KR100435829B1 - METHOD FOR PRODUCING IgY AGAINST SUCRASE AND MALTASE AND COMPOSITIONS CONTAINING SAME FOR INHIBITING CARBOHYDRATE UPTAKE - Google Patents
METHOD FOR PRODUCING IgY AGAINST SUCRASE AND MALTASE AND COMPOSITIONS CONTAINING SAME FOR INHIBITING CARBOHYDRATE UPTAKE Download PDFInfo
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- KR100435829B1 KR100435829B1 KR10-2001-0059027A KR20010059027A KR100435829B1 KR 100435829 B1 KR100435829 B1 KR 100435829B1 KR 20010059027 A KR20010059027 A KR 20010059027A KR 100435829 B1 KR100435829 B1 KR 100435829B1
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- Prior art keywords
- maltase
- yolk
- sucrase
- yolk antibody
- present
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Classifications
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- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07K—PEPTIDES
- C07K16/00—Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies
- C07K16/02—Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies from eggs
-
- A—HUMAN NECESSITIES
- A23—FOODS OR FOODSTUFFS; TREATMENT THEREOF, NOT COVERED BY OTHER CLASSES
- A23L—FOODS, FOODSTUFFS, OR NON-ALCOHOLIC BEVERAGES, NOT COVERED BY SUBCLASSES A21D OR A23B-A23J; THEIR PREPARATION OR TREATMENT, e.g. COOKING, MODIFICATION OF NUTRITIVE QUALITIES, PHYSICAL TREATMENT; PRESERVATION OF FOODS OR FOODSTUFFS, IN GENERAL
- A23L2/00—Non-alcoholic beverages; Dry compositions or concentrates therefor; Their preparation
- A23L2/52—Adding ingredients
- A23L2/66—Proteins
-
- A—HUMAN NECESSITIES
- A23—FOODS OR FOODSTUFFS; TREATMENT THEREOF, NOT COVERED BY OTHER CLASSES
- A23L—FOODS, FOODSTUFFS, OR NON-ALCOHOLIC BEVERAGES, NOT COVERED BY SUBCLASSES A21D OR A23B-A23J; THEIR PREPARATION OR TREATMENT, e.g. COOKING, MODIFICATION OF NUTRITIVE QUALITIES, PHYSICAL TREATMENT; PRESERVATION OF FOODS OR FOODSTUFFS, IN GENERAL
- A23L33/00—Modifying nutritive qualities of foods; Dietetic products; Preparation or treatment thereof
- A23L33/10—Modifying nutritive qualities of foods; Dietetic products; Preparation or treatment thereof using additives
- A23L33/17—Amino acids, peptides or proteins
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- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K39/00—Medicinal preparations containing antigens or antibodies
- A61K39/395—Antibodies; Immunoglobulins; Immune serum, e.g. antilymphocytic serum
- A61K39/39533—Antibodies; Immunoglobulins; Immune serum, e.g. antilymphocytic serum against materials from animals
- A61K39/3955—Antibodies; Immunoglobulins; Immune serum, e.g. antilymphocytic serum against materials from animals against proteinaceous materials, e.g. enzymes, hormones, lymphokines
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- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P3/00—Drugs for disorders of the metabolism
- A61P3/04—Anorexiants; Antiobesity agents
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- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P3/00—Drugs for disorders of the metabolism
- A61P3/08—Drugs for disorders of the metabolism for glucose homeostasis
- A61P3/10—Drugs for disorders of the metabolism for glucose homeostasis for hyperglycaemia, e.g. antidiabetics
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- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07K—PEPTIDES
- C07K16/00—Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies
- C07K16/40—Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies against enzymes
-
- A—HUMAN NECESSITIES
- A23—FOODS OR FOODSTUFFS; TREATMENT THEREOF, NOT COVERED BY OTHER CLASSES
- A23V—INDEXING SCHEME RELATING TO FOODS, FOODSTUFFS OR NON-ALCOHOLIC BEVERAGES AND LACTIC OR PROPIONIC ACID BACTERIA USED IN FOODSTUFFS OR FOOD PREPARATION
- A23V2002/00—Food compositions, function of food ingredients or processes for food or foodstuffs
-
- A—HUMAN NECESSITIES
- A23—FOODS OR FOODSTUFFS; TREATMENT THEREOF, NOT COVERED BY OTHER CLASSES
- A23V—INDEXING SCHEME RELATING TO FOODS, FOODSTUFFS OR NON-ALCOHOLIC BEVERAGES AND LACTIC OR PROPIONIC ACID BACTERIA USED IN FOODSTUFFS OR FOOD PREPARATION
- A23V2200/00—Function of food ingredients
- A23V2200/30—Foods, ingredients or supplements having a functional effect on health
- A23V2200/332—Promoters of weight control and weight loss
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- A—HUMAN NECESSITIES
- A23—FOODS OR FOODSTUFFS; TREATMENT THEREOF, NOT COVERED BY OTHER CLASSES
- A23V—INDEXING SCHEME RELATING TO FOODS, FOODSTUFFS OR NON-ALCOHOLIC BEVERAGES AND LACTIC OR PROPIONIC ACID BACTERIA USED IN FOODSTUFFS OR FOOD PREPARATION
- A23V2250/00—Food ingredients
- A23V2250/54—Proteins
- A23V2250/542—Animal Protein
- A23V2250/5434—Immunoglobulines
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- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07K—PEPTIDES
- C07K2317/00—Immunoglobulins specific features
- C07K2317/10—Immunoglobulins specific features characterized by their source of isolation or production
- C07K2317/11—Immunoglobulins specific features characterized by their source of isolation or production isolated from eggs
Abstract
본 발명은 수크라아제와 말타아제에 대한 난황항체의 생산방법 및 이를 이용한 식이 탄수화물의 흡수 억제용 조성물에 관한 것으로, 구체적으로 돼지 소장 유래의 탄수화물 분해 효소인 수크라아제와 말타아제를 분리하는 단계; 상기 수크라아제와 말타아제를 항원으로 사용하여 산란계에 면역시켜 난황항체를 생산하는 단계; 및 상기 산란계가 낳은 달걀의 난황으로부터 난황항체를 분리하는 단계를 포함하는, 수크라아제와 말타아제에 대한 난황항체의 생산방법 및 상기 방법에 의해 생산된 난황항체를 이용하여 생체 내 탄수화물 분해효소인 수크라아제와 말타아제의 활성을 저해하는 식이 탄수화물의 흡수 억제용 조성물에 관한 것이다. 본 발명의 난황항체는 소장 내에서 탄수화물의 분해를 직접적으로 억제하므로 음식물 섭취의 제한 없이 비만 개선을 위한 다이어트 원료나 당뇨병의 예방 및 치료에 유용하게 사용될 수 있다.The present invention relates to a method for producing yolk antibodies against sucrase and maltase, and to a composition for inhibiting absorption of dietary carbohydrates using the same, specifically, separating sucrase and maltase, which are carbohydrate degrading enzymes derived from swine intestine; Producing yolk antibodies by immunizing the laying hens using the sucrase and maltase as antigens; And separating the yolk antibody from the yolk of the egg laid by the laying hen, the method of producing yolk antibodies against sucrase and maltase and the in vivo carbohydrate degrading enzyme using the yolk antibody produced by the above method. The present invention relates to a composition for inhibiting absorption of dietary carbohydrates that inhibits the activity of kraase and maltase. Since the yolk antibody of the present invention directly inhibits the decomposition of carbohydrates in the small intestine, it can be usefully used for the prevention and treatment of dietary ingredients or diabetes for improving obesity without limiting food intake.
Description
본 발명은 수크라아제와 말타아제에 대한 난황항체의 생산방법 및 이를 이용한 식이 탄수화물의 흡수 억제용 조성물에 관한 것으로, 구체적으로 돼지 소장 유래의 탄수화물 분해 효소인 수크라아제와 말타아제를 분리하는 단계; 상기 수크라아제와 말타아제를 항원으로 사용하여 산란계에 면역시켜 난황항체를 생산하는 단계; 및 상기 산란계가 낳은 달걀의 난황으로부터 난황항체를 분리하는 단계를 포함하는, 수크라아제와 말타아제에 대한 난황항체의 생산방법 및 상기 방법에 의해 생산된 난황항체를 이용하여 생체 내 탄수화물 분해효소인 수크라아제와 말타아제의 활성을 저해하는 식이 탄수화물의 흡수 억제용 조성물에 관한 것이다.The present invention relates to a method for producing yolk antibodies against sucrase and maltase, and to a composition for inhibiting absorption of dietary carbohydrates using the same, specifically, separating sucrase and maltase, which are carbohydrate degrading enzymes derived from swine intestine; Producing yolk antibodies by immunizing the laying hens using the sucrase and maltase as antigens; And separating the yolk antibody from the yolk of the egg laid by the laying hen, the method of producing yolk antibodies against sucrase and maltase and the in vivo carbohydrate degrading enzyme using the yolk antibody produced by the above method. The present invention relates to a composition for inhibiting absorption of dietary carbohydrates that inhibits the activity of kraase and maltase.
일반적으로 섭취한 음식물의 생체 내 소화는 구강 내에서 탄수화물의 초기 분해를 비롯하여 위장에서 일부 단백질의 분해가 일어난다. 그러나, 본격적인 탄수화물 및 지방의 소화, 흡수는 십이지장에서부터 회장부에 이르는 부위에서 주로 일어나며 일반적으로 대장에서는 주로 수분과 염류 등의 재흡수와 유리지방산의 흡수가 일어나는 것으로 알려져 있다. 따라서, 소화 흡수의 가장 중요한 부분이 바로 소장에서 일어나는데 이때 췌장에서 분비되는 트립시노겐, 키모트립시노겐, 카르복시 펩티다아제 등의 단백질 분해 효소, 췌장 리파아제, 스팁신 등의 지질 분해 효소, 췌장 아밀라아제, 아밀롭신, 말타아제 등의 탄수화물 분해 효소 및 소장액에 존재하는 다양한 펩티다아제, 핵산 분해효소, 알기나아제, 포스파타제, 각종 당질 분해효소인 유당 분해 효소 등 여러 가지 소화 효소에 의해서 식괴가 분해되고 소장 표면에 있는 융모세포에서 흡수되어 암죽관과 혈관을 통해서 흡수된 영양분이 체내로 이동하게 된다.In vivo digestion of ingested food usually results in the breakdown of some proteins in the stomach, including the initial breakdown of carbohydrates in the oral cavity. However, full-fledged carbohydrate and fat digestion and absorption occur mainly in the area from the duodenum to the ileum, and in general, it is known that resorption of water and salts and absorption of free fatty acids occur mainly in the large intestine. Therefore, the most important part of digestive absorption occurs in the small intestine, where proteolytic enzymes such as trypsinogen, chymotrypsinogen, and carboxy peptidase, lipolytic enzymes such as pancreatic lipase and sphyxin, pancreatic amylase, amylosin Carbohydrate degrading enzymes such as, maltase and various digestive enzymes such as various peptidase, nucleic acid degrading enzyme, alginase, phosphatase, and lactose degrading enzyme which are various glycolytic enzymes in the small intestine Absorbed by the nutrients absorbed through the dark ducts and blood vessels will be moved into the body.
이러한 융모세포에서의 탄수화물 및 지방 흡수에 가장 중요한 역할을 하는 것이 바로 융모세포 막수송체이다. 융모세포 막수송체는 소장 융모세포의 표면에 존재하는 막수송체 (membrane vesicle)이며 상기 수송체는 SGLT1 (sodium dependent glucose cotransporter 1)이라고 하는 Na 양이온에 의한 단당류의 수송에 매우 중요한 역할을 한다. 즉, 막수송체는 탄수화물의 분해에 의해서 생긴 단당류 중 가장 대표적인 단당류의 체내 능동 수송에 매우 중요한 역할을 담당한다. 또한, 이러한 단당류의 수송에 필수 불가결한 중요한 이당류 분해효소인 수크라아제와 말타아제 및 글루코아밀라아제의 활성이 융모세포 막수송체에서 매우 높게 나타나는데 이러한 효소에 의해서 단당류의 체내 흡수가 증대되는 것으로 알려져 있다. 그러나, 장관내의 이당류 분해효소에 의한 가수분해는 회장 상부에 이르는 동안에는 별로 이루어지지 않는데, 이것은 이른바 융모세포 막수송체가 가지는 탄수화물 분해효소가 작용하는 막소화에 의존하는 바가 크다는 것을 의미한다. 실제로, 수크라아제와 말타아제의 활성이 많이 발견되는 회장부에 이르기 전까지는 단당류의 흡수가 전체 단당류 흡수량에 비해 상대적으로 낮다는 것이 이를 증명한다고 할 수 있다.The most important role in carbohydrate and fat absorption in these chorionic cells is the chorionic cell membrane transporter. The chorionic membrane transporter is a membrane transporter (membrane vesicle) present on the surface of the small intestinal chollocytes and the transporter plays a very important role in the transport of monosaccharides by Na cations called sodium dependent glucose cotransporter 1 (SGLT1). That is, the membrane transporter plays a very important role in the active transport of the most representative monosaccharides of the monosaccharides caused by the decomposition of carbohydrates. In addition, the activity of sucrase, maltase, and glucoamylase, which are important disaccharide degrading enzymes essential for the transport of such monosaccharides, is very high in the chorionic membrane transporter, which is known to increase monosaccharide absorption in the body. However, hydrolysis by disaccharide degrading enzymes in the intestinal tract is rarely performed during the upper ileum, which means that the carbohydrate degrading enzymes of the chorionic cell membrane transporter are largely dependent on membrane thinning. Indeed, it can be proved that the absorption of monosaccharides is relatively low compared to the total monosaccharide absorption until it reaches the ileal region where sucrase and maltase activities are found.
따라서, 탄수화물의 섭취량이 가장 많은 한국인의 식생활 패턴을 고려한다면, 전체 영양소의 섭취를 제한하는 기존의 비만 및 당뇨에 사용되는 식이요법이나 식이섬유를 이용한 장 청소효과 및 지방의 소화 흡수 억제를 주된 기작으로 하는 다이어트 제품은 적합하지 못하므로, 다른 필수적인 무기이온 및 단백질 등의 흡수저해 없이 탄수화물의 흡수만을 저해할 수 있는 한국인에게 적합한 차별화된 방법의 개발이 요구되고 있다.Therefore, considering the dietary patterns of Koreans with the highest intakes of carbohydrates, the main mechanisms are the intestinal cleansing effect using dietary fiber or dietary fiber used for obesity and diabetes, which limit total intake of nutrients, and the inhibition of digestion and absorption of fat. Since the diet product is not suitable, it is required to develop a differentiated method suitable for Koreans who can inhibit the absorption of carbohydrates without inhibiting the absorption of other essential inorganic ions and proteins.
한편, 80년대 후반에서 90년대 초에 이르러 몇몇 연구자들에 의해 조류 중 쉽게 접할 수 있으며 고도로 항체를 생성할 수 있는 산란계가 낳은 달걀을 이용한 난황항체에 대한 연구가 시작되었으며, 이러한 연구는 대부분 혈중 항체가의 예측목적, 즉 질병의 진단을 목적으로 행하여진 것으로, 질병의 예방 및 치료를 위해서는 단지 닭의 전염성 F 낭병 바이러스 (Infectious bursal disease virus), 닭의 로타바이러스 (Rotavirus) 등의 닭 바이러스를 이용하여 수행되었다.In the late 80's and early 90's, however, several researchers began to study egg yolk antibodies using eggs laid by laying hens, which are readily accessible among birds and highly capable of producing antibodies. The purpose of this study is to predict the disease, that is, diagnose the disease. For the prevention and treatment of the disease, only chicken virus such as chicken infectious bursal disease virus and chicken rotavirus are used. Was performed.
암탉의 혈청 내의 면역글로블린인 IgG는 후대에 그대로 물려주게 되어 달걀에도 이러한 면역글로블린이 생기게 되는데, 이와 같이 난황에 생긴 면역글로블린을 난황항체 (IgY, egg yolk IgG)라고 하며 이러한 원리를 이용하여 수동면역의 개념으로서 항원에 특이적인 항체를 대량으로 생산, 이를 이용하는 기술이 많이 연구되고 있다. 일단 암탉이 특정 항원에 대한 항체를 생성하는 것을 '습득'하게 되면, 닭의 일생 동안, 즉 10년에 걸쳐서 항체를 생성할 수 있다. 나아가, 달걀은평균적으로 8 ㎎/㎖의 IgG를 가지는 15㎖의 난황을 함유한다. 닭 이외에도, 기타 가금류, 예컨대 칠면조, 오리, 거위 등을 알의 공급원으로서 사용할 수 있다.IgG, the immunoglobulin in the serum of the hen, is passed on to the later generation, and this immunoglobulin is also produced in the egg. Thus, the immunoglobulin produced in egg yolk is called egg yolk antibody (IgY, egg yolk IgG). As a concept, many techniques for producing and using a large amount of antibodies specific for antigen have been studied. Once a hen has 'learned' to produce antibodies to a particular antigen, it can produce antibodies throughout the chicken's life, ie over 10 years. Furthermore, the egg contains 15 ml of egg yolk with an average of 8 mg / ml IgG. In addition to chickens, other poultry such as turkeys, ducks, geese and the like can be used as a source of eggs.
알을 낳는 닭은 닭에서 발견되는 모든 항체 아이소타입, 즉 IgY, IgM 및 IgA 항체를 알로 전달한다. 난황은 단지 IgY만을 함유하고 IgM 및 IgA는 난백 부분에만 존재하는데, 닭의 혈청 IgY 농도는 항원의 단일 투여 후 (약 1 주일 후) 난황에 영향을 준다. 난황은 3∼25 ㎎ IgY/㎖를 포함하므로 중량에 따라 각 알은 40∼500 ㎎ IgY를 제공할 수 있다.Laying chickens deliver all the antibody isotypes found in chickens, namely IgY, IgM and IgA antibodies, to eggs. Egg yolk contains only IgY and IgM and IgA are present only in the egg white portion, and the serum IgY concentration in chickens affects yolk after a single dose of antigen (after about a week). Egg yolk contains between 3 and 25 mg IgY / ml so each egg can provide between 40 and 500 mg IgY by weight.
난황 항체의 장점은 다량으로 얻을 수 있으며, 이의 추출은 비용을 많이 투자하지 않고도 대규모로 수행할 수 있어 매우 경제적이다. 또한, 난황항체는 포유류 보체, Fc 수용체, 단백질 A 또는 단백질 G와 반응하지 않아 면역반응을 일으키지 않으며, 산 및 열에 대해 큰 내성을 나타낸다. FDA는 난황항체를 약물이라기보다는 식품으로 간주하여 GRAS (일반적으로 안전한 것으로 허용됨) 상태로 승인하였으며, 난황항체를 AIDS 또는 기타 질병에 걸린 인간에게 사용할 수 있도록 FDA가 승인하였기 때문에 그 안정성에 있어도 매우 우수하다.The advantages of egg yolk antibodies can be obtained in large quantities, and their extraction is very economical because they can be carried out on a large scale without costly investment. In addition, yolk antibodies do not react with mammalian complement, Fc receptor, protein A or protein G, and thus do not cause an immune response, and exhibit great resistance to acids and heat. The FDA has approved yolk antibodies as food rather than drugs, and has approved them as GRAS (generally accepted as safe), and the FDA has approved them for use in humans with AIDS or other diseases. Do.
이와 같이 난황항체를 이용하여 항원에 특이적인 항체를 대량으로 생산, 이를 이용하는 기술로는 미국의 CalaGen사와 ImmuCell사에 의해 초유에서 분리한 항체 (IgA)를 이용하여 장내 감염 미생물에 의한 질환 치료제가 개발되어 임상 중에 있으며, 현재 국내에서도 위장병의 원인균인 헬리코박터 파이로리를 비롯하여 대장균, 살모넬라, 충치의 주원인균인 스트렙토코커스 뮤탄스 등에 대한 난황항체를 이용하여 식품 첨가제 및 사료 첨가제 등으로 이용되고 있다.As a technology for producing a large amount of antibodies specific to antigens using egg yolk antibodies, a drug for the treatment of diseases caused by intestinal infectious microorganisms is developed using antibodies (IgA) isolated from colostrum by CalaGen and ImmuCell in the United States. It is currently in clinical trials and is currently used as a food additive and feed additive by using egg yolk antibodies against E. coli, Salmonella, Streptococcus mutans, which are the main causes of caries, including Helicobacter pylori, which is a causative agent of gastrointestinal diseases.
이에 본 발명자들은 탄수화물의 소화 흡수에서 중요한 역할을 하는 효소인 수크라아제와 말타아제를 돼지 소장으로부터 분리하여 이를 항원으로 닭에 면역 접종한 후 생산된 달걀로부터 이에 대한 난황항체를 생산하는 방법을 개발하고 상기 방법에 의해 생산된 난황항체가 생체 내 탄수화물의 소화 흡수를 직접적으로 억제하여 비만 및 당뇨 질환의 개선 및 치료용 조성물로 유용하게 사용될 수 있음을 밝힘으로써 본 발명을 완성하였다.Therefore, the present inventors have developed a method for producing yolk antibodies from eggs, which are isolated from the small intestine of sucrase and maltase, enzymes that play an important role in the digestion and absorption of carbohydrates from pig intestine, and then immunized with chicken. The present invention was completed by revealing that the yolk antibody produced by the method directly inhibits digestion and absorption of carbohydrates in vivo, and thus can be usefully used as a composition for improving and treating obesity and diabetes diseases.
본 발명의 목적은 산란계에서 탄수화물 분해효소에 대한 난황항체를 생산하는 방법을 제공하는 것이다.An object of the present invention is to provide a method for producing egg yolk antibodies against carbohydrate degrading enzymes in laying hens.
본 발명의 다른 목적은 상기 난황항체를 포함하는 탄수화물 흡수 억제용 조성물을 제공하는 것이다.Another object of the present invention to provide a composition for inhibiting carbohydrate absorption comprising the yolk antibody.
도 1은 본 발명에 따라 음이온 교환 컬럼 크로마토그라피를 이용하여 돼지 소장의 막 단백질로부터 수크라아제와 말타아제를 분리한 결과이고,1 is a result of separating sucrase and maltase from membrane proteins of the small intestine using anion exchange column chromatography according to the present invention,
도 2는 도 1에서 분리된 수크라아제와 말타아제의 온도에 따른 반응 속도의 변화를 나타낸 것이고,Figure 2 shows the change in reaction rate with the temperature of the sucrase and maltase isolated in Figure 1,
도 3은 도 1에서 분리된 수크라아제와 말타아제의 pH에 따른 반응 속도의 변화를 나타낸 것이고,Figure 3 shows the change in the reaction rate according to the pH of the sucrase and maltase isolated in Figure 1,
도 4는 도 1에서 분리된 수크라아제와 말타아제를 항원으로 면역접종 시 접종 횟수에 따른 산란계의 혈액 중 항 말타아제 항체의 역가를 나타낸 것이고,Figure 4 shows the titer of the anti-maltase antibody in the blood of the laying hen according to the number of inoculations when immunized with the sucrase and maltase isolated in Figure 1,
도 5는 본 발명에 따라 제조된 난황항체에 의해 돼지 소장 유래 말타아제의 활성이 직접적으로 억제되는 것을 나타낸 것이고,Figure 5 shows that the activity of porcine small intestine-derived maltase is directly inhibited by the yolk antibody prepared according to the present invention,
도 6은 본 발명에 따라 제조된 난황항체에 의해 돼지 소장 유래 수크라아제의 활성이 직접적으로 억제되는 것을 나타낸 것이고,Figure 6 shows that the activity of porcine small intestine-derived sucrase is directly inhibited by the yolk antibody prepared according to the present invention,
도 7은 동물모델인 랫트를 이용한 수크로스 과부하 실험 시에 본 발명의 난황항체에 의한 체내 당 농도 증가의 억제를 측정한 결과이고,7 is a result of measuring the inhibition of the increase in the body sugar concentration by the yolk antibody of the present invention during the sucrose overload experiment using a rat animal model,
도 8은 동물모델인 랫트를 이용한 말토스 과부하 실험 시에 본 발명의 난황항체에 의한 체내 당 농도 증가의 억제를 측정한 결과이다.8 is a result of measuring the inhibition of the increase in the body sugar concentration by the yolk antibody of the present invention during the maltose overload experiment using the rat animal model.
상기 목적을 달성하기 위하여, 본 발명은 수크라아제와 말타아제를 항원으로 사용하여 산란계에서 난황항체를 생산하는 방법을 제공한다.In order to achieve the above object, the present invention provides a method for producing egg yolk antibodies in laying hens using sucrase and maltase as antigens.
또한, 본 발명은 상기 방법에 의해 생산된 난황항체를 유효성분으로 함유하는 탄수화물 흡수 억제용 약학 조성물을 제공한다.The present invention also provides a pharmaceutical composition for inhibiting carbohydrate absorption containing the yolk antibody produced by the above method as an active ingredient.
아울러, 본 발명은 상기 방법에 의해 생산된 난황항체를 유효성분으로 함유하는 식품 및 음료 조성물을 제공한다.In addition, the present invention provides a food and beverage composition containing the yolk antibody produced by the method as an active ingredient.
이하, 본 발명을 상세히 설명한다.Hereinafter, the present invention will be described in detail.
본 발명은 수크라아제와 말타아제를 항원으로 사용하여 산란계에서 난황항체를 생산하는 방법을 제공한다.The present invention provides a method for producing yolk antibodies in a laying hen using sucrase and maltase as antigens.
상기 생산방법은The production method
1) 수크라아제와 말타아제 단백질을 항원으로 사용하여 산란계에 면역시키고 이로부터 난황항체를 생산하는 단계; 및1) immunizing laying hens using sucralase and maltase proteins as antigens to produce egg yolk antibodies therefrom; And
2) 상기 산란계가 낳은 달걀의 난황으로부터 난황항체를 분리하는 단계를 포함한다.2) separating the yolk antibody from the yolk of the egg laid by the laying hen.
이하 상기 단계를 보다 구체적으로 설명한다.The above steps will be described in more detail below.
본 발명의 바람직한 실시예로서 단계 1)에서는 돼지 소장으로부터 막단백질을 분리하고 음이온 교환 컬럼 크로마토그라피를 이용하여 수크라아제와 말타아제를 정제한다 (도 1 참조). 정제된 수크라아제와 말타아제의 효소활성을 측정하기 위하여 각 효소활성의 최적 반응온도와 pH를 조사한 결과, 수크라아제는 40℃와 약산성 pH (pH 5 내지 6) 부근에서, 말타아제는 50℃와 중성 pH (pH 6 내지 7) 부근에서 최고의 활성을 나타내었다 (도 2 및 도 3 참조).In a preferred embodiment of the present invention, in step 1), the membrane protein is separated from the swine small intestine and the sucrase and maltase are purified using anion exchange column chromatography (see FIG. 1). In order to determine the enzymatic activity of purified sucrase and maltase, the optimum reaction temperature and pH of each enzyme activity were examined. As a result, sucrase was near 40 ° C and weakly acidic pH (pH 5-6), and maltase was 50 ° C. The highest activity was found near neutral pH (pH 6-7) (see Figures 2 and 3).
본 발명에서 항원 단백질로 사용된 수크라아제와 말타아제는 돼지 소장뿐만 아니라 랫트, 마우스, 기니아픽, 토끼 또는 사람 및 사람 유래 세포주로부터 분리될 수 있으며, 이들 효소 단백질을 암호화하는 유전자를 포함하는 재조합 미생물에 발현된 것을 분리하여 사용할 수 있고, 화학적으로 합성된 것을 사용할 수도 있다.The sucrase and maltase used as antigenic proteins in the present invention can be isolated from pig small intestine as well as from rat, mouse, guinea pig, rabbit or human and human derived cell lines, and recombinant microorganisms comprising genes encoding these enzyme proteins. The one expressed in the can be used separately, and a chemically synthesized one can also be used.
상기에서 분리된 수크라아제 및 말타아제 단백질을 항원으로 이용하여 산란계에 면역 접종한 후 이로부터 난황항체를 생산할 수 있다. 이용되는 산란계로는 그 종류가 특별히 한정되지는 않지만, 예를 들면 산란율이 높은 백색 레그혼계, 로드아일랜드계, 하이라인 브라운계 등을 이용하는 것이 바람직하다.The isolated sucralase and maltase proteins as antigens can be used to immunize the laying hens to produce egg yolk antibodies therefrom. Although the kind is not specifically limited as a scattering system used, For example, it is preferable to use a white leg horn system, a Rhode island type, a high-line brown type etc. with a high scattering rate.
항원 단백질을 산란계에 피하, 복강내, 근육내 또는 정맥내 주사나 경구 투여와 같은 임의의 적절한 경로로 접조하여 면역화시킨다. 바람직한 면역화 방법은 근육내 주사하는 것이며, 목에 피하 주사도 가능하다. 면역화를 증가시키기 위해서 적절한 보조제가 항원과 함께 투여되는 것이 좋은데, 이를 위해 유용한 보조제는 완전 또는 불완전 프로인트 보조제 (incomplete or complete Freund's adjuvant)와 같은 유중수 유화 보조제이다. 적절한 보조제를 사용하면 장기간 동안 면역화된 산란계의 알에서 높은 항체 역가를 유지하는 데 매우 효과적이며, 따라서 소정의 항체 함유 물질을 효과적으로 생성할 수 있다. 항원의 용량은 일반적으로 10 내지 200 ㎍/㎏ 체중 범위이나 항원과 보조제의 유형, 면역 상태가 과도한 항원 독성 형성 없이 산란계에서 유도될 수 있는 방식의 투여 경로에 따라 변화될 수 있다.The antigenic protein is immunized by laying down the laying hens by any suitable route, such as subcutaneous, intraperitoneal, intramuscular or intravenous injection or oral administration. Preferred immunization methods are intramuscular injection, and subcutaneous injection into the neck is also possible. Appropriate adjuvant is preferably administered with the antigen to increase immunization, useful adjuvant for this is water-in-oil emulsification adjuvant such as incomplete or complete Freund's adjuvant. Using the appropriate adjuvant is very effective in maintaining high antibody titers in eggs of the immunized laying hens for long periods of time, thus effectively producing the desired antibody-containing material. The dose of antigen may vary depending on the route of administration, generally in the range of 10 to 200 μg / kg body weight or type of antigen and adjuvant, and in a manner in which the immune status can be induced in laying hens without formation of excessive antigenic toxicity.
일반적으로 초기 면역화 (접종) 후 몇 주 내에 산란계는 항원에 대한 감응성이 생긴다. 즉, 항원에 대해 면역화된다. 항원에 대한 특이 항체는 산란계의 몸에서 생성되며, 산란계가 낳은 알은 특이 항체를 포함하고 있다. 산란계와 알에서 항원에 대한 특정 항체의 존재 및 역가 농도는 당업계에 공지된 각종 면역학 시험으로 확인할 수 있는데, 본 발명에서는 바람직한 실시예로서 효소면역 측정법 (enzyme-linked immunosorbent assay, ELISA) 등을 사용하여 난황과 혈청의 항체활성을 측정한다.In general, within a few weeks after the initial immunization (inoculation) the laying hens become sensitive to the antigen. That is, it is immunized against the antigen. Antibodies specific for antigens are produced in the body of a laying hen, and the eggs laid by the laying hens contain specific antibodies. The presence and titer concentrations of specific antibodies to antigens in laying hens and eggs can be confirmed by various immunological tests known in the art. In the present invention, an enzyme-linked immunosorbent assay (ELISA) is used as a preferred embodiment. The antibody activity of yolk and serum was measured.
항원에 대한 초기 면역화 이후, 적절한 용량의 1회 이상의 추가 항원을 투여하여 산란계에서 높은 항체 역가를 유지할 수 있다. 각각의 추가 항원 투여에서, 적절한 보조제는 항원과 함께 사용될 수 있다. 초기 면역화와 1차 추가 항원 투여 사이의 간격과, 개별 추가 항원 투여 사이의 간격은 항원의 특성에 좌우되며, 2주 이상인 것이 좋다.After initial immunization against the antigen, an appropriate dose of one or more additional antigens can be administered to maintain high antibody titers in the laying hens. In each additional antigen administration, appropriate adjuvants may be used with the antigen. The interval between the initial immunization and the administration of the first additional antigen, and the interval between the individual additional antigen administrations, depends on the nature of the antigen and is preferably at least two weeks.
소정의 특이 항체의 적절한 역가가 면역화된 산란계가 낳은 알에 존재하는 것을 확인한 후에, 산란계가 낳은 알을 모으고 필요에 따라 사용 전까지 저장한다. 동일한 항체에 대해 면역화한 1종 이상의 산란계가 낳은 여러 개의 알을 모으고 함께 처리하여 항체를 포함하는 소정의 물질을 생성하는 것이 편리하다.After confirming that the appropriate titers of the specific specific antibodies are present in the eggs laid by the immunized laying hens, the eggs laid by the laying hens are collected and stored as needed before use. It is convenient to collect several eggs from one or more laying hens immunized against the same antibody and process them together to produce the desired material comprising the antibody.
단계 2)는 산란계가 낳은 달걀의 난황으로부터 난황항체를 분리하는 단계로서, 달걀의 난황은 고농도의 지방분을 포함하고 있어 난황황체의 작용을 용이하게 하기 위해서는 고효율로 순수 분리하는 것이 필요하며, 특히 생체에 유해하지 않아야 한다. 이를 위하여, 산란계에서 회수한 달걀로부터 난황항체를 정제하기 위한 추출 재료로 λ-카라기난과 다당류 및 증류수 또는 카프릴산 (caprylic acid)을 이용한 추출 등이 이용될 수 있다. 본 발명의 바람직한 실시예에서는 분리한 난황을 증류수로 희석시킨 용액에 카라기난 용액을 첨가한 후 원심분리하여 난황 리포 단백질을 침전시킨 후 이로부터 얻은 상등액을 염출하여 난황 수용성 단백질만을 분리한다. 특히, 카라기난 용액은 식품첨가물로서 공인된 검 용액으로 생체안정성과 항체 회수율이 우수하고 회수한 항체의 역가를 높게 유지할 수 있다.Step 2) is to separate egg yolk antibodies from egg yolks laid by laying hens. Egg yolks contain high concentrations of fat, so it is necessary to separate them with high efficiency to facilitate the action of egg yolks. Should not be harmful to To this end, extraction using λ-carrageenan and polysaccharides and distilled water or caprylic acid may be used as an extraction material for purifying egg yolk antibodies from eggs recovered from a laying hen. In a preferred embodiment of the present invention, after adding the carrageenan solution to the diluted solution of the egg yolk diluted with distilled water, and centrifugation to precipitate the yolk lipo protein, the supernatant obtained therefrom is salted to separate only the yolk soluble protein. In particular, the carrageenan solution is a gum solution certified as a food additive, and has excellent biostability, antibody recovery rate, and can maintain high titer of recovered antibody.
이와 같이 분리·정제된 난황항체는 말타아제와 수크라아제의 효소활성을 효과적으로 억제하며 (도 4 및 도 5 참조), 생체 내 적용 시 상기 효소활성 억제를 통해 탄수화물의 흡수를 효과적으로 저해함으로써 혈당량을 감소시킴을 확인하였다 (도 6 및 도 7 참조).The isolated and purified egg yolk antibody effectively inhibits the enzymatic activity of maltase and sucrase (see FIGS. 4 and 5), and reduces blood glucose by effectively inhibiting the absorption of carbohydrates through the inhibition of the enzyme activity in vivo. Confirmation was made (see FIGS. 6 and 7).
또한, 본 발명은 상기 방법에 의해 생산된 난황항체를 유효성분으로 함유하는 탄수화물 흡수 억제용 약학 조성물을 제공한다.The present invention also provides a pharmaceutical composition for inhibiting carbohydrate absorption containing the yolk antibody produced by the above method as an active ingredient.
본 발명에 따라 생산된 수크라아제와 말타아제에 대한 난황항체는 생체 내에서 탄수화물의 분해를 직접적으로 억제하여 혈당량을 감소시키므로 상기 난황항체를 유효성분으로 하는 약학 조성물은 음식물 섭취의 제한 없이 과도한 탄수화물의 흡수에 기인한 질환들, 예를 들어, 비만, 당뇨병, 고혈압 등의 예방 및 치료에 유용하게 사용될 수 있다.The yolk antibody to sucralase and maltase produced according to the present invention directly inhibits the breakdown of carbohydrates in vivo, thereby reducing blood sugar levels. Thus, the pharmaceutical composition comprising the yolk antibody as an active ingredient may be used as an excess of carbohydrate without limiting food intake. It can be usefully used for the prevention and treatment of diseases due to absorption, for example, obesity, diabetes, hypertension and the like.
본 발명의 조성물을 이용하여 통상적인 방법에 따라 약학 제형을 제조할 수 있다. 제형은 정제, 알약, 분말, 새세이, 엘릭서, 현탁액, 에멀젼, 용액, 시럽, 에어로졸, 연질 및 경질 젤라틴 캅셀, 멸균 주사용액, 멸균 포장 분말 등의 형태일 수 있다.The pharmaceutical formulations can be prepared according to conventional methods using the compositions of the present invention. The formulation may be in the form of tablets, pills, powders, assays, elixirs, suspensions, emulsions, solutions, syrups, aerosols, soft and hard gelatin capsules, sterile injectable solutions, sterile packaged powders and the like.
적당한 담체, 부형제 및 희석제의 예로는, 락토즈, 덱스트로즈, 수크로즈, 솔비톨, 만니톨, 전분, 아카시아 검, 알긴산염, 젤라틴, 칼슘 포스페이트, 칼슘 실리케이트, 셀룰로즈, 메틸 셀룰로즈, 미정질 셀룰로즈, 폴리비닐피롤리돈, 물, 메틸하이드록시벤조에이트, 프로필하이드록시벤조에이트, 탈크, 마그네슘 스테아레이트 및 광물유를 들 수 있다. 제형은 충진제, 항응집제, 윤활제, 습윤제, 향료, 유화제, 방부제 등을 추가로 포함할 수 있다. 본 발명의 조성물은 포유 동물에 투여된 후 활성 성분의 신속, 지속 또는 지연된 방출을 제공할 수 있도록 당업계에 공지된 방법을 사용하여 제형화할 수 있다.Examples of suitable carriers, excipients and diluents include lactose, dextrose, sucrose, sorbitol, mannitol, starch, acacia gum, alginate, gelatin, calcium phosphate, calcium silicate, cellulose, methyl cellulose, microcrystalline cellulose, poly Vinylpyrrolidone, water, methylhydroxybenzoate, propylhydroxybenzoate, talc, magnesium stearate and mineral oil. The formulation may further comprise fillers, anti-coagulants, lubricants, wetting agents, fragrances, emulsifiers, preservatives and the like. Compositions of the present invention can be formulated using methods known in the art to provide rapid, sustained or delayed release of the active ingredient after administration to a mammal.
본 발명의 약학 조성물은 경구, 경피, 피하, 정맥내 또는 근육내를 포함한 여러 경로를 통해 투여될 수 있다. 사람의 경우 난황항체의 통상적인 1일 투여량은 5 내지 30 mg/㎏ 체중, 바람직하게는 10 내지 20 mg/㎏ 체중의 범위일 수 있고, 1회 또는 수회로 나누어 투여할 수 있다.The pharmaceutical compositions of the invention can be administered via several routes including oral, transdermal, subcutaneous, intravenous or intramuscular. In humans a typical daily dose of yolk antibody may range from 5 to 30 mg / kg body weight, preferably 10 to 20 mg / kg body weight, and may be administered once or in several doses.
그러나, 활성 성분의 실제 투여량은 치료할 질환, 선택된 투여 경로, 환자의 연령, 성별, 체중 및 환자의 증상의 중증도 등의 여러 관련 인자에 비추어 결정되어야 하는 것으로 이해되어야 하며, 따라서 상기 투여량은 어떠한 방법으로도 본 발명의 범위를 한정하는 것이 아니다.However, it should be understood that the actual dosage of the active ingredient should be determined in light of several relevant factors such as the disease to be treated, the route of administration chosen, the age, sex, weight of the patient and the severity of the patient's symptoms, and thus the dosage may be The method does not limit the scope of the present invention.
아울러, 본 발명은 상기 방법에 의해 생산된 난황항체를 유효성분으로 함유하는 식품 및 음료 조성물을 제공한다.In addition, the present invention provides a food and beverage composition containing the yolk antibody produced by the method as an active ingredient.
본 발명의 식품 및 음료 조성물은 체내에서 탄수화물의 분해를 억제하므로 비만 억제, 혈당량 조절 등을 통하여 건간을 유지 및 향상시킬 수 있다.Since the food and beverage composition of the present invention inhibits the breakdown of carbohydrates in the body, it is possible to maintain and improve dryness through inhibition of obesity, blood sugar control, and the like.
본 발명의 난황항체는 또한 비만 개선을 위한 다이어트 원료로서, 또는 과도한 탄수화물의 흡수에 기인한 질환, 예를 들어 당뇨병 등의 예방 및 치료 효과를 나타낼 목적으로 식품 또는 음료에 첨가제 또는 식품 보조제로서 혼입될 수 있다. 상기 식품 또는 음료로는, 육류; 야채 쥬스 (예를 들어, 당근 쥬스 및 토마토 쥬스) 및 과일 쥬스 (예를 들어, 오렌지 쥬스, 포도 쥬스, 파인애플 쥬스, 사과 쥬스및 바나나 쥬스); 초콜렛; 스넥류; 과자류; 피자; 빵, 케익, 크래커, 쿠키, 비스킷, 누들 등과 같이 곡물 분말로 만들어진 식품류; 껌류; 우유, 치즈, 요구르트 및 아이스크림과 같은 유제품; 스프; 육즙; 페이스트, 케찹 및 쏘스; 차; 알콜성 음료류; 탄산 음료류; 비타민 복합체; 및 다양한 건강 식품류 등이 있다. 이 경우, 식품 또는 음료 중 난황항체의 함량은 0.05 내지 0.5 중량%, 바람직하게는 0.1 내지 0.2 중량%의 범위일 수 있다.The yolk antibody of the present invention may also be incorporated as a dietary ingredient for improving obesity, or as an additive or food supplement in foods or beverages for the purpose of exhibiting a prophylactic and therapeutic effect such as diseases caused by excessive carbohydrate absorption, such as diabetes. Can be. As the food or beverage, meat; Vegetable juices (eg, carrot juice and tomato juice) and fruit juices (eg, orange juice, grape juice, pineapple juice, apple juice and banana juice); Chocolate; Snacks; confectionery; Pizza; Food products made of grain powder such as bread, cakes, crackers, cookies, biscuits, noodle, etc .; Gums; Dairy products such as milk, cheese, yogurt and ice cream; soup; Juicy; Pastes, ketchups and sauces; car; Alcoholic beverages; Carbonated beverages; Vitamin complexes; And various health foods. In this case, the content of the yolk antibody in the food or beverage may be in the range of 0.05 to 0.5% by weight, preferably 0.1 to 0.2% by weight.
이하, 본 발명을 실시예에 의해 상세히 설명한다.Hereinafter, the present invention will be described in detail by way of examples.
단, 하기 실시예는 본 발명을 예시하는 것일 뿐, 본 발명의 내용이 하기 실시예에 한정되는 것은 아니다.However, the following examples are merely to illustrate the invention, but the content of the present invention is not limited to the following examples.
<실시예 1> 수크라아제와 말타아제 난황항체의 제조Example 1 Preparation of Sucrase and Maltase Egg Yolk Antibody
(단계 1) 돼지 소장으로부터 수크라아제와 말타아제의 분리(Step 1) Separation of sucrase and maltase from pig small intestine
소화 효소에 관여하는 수크라아제와 말타아제의 분리를 위하여 신선한 돼지의 소장을 생리식염이 포함된 인산염 완충액 (sodium phosphate saline buffer, 이하 'PBS'로 약칭함)으로 세척하고 점막층을 긁어낸 후, 200 mM 만니톨을 포함하는 20 mM Tris-HCl 완충액 (pH 6)에 1:10의 비율로 혼합하였다. 상기 혼합액을 균질화하고 50 mM의 염화칼슘을 첨가하여 방치한 후 원심분리하여 상층액만을 회수하였다. 회수된 상층액을 35,000× g로 초원심분리하여 침전된 막단백질을 분리하였다. 분리된 막단백질을 50 mM Tris-HCl 완충액 (pH 8)으로 평형화시킨 DEAE-세파로오스 (DEAE-Sepharose) 컬럼 (아머샴파마시아바이오텍사)에 단백질을 흡착시키고 0 내지 1.0 M 염화나트륨을 포함하는 동일 완충액으로 선택적으로 단백질들을 분획하여 수크라아제와 말타아제를 분리하였다 (도 1).In order to separate sucrase and maltase involved in digestive enzymes, fresh pig small intestine was washed with phosphate buffer containing physiological salt (abbreviated as 'PBS') and scraped off the mucosa. 20 mM Tris-HCl buffer (pH 6) containing mM mannitol was mixed at a ratio of 1:10. The mixture was homogenized, left to stand by addition of 50 mM calcium chloride and centrifuged to recover only the supernatant. The recovered supernatant was ultracentrifuged at 35,000 x g to separate the precipitated membrane protein. The isolated membrane protein was adsorbed onto a DEAE-Sepharose column (Amersham Pharmacia Biotech Co., Ltd.) equilibrated with 50 mM Tris-HCl buffer (pH 8) and the same containing 0-1.0 M sodium chloride. Proteins were selectively fractionated with buffer to separate sucrase and maltase (FIG. 1).
이들 소장 유래 막 단백질들은 당과 결합된 당단백질로 수크라아제 활성과 말타아제 활성을 가지는 소단위 (subunit)로 구성되어 있으며 14 내지 15만 정도의 분자량을 가진다. 또한, 장내 부위에 따라 분자량 26만 정도의 하나의 긴 폴리펩티드 사슬로도 나타난다 (Siostrom, H.et al.,J. Biolog. Chem.255(23), 1980). 상기에서 분리된 수크라아제와 말타아제 단백질 분획을 SDS-PAGE 전기영동으로 분석한 결과, 분자량 20만 이상과 15만 정도의 위치에서 단백질 밴드가 검출됨을 확인하였다.These small intestine-derived membrane proteins are glycoproteins linked with sugars, and are composed of subunits having sucrase activity and maltase activity, and have molecular weights of about 14 to 150,000. It also appears as one long polypeptide chain with a molecular weight of about 260,000 depending on the intestinal site (Siostrom, H. et al ., J. Biolog. Chem. 255 (23), 1980). As a result of SDS-PAGE electrophoresis analysis of the isolated sucralase and maltase protein fractions, it was confirmed that protein bands were detected at positions of at least 200,000 and about 150,000 molecular weights.
(단계 2) 분리된 수크라아제와 말타아제의 효소활성 측정(Step 2) Determination of Enzyme Activity of Isolated Sucrase and Maltase
상기 단계 1에서 분리된 효소의 활성을 조사하기 위하여 기질로 수크로스와 말토스 각각을 첨가하여 효소 반응을 수행하였다. 반응액은 기질 1%, 50 mM 인산염 완충액, 효소 (0.2 munit), 증류수를 포함하며 반응용량은 0.1 ㎖로 37℃에서 20분간 반응시켰다. 이때, 효소의 최적 반응 온도와 pH의 조사를 위하여 온도는 30℃ 내지 70℃까지의 온도범위에서 반응시켰으며 pH는 3 내지 9까지의 pH 범위에서 반응시켰다. 반응 후 100℃에서 효소활성을 정지시켰으며 생성된 포도당 농도는 포도당 산화효소를 이용한 GOD-POD 비색방법인 지엘자임키트 (신양화학약품사)를 이용하여 정량하였다.In order to investigate the activity of the enzyme isolated in step 1, sucrose and maltose were added to the substrate, respectively, to perform an enzyme reaction. The reaction solution contains a substrate 1%, 50 mM phosphate buffer, enzyme (0.2 munit), distilled water and the reaction volume was reacted for 20 minutes at 37 ℃ with 0.1 ml. At this time, the temperature was reacted in the temperature range of 30 ℃ to 70 ℃ for the investigation of the optimum reaction temperature and pH of the enzyme and the pH was reacted in the pH range of 3 to 9. After the reaction, the enzyme activity was stopped at 100 ° C, and the resulting glucose concentration was quantified using GEL-zyme kit (Shinyang Chemical Co., Ltd.), a GOD-POD colorimetric method using glucose oxidase.
그 결과, 수크라아제는 40℃와 약산성 (pH 5 내지 6) 부근에서 최고의 효소활성을 보였으며 말타아제는 50℃와 중성 (pH 6 내지 7)에서 최고의 활성을 나타내었다(도 2 및 도 3).As a result, sucrase showed the highest enzymatic activity at 40 ° C. and weak acid (pH 5-6) and maltase showed the highest activity at 50 ° C. and neutral (pH 6-7) (FIGS. 2 and 3). .
(단계 3) 산란계의 면역(Step 3) Immune of laying hens
상기와 같이 돼지 소장으로부터 분리·정제된 수크라아제와 말타아제를 항원으로 이용하여 보아스 브라운 (Boas brown) 종 산란계 20마리의 다리 근육에 100 ㎍/㎏의 농도로 면역 보조제인 프로인트 불완전 보조제와 함께 3주 간격으로 3회 접종 후 마지막 4회는 면역 보조제 없이 항원만으로 면역 접종을 실시하였다. 달걀은 매일 수집한 후 4℃에서 보관하고, 면역 접종된 산란계에서 주입된 항원에 대한 항체의 형성 여부를 확인하기 위하여 면역 접종 횟수별로 혈액을 채혈한 후 혈청을 분리하여 하기와 같이 효소 면역 측정법 (ELISA)을 수행하였다.Suprase and maltase isolated and purified from porcine small intestine were used as antigens with the Freund's incomplete adjuvant, an immunoadjuvant at a concentration of 100 μg / kg in 20 muscles of Boas brown species laying hens. After inoculation three times at three week intervals, the last four were immunized with antigen alone without an adjuvant. Eggs are collected daily and stored at 4 ° C., and blood is collected by the number of immunizations to determine the formation of antibodies to the injected antigen in the inoculated laying hens. ELISA) was performed.
효소 면역 측정법을 위한 항원으로 상기 단계 1에서 분리한 수크라아제와 말타아제를 96 웰 마이크로플레이트에 1 내지 100 ㎍을 분주하여 밤새 코팅한 다음, 비특이적 항체의 결합을 방지하기 위하여 5% 탈지유 (skim milk)를 처리하였다. 상기 웰 플레이트를 완충액으로 3회 세척하고, 항혈청을 3,000배 희석하여 37℃에서 30 내지 60분간 일차 항체로서 반응시킨 후, 결합하지 않은 항체를 0.02% 트윈 20이 함유된 생리식염 함유 인산염 완충액으로 3회 세척하였다. 여기에 다시 알카라인 포스파타아제가 결합된 항-닭 IgG (시그마알드리치)를 1,000배 희석하여 이차 항체로서 실온에서 60분간 결합시켰다. 반응이 종결된 후 상기 플레이트를 0.02% 트윈 20이 함유된 완충액으로 5회 세척하고 알카라인 포스파타아제의 기질인 PNPP (p-nitrophenyl phosphate in diethanolamine buffer, 시그마알드리치) 1 ㎎/㎖을 첨가하여 40분간 반응시킨 후 450 ㎚에서 ELISA 판독기로 각 웰의 흡광도를 측정하였다. 그 결과, 2차 접종 이후에 말타아제에 대한 항체가 산란계의 혈청 내에서생성되기 시작하였으며 3차 접종이후 최고치를 유지하였다(도 4).Sucase and maltase isolated in step 1 as an antigen for enzymatic immunoassay were coated overnight by dispensing 1-100 μg into 96 well microplates, and then 5% skim milk to prevent binding of nonspecific antibodies. ). The well plate was washed three times with buffer, the antiserum was diluted 3,000 times and reacted as a primary antibody at 37 ° C. for 30 to 60 minutes, and then the unbound antibody was washed with physiological salt-containing phosphate buffer containing 0.02% Tween 20. Washed twice. Here again, alkaline phosphatase-bound anti-chicken IgG (Sigma Aldrich) was diluted 1,000-fold and bound for 60 minutes at room temperature as a secondary antibody. After the reaction was completed, the plate was washed five times with a buffer containing 0.02% Tween 20 and 40 mg of PNPP (p-nitrophenyl phosphate in diethanolamine buffer, Sigma Aldrich), a substrate of alkaline phosphatase, was added for 40 minutes. After the reaction, the absorbance of each well was measured with an ELISA reader at 450 nm. As a result, after the second inoculation, antibodies to maltase began to be generated in the serum of the laying hens and maintained their maximum after the third inoculation (FIG. 4).
(단계 4) 난황항체의 분리(Step 4) Isolation of Yolk Antibody
상기에서 수크라아제와 말타아제 항원 단백질에 대한 항체의 형성이 확인된 산란계로부터 회수한 달걀의 난황을 분리한 후 증류수와 1:1의 부피로 혼합하였다. 여기에 λ-카라기난 (carrageenan, 1 ㎎/㎖ in D.W., 시그마알드리치) 용액을 2배로 첨가한 후 실온에서 30분간 방치하였다. 상기 혼합액을 원심분리 (10,000× g, 15분, 20℃)하여 상등액만을 취하고 와트만 여과지 (Watman No. 2 filter paper)로 여과한 후 통과된 여액에 19% 황화 나트륨 (sodium sulfate)을 첨가하여 염출을 수행하였다. 이를 다시 원심분리 (10,000× g, 15분, 20℃)하여 침전물만을 회수한 후 PBS에 재현탁시키고 황화 나트륨을 이용하여 염출과 원심분리 (10,000× g, 15분)를 수행하였다. PBS에 재현탁된 시료를 10 mM PBS로 투석한 후 이로부터 얻은 투석액을 동결건조하여 난황항체를 얻었다.The egg yolk of the eggs recovered from the laying hens, in which the formation of antibodies to the sucrase and maltase antigen proteins was confirmed, was separated and mixed with distilled water in a volume of 1: 1. The solution of λ-carrageenan (1 mg / ml in D.W., Sigma Aldrich) was added twice and allowed to stand at room temperature for 30 minutes. The mixture was centrifuged (10,000 × g, 15 minutes, 20 ° C.) to take only the supernatant, filtered with a Wattman No. 2 filter paper, and then added 19% sodium sulfate to the filtrate. The brine was performed. This was again centrifuged (10,000 × g, 15 min, 20 ° C.) to recover only the precipitate and then resuspended in PBS, followed by brine and centrifugation (10,000 × g, 15 min) using sodium sulfide. The sample resuspended in PBS was dialyzed with 10 mM PBS, and the dialysate obtained therefrom was lyophilized to obtain an yolk antibody.
<실시예 2> 난황항체의 효소활성 억제 확인<Example 2> Confirmation of inhibition of enzyme activity of egg yolk antibody
상기 실시예 1로부터 분리·정제된 난황항체가 실제로 융모세포 막수송체의 수크라아제와 말타아제의 활성을 억제할 수 있는지의 여부를 확인하기 위해서 상기 실시예 1의 단계 2와 동일한 방법으로 각각 수크라아제와 말타아제의 효소활성을 측정하였다. 효소반응 시에 난황항체를 1 ㎎/㎖의 농도로 첨가하여 효소의 활성저해 정도를 측정하였다. 수크라아제와 말타아제에 대한 난황항체의 활성저해를 비교하기 위해 효소를 첨가하지 않은 대조군과 항체 미첨가군, 일반 난황항체 첨가군, 수크라아제와 말타아제에 면역화된 난황항체 첨가군을 이용하였다.In order to confirm whether the yolk antibody isolated and purified from Example 1 can actually inhibit the activity of sucrase and maltase of chorion cell membrane transporter, Enzyme activity of Kraase and Maltase was measured. During the enzymatic reaction, yolk antibody was added at a concentration of 1 mg / ml to determine the degree of activity inhibition. In order to compare the activity of yolk antibodies against sucrase and maltase, a control group without an enzyme, no antibody addition group, a general yolk antibody addition group, and a yolk antibody addition group immunized to sucrase and maltase were used.
그 결과, 도 5 및 도 6에 나타난 바와 같이, 본 발명에 따라 제조된 난황항체에 의해 수크라아제와 말타아제 모두 약 60% 정도의 효소활성이 저해됨을 확인하였다.As a result, as shown in Figures 5 and 6, it was confirmed that about 60% of the enzyme activity of both sucrase and maltase were inhibited by the yolk antibody prepared according to the present invention.
<실시예 3> 생체 내 탄수화물의 흡수 억제 활성Example 3 Inhibitory Activity of Carbohydrates in Vivo
본 발명에 따라 제조된 난황항체가 생체 내 탄수화물의 흡수 억제 활성을 나타내는지 여부를 SD 랫트를 이용하여 조사하였다. 체중 400 g의 10 주령 SD 랫트 (대한실험동물)를 각 군당 10마리씩 4군으로 분리하여 12시간 동안 절식시킨 후, 대조군에는 생리식염수만 투여하였고, 실험군에는 본 발명에 따라 제조된 난황항체를 체중 1 ㎏당 1 ㎎ 또는 5 ㎎으로 투여하였다. 투여 시 항체를 생리식염이 함유된 인산염 완충액에 분산시킨 주사액을 존대를 이용하여 경구투여하였다. 난황항체 투여 후 10분 경과한 뒤 200 ㎎/㎏의 수크로오스 및 말토스를 각각 경구 투여하였고 시간별로 혈액을 채취하여 혈당량을 정량하였다. 혈액 내 포도당 농도는 포도당 산화효소를 이용한 GOD-POD 비색방법인 지엘자임키트 (신양화학약품)를 이용하여 정량하였다.Whether the yolk antibody prepared according to the present invention exhibits the absorption inhibitory activity of carbohydrates in vivo was investigated using SD rats. 10-week-old SD rats (Korean experimental animals) weighing 400 g were divided into 4 groups of 10 rats in each group and fasted for 12 hours, and then control group was administered only saline, and the experimental group weighed yolk antibodies prepared according to the present invention. Administration at 1 mg or 5 mg per kg. At the time of administration, the injection solution in which the antibody was dispersed in phosphate buffer containing physiological salts was administered orally using horn. After 10 minutes after yolk antibody administration, 200 mg / kg of sucrose and maltose were orally administered, respectively, and blood was collected by time to quantify blood glucose levels. Blood glucose levels were quantified using GEL-zyme kit (Shinyang Chemical), a GOD-POD colorimetric method using glucose oxidase.
그 결과, 난황항체를 투여하지 않은 대조군에서는 혈당량이 시간이 경과함에 따라 증가하였으며, 30분째에 12 ㎎/㎗, 4시간째에 35 ㎎/㎗가 증가하였다. 체중 1 ㎏당 1 ㎎ 또는 5 ㎎의 난황항체가 투여된 실험군에서는 혈당량이 30분째에 각각 5 ㎎/㎗와 4 ㎎/㎗의 증가량을 보여 대조군에 대하여 각각 58% 및 67%의 혈당 흡수 억제 효과를 보였으며, 4시간째에는 22 ㎎/㎗ 및 13 ㎎/㎗의 혈당 증가량을 보여 대조군에 대비하여 37% 및 65%의 억제 효과를 보였다(도 7).As a result, in the control group that did not receive the yolk antibody, blood glucose levels increased with time, 12 mg / dL at 30 minutes, and 35 mg / dL at 4 hours. In the experimental group administered with 1 mg or 5 mg of yolk antibody per 1 kg of body weight, blood glucose levels increased by 5 mg / dL and 4 mg / dL at 30 minutes, respectively. At 4 hours, blood glucose increases of 22 mg / dL and 13 mg / dL were shown, indicating an inhibitory effect of 37% and 65% compared to the control group (FIG. 7).
말토스의 경우에는, 대조군에서는 혈당량이 30분째에 10.6 ㎎/㎗, 4시간째에 23.9 ㎎/㎗로 증가한 반면, 난황항체가 각각 체중 1 ㎏당 1 ㎎ 또는 5 ㎎ 농도로 투여된 실험군에서는 혈당량이 각각 30분째에 9.6 ㎎/㎗ 및 7.8 ㎎/㎗의 증가량을 보여 대조군에 대비하여 9% 및 26%의 혈당량 증가 억제 효과를 보였다. 4시간째에 도 혈당 증가량은 19.3 ㎎/㎗ 및 12.4 ㎎/㎗로 대조군 대비 19%와 48%의 억제 효과를 보였다(도 8).In the case of maltose, the blood glucose level in the control group increased to 10.6 mg / dL at 30 minutes and 23.9 mg / dL at 4 hours, whereas in the experimental group in which yolk antibody was administered at a concentration of 1 mg or 5 mg per kg of body weight, respectively. At 30 minutes, 9.6 mg / dL and 7.8 mg / dL increased, respectively, which showed 9% and 26% inhibition of blood glucose increase compared to the control group. At 4 hours, blood glucose increase was 19.3 mg / dL and 12.4 mg / dL, showing 19% and 48% inhibitory effect compared to the control group (FIG. 8).
이로부터 본 발명에 따라 제조된 난황항체가 농도 의존적 양상으로 생체 내 당 흡수를 효과적으로 억제함을 확인하였다.From this, it was confirmed that the yolk antibody prepared according to the present invention effectively inhibits the absorption of glucose in vivo in a concentration-dependent manner.
<제제예 1> 약학적 제제의 제조Preparation Example 1 Preparation of Pharmaceutical Formulation
다음의 성분들을 혼합하여 경질 젤라틴 캅셀에 충진함으로써 캅셀제를 제조하였다:Capsules were prepared by mixing the following ingredients to fill hard gelatine capsules:
양 (㎎/캅셀)Volume (mg / capsule)
활성 성분 (실시예 1의 난황항체) 20Active Ingredients (An yolk Antibody of Example 1) 20
건조 전분 160Dry starch 160
마그네슘 스테아레이트 20Magnesium Stearate 20
총 200 ㎎Total 200 mg
<제제예 2> 난황항체를 포함하는 기능성 식품의 제조Preparation Example 2 Preparation of Functional Food Containing Egg Yolk Antibody
본 발명의 난황항체를 포함하는 기능성 식품들을 하기와 같이 제조하였다.Functional foods comprising the yolk antibody of the present invention were prepared as follows.
(1) 유제품 (dairy products)의 제조(1) Manufacture of dairy products
난황항체를 우유에 5 중량%의 양으로 첨가하고 이 우유를 이용하여 버터 및 아이스크림과 같은 다양한 유제품을 제조하였다.Egg yolk antibody was added to the milk in an amount of 5% by weight and milk was used to prepare various dairy products such as butter and ice cream.
(2) 혼합 음료의 제조(2) Preparation of Mixed Drinks
난황항체 1 g을 토마토, 당근, 사과 또는 포도 쥬스 1,000 ㎖에 가하여 건강 증진용 혼합 음료를 수득하였다.1 g of egg yolk antibody was added to 1,000 ml of tomato, carrot, apple or grape juice to obtain a mixed beverage for health promotion.
상기에서 살펴본 바와 같이, 본 발명에 따라 산란계로부터 생산된 수크라아제와 말타아제에 대한 난황항체는 산란계를 이용하여 안전하게 대량으로 생산이 가능하여 매우 경제적일 뿐만 아니라 다른 필수적인 무기이온 및 단백질 등의 흡수 저해 없이 탄수화물의 흡수만을 효과적으로 저해함으로써 비만 및 당뇨 질환의 개선 및 치료용 조성물로 유용하게 사용될 수 있다.As described above, egg yolk antibodies to sucrase and maltase produced from a laying hen can be produced in large quantities safely using a laying hen, which is very economical and inhibits absorption of other essential inorganic ions and proteins. By effectively inhibiting only the absorption of carbohydrates can be usefully used as a composition for the improvement and treatment of obesity and diabetes diseases.
Claims (8)
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| KR10-2001-0059027A KR100435829B1 (en) | 2001-09-24 | 2001-09-24 | METHOD FOR PRODUCING IgY AGAINST SUCRASE AND MALTASE AND COMPOSITIONS CONTAINING SAME FOR INHIBITING CARBOHYDRATE UPTAKE |
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| KR20050121250A (en) * | 2003-04-10 | 2005-12-26 | 겐 코오포레이션 | Antiobestic agent using hen's egg antibody against digestive enzymes |
| CN101792750A (en) * | 2010-03-03 | 2010-08-04 | 珠海市英平生物科技有限公司 | Yolk antibody for resisting activity of alpha-glucosidase and antigen, preparation method and application thereof |
| CN102908619A (en) * | 2011-08-04 | 2013-02-06 | 广州格拉姆生物科技有限公司 | Preparation method of egg yolk antibody injection for treating porcine respiratory syndrome |
| CN102908620A (en) * | 2011-08-04 | 2013-02-06 | 广州格拉姆生物科技有限公司 | Preparation method of egg yolk antibody injection for treating piglet diarrhea |
| US10538593B2 (en) | 2013-12-02 | 2020-01-21 | Ostrich Pharma Kk | Method for manufacturing digestive enzyme antibody and egg having same, and for manufacturing processed product containing egg as ingredient thereof and composition including antibody |
| WO2015083374A1 (en) * | 2013-12-02 | 2015-06-11 | オーストリッチファーマ株式会社 | Method for manufacturing digestive enzyme antibody and egg having same, and for manufacturing processed product containing egg as ingredient thereof and composition including antibody |
Citations (5)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| KR930001925A (en) * | 1991-07-08 | 1993-02-22 | 스무라 가즈오 | Sucrase Inhibition Method |
| JP2000186044A (en) * | 1998-12-22 | 2000-07-04 | Showa Sangyo Co Ltd | Carbohydrate decomposing enzyme inhibitor and food or medicine containing the same |
| KR20010056229A (en) * | 1999-12-08 | 2001-07-04 | 박관화 | Anti-obese compound with hypoglycemic activity and prepartion method thereof |
| KR20030014954A (en) * | 2001-08-13 | 2003-02-20 | 최태부 | A method for producing diet and blood glucose regulating foods using antibody against enzymes included in extracts derived from the mucosa of small intestine |
| KR20030017260A (en) * | 2001-08-24 | 2003-03-03 | 최태부 | A method for producing eggs for regulating diet and blood glucose, containing antibody against enzymes included in extracts derived from the mucosa of small intestine |
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Patent Citations (5)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| KR930001925A (en) * | 1991-07-08 | 1993-02-22 | 스무라 가즈오 | Sucrase Inhibition Method |
| JP2000186044A (en) * | 1998-12-22 | 2000-07-04 | Showa Sangyo Co Ltd | Carbohydrate decomposing enzyme inhibitor and food or medicine containing the same |
| KR20010056229A (en) * | 1999-12-08 | 2001-07-04 | 박관화 | Anti-obese compound with hypoglycemic activity and prepartion method thereof |
| KR20030014954A (en) * | 2001-08-13 | 2003-02-20 | 최태부 | A method for producing diet and blood glucose regulating foods using antibody against enzymes included in extracts derived from the mucosa of small intestine |
| KR20030017260A (en) * | 2001-08-24 | 2003-03-03 | 최태부 | A method for producing eggs for regulating diet and blood glucose, containing antibody against enzymes included in extracts derived from the mucosa of small intestine |
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