)を用いて実施した。
詳細には、前述のRT産物と、VEGF、FGF7および内在性コントロールとしてGAPDHのTaqMan(登録商標) プライマー(ライフテクノロジーズ・ジャパン)、TaqMan(登録商標) Gene Expression Master Mix(ライフテクノロジーズ・ジャパン)を用いて、ΔΔCT法により遺伝子発現量の比較を行った。
RT reaction and real-time PCR
Using the extracted Total RNA, RT reaction was performed according to the attached manual using High-Capacity RNA-to- cDNA Kit (Life Technologies Japan).
Real-time PCR was performed using the 7500 Real-Time PCR System (Life Technologies Japan).
Specifically, the above-mentioned RT products and TaqMan (registered trademark) primer (Life Technologies Japan) and TaqMan (registered trademark) Gene Expression Master Mix (Life Technologies Japan) of GAPDH as VEGF, FGF7 and endogenous control are used. Then, the gene expression levels were compared by the ΔΔCT method.
結果を図1に示す。 The results are shown in FIG.
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Biomol Ther., 2012, Vol.20 No.6, p.520-525 |
生化学, 2009, Vol.81 No.7, p.592-597 |
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