JP2006083089A - Interferon production enhancing agent and food and drink - Google Patents

Abstract

<P>PROBLEM TO BE SOLVED: To provide an interferon-α production enhancing agent and/or an interferon-β production enhancing agent each of which contains orally ingestible lactoferrin as an active ingredient. <P>SOLUTION: What is provided is: an interferon-α production enhancing agent and/or an interferon-β production enhancing agent in mammals including human containing lactoferrin as an active ingredient; a food and drink containing the interferon-α production enhancing agent and/or the interferon-β production enhancing agent; and a food and drink containing lactoferrin and having an annexed indication that it is used for enhancing the production of interferon-α and/or interferon-β. <P>COPYRIGHT: (C)2006,JPO&NCIPI

Description

  The present invention comprises an interferon-α production enhancer and an interferon-β production enhancer having an effect of antiviral, antitumor, cell growth suppression, immunomodulating action, and the like containing lactoferrin as an active ingredient, and the same. It relates to food and drink.

  Lactoferrin (LF) has been reported to have various immunostimulatory actions. In particular, in animal experiments of various pathological models, oral administration of bovine lactoferrin exerts a pathological condition improving effect, and it is explained that these are brought about through the immunostimulatory action of bovine lactoferrin. Among the immunostimulatory effects of bovine lactoferrin, there are several that show enhanced production of interferon (IFN) -γ. IFN-γ is a factor that plays a central role in the regulation of cellular immunity, and its production is induced by cytokines such as interleukin-12 (IL-12) and interleukin-18 (IL-18).

  Interferon is roughly classified into type I and type II, but IFN-γ is known as the only type II interferon. On the other hand, IFN-α, -β, -κ, -ω, -τ, limitin, etc. belong to type I interferons, and 14 subtypes have been reported for IFN-α. ing. The type I INF gene is encoded on the 4th chromosome of the mouse and the 9th chromosome of the human, and the type II INF gene is encoded on the 10th chromosome of the mouse and the 12th chromosome of the human. Furthermore, there is no molecular homology in both type I and type II, and type II is acid-stable, whereas type II is acid-labile.

  Both type I and type II IFNs have antiviral, antitumor, cell growth suppression, immunomodulating actions, etc., but the action mechanism is different for all effects. IFN-α and IFN-β transmit signals to cells via the common receptors IFNAR1 and IFNAR2c, and IFN-γ transmits signals to cells via IFNGR1 and IFNGR2.

  For example, with respect to antiviral activity, IFN-α and IFN-β suppresses viral growth by increasing the expression of PKR (dsRNA-dependent protein kinase) or Mx protein in infected cells, whereas IFN-γ is the NOS of macrophages. It exerts antiviral action by increasing the expression of (nitric oxide synthase).

  The main production cells of IFN-γ are T cells and macrophages. Production is induced by IL-12, IL-18, and IFN-γ itself, and cytotoxic T cells, NK cells, and macrophages responsible for cellular immunity are Activate.

  On the other hand, IFN-α and IFN-β are produced in macrophages, dendritic cells, and epithelial cells, or are produced by stimulation of microorganisms and viruses to activate NK cells and serve as an initial defense mechanism against these infections. In addition to acting, it induces the production of cellular immunity by inducing IFN-α production from NK cells.

IFN-α is currently approved as the only treatment for chronic hepatitis C. IFN-α and IFN-β are multiple sclerosis, psoriasis, hepatocellular carcinoma, melanoma, SARS (Severe Acute Respiratory Syndrome), demyelinating multiple radiculitis (Guillan-Barre Syndrome) has been reported to have a therapeutic effect, and an antiviral effect in a wider spectrum has also been reported (Non-patent Document 1). In addition, it has been clarified that IFN-β is an essential factor for maintaining a normal balance of bone remodeling (Non-patent Document 2).
Although it is an interferon having various effects as described above, clinically used IFN-α has been reported to cause side effects when administered in large quantities, and the administration method is limited to intravenous administration. .

Lactoferrin is known to enhance the therapeutic effect of IFN-α on patients with chronic hepatitis C (Patent Document 1). In addition, lactoferrin is disclosed to have an effect of inhibiting hepatitis B virus hepatocyte infection (Patent Document 2) and an effect of inhibiting hepatitis C virus hepatocyte infection (Patent Document 3), respectively. ing.
Furthermore, an IFN-γ production enhancer composition for mammals including humans containing lactoferrin or a hydrolyzate thereof and ceramides is disclosed (Patent Document 4).
On the other hand, the effect of inducing or enhancing the production of IFN-α and IFN-β having different classification and structure from IFN-γ by lactoferrin has not been reported so far.

International Publication No. 2002/043752 Pamphlet International Publication No. 2002/043753 Pamphlet JP 2002-332242 A International Publication No. 01/051079 Pamphlet Cytokine therapy, Fumitaka Hisahi, Nankodo, 1992, p. 89-97 Nature, 416, 2002, p. 744-749

  Patients who have the same effect as type I interferon and expect to exhibit the effect by oral ingestion, or diseases outside the indication of IFN-α preparation, such as multiple sclerosis, hepatocellular carcinoma, melanoma Use an IFN-α preparation that has many side effects and restricts the administration method for patients who expect therapeutic effects against the above, or when it is supposed to be used prophylactically rather than therapeutically. Was difficult.

  The invention of Patent Document 1 discloses that bovine lactoferrin enhances the therapeutic effect of IFN therapy based on IFN-α-like activity for patients with chronic hepatitis C, but IFN-α itself There was no mention of inducing the production of. Similarly, in Patent Document 2 and Patent Document 3, although the anti-hepatitis virus effect by lactoferrin has been confirmed, there has been no description or suggestion of inducing or enhancing interferon itself.

  Patent Document 4 discloses the effect of enhancing IFN-γ production by lactoferrin and ceramides, but it does not describe the effect of enhancing IFN-α and IFN-β, which are different in type and structure from IFN-γ. The problem of treatment required for patients requiring IFN-α and IFN-β formulations, and problems that can only be solved with IFN-α and IFN-β, remained. .

  In view of the above problems, the present inventors have searched for useful substances that have almost no side effects, high safety, and can be substituted for IFN-α preparations. As a result, by ingesting bovine lactoferrin, IFN- It was found that not only α but also IFN-β was remarkably induced to increase the expression of IFN-α and IFN-β in Peyer's patch, an intestinal lymphoid tissue, and the present invention was completed. . In particular, the effect of enhancing the production of IFN-β by lactoferrin is not described at all in the cited document, and is an effect found for the first time by the present invention.

  This is useful for diseases for which IFN-α and / or IFN-β has not been clinically applied, and has fewer side effects for drug treatment for patients who need to directly administer IFN-α preparations. Multiple sclerosis, psoriasis, hepatocellular carcinoma, melanoma, SARS (Severe Acute Respiratory Syndrome), multiple demyelination due to lactoferrin, which has not been known in the past because it can also be used as an adjuvant They have discovered a novel medicinal use as a therapeutic adjuvant for radiculitis (Guillan-Barre syndrome) and the like, or as a therapeutic or prophylactic agent for various diseases and complications caused by the proliferation of cancer cells and the like.

  Furthermore, IFN-α and IFN-β are known to enhance the activity of NK cells and are used in treatment and prevention with NK cells activated with interferon, so-called IFNANK therapy (IFN activated NK cells). Thus, the present invention has also found a novel pharmaceutical use with lactoferrin, which has not been known so far, in that it can be used as an adjuvant for IFNANK therapy.

  INDUSTRIAL APPLICABILITY The present invention is useful as an alternative preparation of an IFN-α preparation for diseases that are not clinically applied as an interferon preparation, and can be orally ingested and / or an interferon-β enhancer. The first object is to provide a production enhancer.

  Furthermore, the present invention provides a food or drink containing an interferon-α production enhancer and / or an interferon-β production enhancer containing lactoferrin as an active ingredient, or lactoferrin, and producing interferon-α and / or interferon-β. A second object of the present invention is to provide a food or drink with a label indicating that it has an enhancing action and is used for enhancing production of interferon-α and / or interferon-β. Yes.

  The first invention of the present invention that solves the above-mentioned problems is an interferon-α production enhancer containing lactoferrin as an active ingredient, wherein the lactoferrin is from the group consisting of a metal saturated type, a metal partially saturated type, and an apo type It is a preferred embodiment that it is one or a mixture of two or more selected.

  2nd invention of this invention which solves the said subject is food-drinks formed by containing the interferon-alpha production enhancer of said 1st invention.

  A third invention of the present invention that solves the above-mentioned problems is characterized in that it contains lactoferrin and has an interferon-α production enhancing action, and is used for enhancing interferon-α production. It is a food or drink with a display.

  A fourth invention of the present invention that solves the above-mentioned problems is an interferon-β production enhancer containing lactoferrin as an active ingredient, wherein the lactoferrin is from the group consisting of a metal saturated type, a metal partially saturated type, and an apo type It is a preferred embodiment that it is one or a mixture of two or more selected.

  A fifth invention of the present invention that solves the above-mentioned problems is a food or drink comprising the interferon-β production enhancer of the fourth invention.

  A sixth invention of the present invention that solves the above-mentioned problems is characterized in that it contains lactoferrin and has an interferon-β production enhancing action, and is used for enhancing interferon-β production. It is a food or drink with a display.

  The interferon production-enhancing agent and food and drink of the present invention are suitable for diseases that have not been clinically applied to IFN-α and / or IFN-β by enhancing production of IFN-α and IFN-β induced by oral administration or ingestion. For patients who need to administer the IFN-α preparation directly, they can also be used as adjuvants with few side effects for drug treatment.

  In addition, multiple sclerosis, psoriasis, hepatocellular carcinoma, melanoma, SARS (Severe Acute Respiratory Syndrome), myelin exfoliative multiple, which are known to have therapeutic effects by IFN-α and IFN-β Treatment aids for radiculitis (Guillan-Barre syndrome) and cancer cells (myeloma, non-Hodgkin lymphoma, malignant lymphoma, breast cancer, osteosarcoma, melanoma, oral papilloma, acute leukemia, etc.) and viruses (herpes simplex virus) , Cytomegalovirus, SARS virus, and the like) and is useful as a therapeutic or prophylactic agent for various diseases and complications resulting from the growth.

  Furthermore, IFN-α and IFN-β are known to enhance the activity of NK cells and are used in treatment and prevention with NK cells activated with interferon, so-called IFNANK therapy (IFN activated NK cells). Therefore, the present invention can also be used as an adjuvant for IFNANK therapy.

  Further, since the gene expression of IFN-β is enhanced by lactoferrin, it is considered useful as a therapeutic agent or adjuvant in gene therapy based on the IFN-β gene.

  Next, a preferred embodiment of the present invention will be described in detail. However, the present invention is not limited to the following preferred embodiments, and can be freely changed within the scope of the present invention. In the present specification, the percentage is expressed by mass unless otherwise specified.

  The present invention relates to interferon (IFN) -α production enhancer and / or interferon (IFN) -β production enhancer (in the present invention, interferon-α production enhancer and / or interferon-β production) containing lactoferrin as an active ingredient. The enhancer may be abbreviated as “interferon (IFN) production enhancer”.)

  The lactoferrin used in the present invention is commercially available lactoferrin, mammals (eg, humans, cows, goats, sheep, horses, etc.) colostrum, transitional milk, regular milk, end milk, or processed products of these milks. Non-fat milk, whey, etc. as raw materials can be used, and for example, lactoferrin obtained by separation from the raw materials by a conventional method such as ion exchange chromatography can be used. Among them, it is preferable to use commercially available lactoferrin (for example, manufactured by Morinaga Milk Industry Co., Ltd.) manufactured on an industrial scale. Furthermore, it is also possible to use lactoferrin produced in microorganisms, animal cells, transgenic animals, etc. by genetic engineering techniques.

  In the effect of the interferon production enhancer of the present invention, the metal content in lactoferrin is not particularly limited. In the present invention, apo-type lactoferrin obtained by removing iron from lactoferrin with hydrochloric acid, citric acid or the like; From a group consisting of metal saturated lactoferrin in a state of 100% saturation obtained by chelating with a metal such as copper, zinc, manganese; and metal partially saturated lactoferrin in a state in which the metal is bound at various saturations of less than 100% Any one or a mixture of two or more selected can be used.

  The various lactoferrin mentioned above has an effect of enhancing production of IFN-α and / or IFN-β. Here, in the present invention, “enhanced production of IFN-α and / or IFN-β” refers to enhancing production of IFN-α and / or IFN-β in IFN-α and / or IFN-β producing cells. Means to induce production. Therefore, the IFN-α production enhancer and / or IFN-β production enhancer (IFN production enhancer) in the present invention is an IFN-α production inducer and / or an IFN-β production inducer (IFN production inducer). In other words, it is possible.

  In addition, cells (or organs) that enhance production of IFN-α and / or IFN-β upon stimulation with the IFN production enhancer of the present invention are leukocytes, NK cells, dendritic cells, fibroblasts, Peyer's patch tissue. (For example, Peyer's patches distributed on the small intestinal mucosa) and the like, and the IFN production enhancer of the present invention works effectively on the organs that produce the above cells and efficiently converts IFN-α and / or IFN-β. It is possible to produce well.

  The interferon production enhancer of the present invention is a prophylactic / therapeutic agent for diseases involving interferon, such as multiple sclerosis, psoriasis, melanoma, demyelinating multiple radiculitis (Guillan-Barre syndrome), or cancer cells. Growth and metastasis inhibitors and viruses (herpes simplex virus, cytomegalovirus, SARS, etc.) (myeloma, non-Hodgkin lymphoma, malignant lymphoma, breast cancer, hepatocellular carcinoma, osteosarcoma, melanoma, oral papilloma, acute leukemia, etc.) (Severe Acute Respiratory Syndrome: Severe Acute Respiratory Syndrome) virus). Furthermore, the interferon production-enhancing agent of the present invention includes cancer cells (myeloma, non-Hodgkin lymphoma, malignant lymphoma, breast cancer, osteosarcoma, melanoma, oral papilloma, acute leukemia, etc.) and viruses (herpes simplex virus, cytomegalovirus). It is possible to treat or prevent various diseases and complications resulting from the proliferation of SARS virus and the like, and to reduce the risk of these diseases and complications.

  The interferon production enhancer of the present invention may be used alone, but can also be used in combination with a known prophylactic / therapeutic agent for the disease or the viral growth inhibitor. By using in combination, the effect of preventing or treating the disease or the effect of inhibiting the growth of the virus can be enhanced. The prophylactic / therapeutic agent for the disease or the viral growth inhibitor used in combination may be contained as an active ingredient in the composition of the present invention, or a separate drug without being contained in the composition of the present invention. May be combined and commercialized.

  As a drug that can be used in combination with the interferon production enhancer of the present invention, in addition to known antiviral agents and antitumor agents, a factor generally called an interferon inducer, a drug containing this factor, a bacterial endotoxin Examples include bacteria, among others, synthetic or natural double-stranded nucleic acids (double-stranded RNA, poly IC, etc.), lipopolysaccharides, polysaccharides (β-glucan, etc.), anticancer agents such as taxol, defensin, Heat shock proteins, fibrinogen, hyaluronic acid degradation products and the like are preferable. In addition, when these interferon inducers are used in combination, it is also possible to produce (manufacture) interferon on an industrial scale.

  The interferon production enhancer of the present invention can be administered to mammals including humans orally or parenterally in combination with a pharmaceutically acceptable pharmaceutical carrier of lactoferrin. The dosage unit form of the preparation of the present invention is not particularly limited, and can be appropriately selected according to the purpose of treatment. Specifically, tablets, pills, powders, solutions, suspensions, emulsions, granules, capsules, syrups Examples include suppositories, suppositories, injections, ointments, patches, eye drops, nasal drops and the like. Additives such as excipients, binders, disintegrants, lubricants, stabilizers, flavoring agents, diluents, surfactants, solvents for injections, etc. that are commonly used as pharmaceutical carriers for pharmaceutical preparations. Can be used.

  The amount of lactoferrin contained in the preparation of the present invention is not particularly limited and may be appropriately selected. For example, all of them are usually 0.01 to 60% by mass, preferably 0.1 to 40% by mass in the preparation. Is good.

  The administration method of the preparation of the present invention is not particularly limited, and is determined according to various preparation forms, the patient's age, sex, other conditions, the degree of symptoms of the patient, and the like. The dosage of the active ingredient in the preparation of the present invention is appropriately selected depending on the usage, patient age, sex, disease severity, other conditions, and the like. Usually, the amount of lactoferrin as an active ingredient is 0.1 to 1000 mg / kg / day, preferably 0.6 to 600 mg / kg / day, particularly preferably 6 to 300 mg / kg / day. It can be administered once or several times a day.

  The food / beverage products containing the interferon production enhancer of the present invention can be produced by adding lactoferrin to foods or beverages, and can be taken orally. Drinks and beverages include soft drinks, carbonated drinks, nutritional drinks, fruit juice drinks, lactic acid bacteria drinks and other drinks (including concentrated concentrates and powders for adjustment of these drinks); ice creams such as ice cream, sorbets, shaved ice, etc .; , Chewing gum, candy, gum, chocolate, tablet confectionery, snack confectionery, biscuits, jelly, jam, cream, baked confectionery, etc .: dairy products such as processed milk, milk drinks, fermented milk, butter; bread; enteral nutrition And liquid foods, milk for childcare, sports drinks, and other functional foods.

  In the food and drink of the present invention, the amount of lactoferrin added is appropriately set depending on the form of the food or drink, but is 0.01 to 60% by mass, preferably 0.1 to 40% by mass in normal food or beverage. It may be added as follows.

  As a use in foods and drinks containing the interferon production enhancer of the present invention, it has an effect of enhancing production of interferon-α and / or interferon-β, and enhances production of interferon-α and / or interferon-β. Use, specifically, prevention / treatment of diseases involving interferon, such as multiple sclerosis, psoriasis, melanoma, demyelinating polyradiculitis (Guillan-Barre syndrome), or cancer cells ( Suppression of proliferation and metastasis of myeloma, non-Hodgkin lymphoma, malignant lymphoma, breast cancer, hepatocellular carcinoma, osteosarcoma, melanoma, oral papilloma, acute leukemia, etc., virus (herpes simplex virus, cytomegalovirus, SARS virus, etc.) ) Can be used for various purposes that utilize effects such as growth inhibition. Furthermore, foods and drinks containing the interferon production enhancer of the present invention include cancer cells (myeloma, non-Hodgkin lymphoma, malignant lymphoma, breast cancer, osteosarcoma, melanoma, oral papilloma, acute leukemia, etc.) and viruses (herpes simplex). Virus, cytomegalovirus, SARS virus, etc.) due to the growth of various diseases and complications, and the risk of these diseases and complications can be reduced.

  The food / beverage products containing the interferon production enhancer of the present invention have an interferon-α and / or interferon-β production enhancing action, and are capable of enhancing the production of interferon-α and / or interferon-β. Foods and beverages that are labeled for use, specifically diseases involving interferon, such as multiple sclerosis, psoriasis, melanoma, demyelinating multiple radiculitis (Guillan-Barre syndrome), etc. Prevention or treatment of cancer, suppression of proliferation and metastasis of cancer cells (myeloma, non-Hodgkin lymphoma, malignant lymphoma, breast cancer, hepatocellular carcinoma, osteosarcoma, melanoma, oral papilloma, acute leukemia, etc.), virus (herpes simplex As a food or drink displaying various uses such as growth suppression of viruses, cytomegalovirus, SARS virus, etc.) It is preferable to sales. For example, it is preferable to sell as “a food / beverage product for enhancing production of interferon containing lactoferrin”, “a food / beverage product containing lactoferrin displayed for enhancing production of interferon”, or the like. The interferon production enhancer of the present invention is a cancer cell (myeloma, non-Hodgkin lymphoma, malignant lymphoma, breast cancer, osteosarcoma, melanoma, oral papilloma, acute leukemia, etc.) or virus (herpes simplex virus, cytomegalovirus, Since it has an effect such as prevention of various diseases and complications caused by proliferation of SARS virus etc., the display for enhancing interferon production includes cancer cells (myeloma, non-Hodgkin lymphoma, malignant lymphoma, breast cancer, (Such as osteosarcoma, melanoma, oral papilloma, acute leukemia) and prevention of various diseases and complications caused by the growth of viruses (herpes simplex virus, cytomegalovirus, SARS virus, etc.) I think that. Therefore, the food and drink of the present invention include “cancer cells (myeloma, non-Hodgkin lymphoma, malignant lymphoma, breast cancer, osteosarcoma, melanoma, oral papilloma, acute leukemia, etc.) and viruses (herpes simplex virus, cytomegalovirus, “For prevention of various diseases and complications caused by the growth of SARS virus and the like”. In other words, the indication for enhancing interferon production includes such “cancer cells (myeloma, non-Hodgkin lymphoma, malignant lymphoma, breast cancer, osteosarcoma, melanoma, oral papilloma, acute leukemia, etc.) and viruses (herpes simplex). "Prevention of various diseases and complications caused by proliferation of viruses, cytomegalovirus, SARS virus, etc.)".

  Note that the terminology used for the above indications is “for enhancing interferon production” or “cancer cells (myeloma, non-Hodgkin lymphoma, malignant lymphoma, breast cancer, osteosarcoma, melanoma, oral papilloma, Acute leukemia, etc.) and viruses (herpes simplex virus, cytomegalovirus, SARS virus, etc.) are not limited to the phrase “for the prevention of various diseases and complications resulting from the growth of the virus”. Even if interferon production is enhanced, cancer cells (myeloma, non-Hodgkin lymphoma, malignant lymphoma, breast cancer, osteosarcoma, melanoma, oral papilloma, acute leukemia, etc.) and viruses (herpes simplex virus, cytomegalovirus, SARS) Any word representing the effect of preventing or preventing various diseases and complications resulting from the growth of viruses etc. is included in the scope of the present invention. Is it is needless to say. Such terms include, for example, increased interferon production or cancer cells (myeloma, non-Hodgkin lymphoma, malignant lymphoma, breast cancer, osteosarcoma, melanoma, oral papilloma, acute leukemia, etc.) It is also possible to make a display based on various uses for recognizing the effect of preventing various diseases and complications caused by the growth of viruses (herpes simplex virus, cytomegalovirus, SARS virus, etc.).

  The “display” means all acts for informing the consumer of the use, and if it is a display that can recall and analogize the use, the purpose of the display, the content of the display, the display Regardless of the target object / medium, etc., all fall under the “display” of the present invention. However, it is preferable to display in such an expression that the consumer can directly recognize the application. Specifically, the act of describing the above-mentioned use in the product or product packaging relating to the food or drink of the present invention, the product or product packaging describing the above-mentioned use is transferred, and displayed for delivery, transfer or delivery And importing, displaying advertisements on products, price lists or transaction documents for display or distribution, or describing the above uses in information containing these, electromagnetic (Internet, etc.) methods The act provided by can be exemplified.

  On the other hand, the display is preferably a display approved by the government or the like (for example, a display which is approved based on various systems determined by the government and is performed in a mode based on such approval). Display on advertising materials at sales sites such as catalogs, pamphlets, and POPs, and other documents is preferable.

  In addition, for example, indications such as health foods, functional foods, enteral nutrition foods, special-purpose foods, nutritional functional foods, quasi-drugs, and other indications approved by the Ministry of Health, Labor and Welfare, for example, , Foods for specified health use, and labeling approved under a similar system. Examples of the latter can include a display as a food for specified health use, a display as a condition specific food for specified health use, a display that affects the structure and function of the body, a display for reducing disease risk, etc. Speaking of the health promotion law enforcement regulations (April 30, 2003 Ministry of Health, Labor and Welfare Ordinance No. 86) labeling as food for specified health use (especially labeling the use of health), and similar The display can be listed as a typical example.

Next, the present invention will be described in detail with reference to test examples.
[Test Example 1]
This test was conducted to examine the expression of interferon-β by oral administration of lactoferrin at the gene level.

(1) Test method 27 7-week-old C57BL / 6 mice (purchased from Japan Charles River) were bred for 1 week, then divided into 3 groups of 9 mice per group, each of which was lactoferrin (LF) group, bovine Serum albumin (BSA) group and physiological saline (control) group were used. In mice in the LF group, 200 μl of bovine lactoferrin solution dissolved in physiological saline (manufactured by Otsuka Pharmaceutical Co., Ltd.) so that the dose of bovine lactoferrin (manufactured by Morinaga Milk Industry Co., Ltd.) is 300 mg / kg body weight, Used for 7 consecutive days. Similarly, in a BSA group of mice, 200 μl of BSA solution dissolved in physiological saline was used for 7 days using an oral sonde so that the dose of bovine serum albumin (manufactured by Sigma) was 300 mg / kg body weight. It was administered continuously. In addition, 200 μl of physiological saline was administered to the control group mice continuously for 7 days using an oral sonde. After administration, Peyer's patch tissue scattered in the small intestine of mice is collected, and total RNA is extracted from Peyer's patch tissue using a reagent for total RNA extraction (product name: RNA-Bee ^TM Reagent, manufactured by Cosmo Bio). Extraction, primer (sense strand sequence: TTCCTGCTGTGCTTCTCCAC, antisense strand sequence: GATTCACTACCAGTCCCAGAGTC, A: adenine, G: guanine, T: thymine, C: cytosine) and PCR reagent (product) Name: iQ SYBR Green Supermix [Catalog Number: 170-8885], Bio-Rad) was used to perform real-time PCR using a thermal cycler (Bio-Rad).

(2) Test results The results of this test are as shown in Table 1. From Table 1, it was found that the mRNA expression level of IFN-β in the LF administration group was remarkably increased (about 2 times) as compared with the control group. In the BSA group, an increase in IFN-β mRNA expression level was not confirmed.

[Test Example 2]
This test was conducted to examine the production of interferon-α by oral administration of lactoferrin by Western blotting.

(1) Preparation of samples About 7 7-week-old C57BL / 6 mice (purchased from Nippon Charles River), after acclimation and breeding for 1 week, each group was divided into 2 groups of 2 mice, each of which was a lactoferrin (LF) group, Saline (control) group. In mice in the LF group, 200 μl of bovine lactoferrin solution dissolved in physiological saline (manufactured by Otsuka Pharmaceutical Co., Ltd.) so that the dose of bovine lactoferrin (manufactured by Morinaga Milk Industry Co., Ltd.) is 300 mg / kg body weight, Used for 7 consecutive days. Similarly, 200 μl of physiological saline was administered to the control group mice for 7 consecutive days using an oral sonde. After completion of the administration, Peyer's patch tissue scattered in the small intestine of each mouse of each administration group was collected, and the collected Peyer's patch tissue was put into a hand homogenizer, and further homogenized reagent [9.1 mM disodium hydrogen phosphate (Japanese Phosphate buffer solution pH 7.4 containing 1.7 mM sodium dihydrogen phosphate (Wako Pure Chemical Industries) and 150 mM sodium chloride (Wako Pure Chemical Industries), and final concentration 1 % NP-40 (manufactured by Sigma), final concentration 0.5% sodium deoxycholate (manufactured by Wako Pure Chemical Industries, Ltd.), final concentration 0.1% sodium dodecyl sulfate (SDS: manufactured by Wako Pure Chemical Industries, Ltd.), final 100 μg / ml (p-amidinophenyl) methanesulfonyl fluoride hydrochloride (manufactured by Wako Pure Chemical Industries, Ltd.)] 0.5 ml each was added and homogenized . Thereafter, the entire homogenized solution is transferred to a microtube, centrifuged at 12,000 rpm at 4 ° C. for 10 minutes to recover the supernatant, and then centrifuged again under the same conditions to recover the supernatant. Sample solutions for each administration group were prepared.

(2) Test method The protein concentration of each sample solution was quantified, and an amount corresponding to 30 μg was taken as an electrophoresis sample. Recombinant IFN-α (rIFN-α: manufactured by PBL Biomedical Laboratories, catalog number 12100) -1) was used as a positive control sample, and each was subjected to SDS polyacrylamide gel electrophoresis. After electrophoresis, the proteins separated in the gel were transferred to a polyvinylidene difluoride (PVDF) membrane filter (Amersham Pharmacia Biotech), and the PVDF membrane was blocked with Block Ace (Snow Brand Milk Products). An IFN-α anti-rabbit antibody (PBL Biomedical Laboratories, catalog number 32100-1) solution was reacted as a primary antibody. Furthermore, an anti-rabbit IgG-anti-goat antibody (manufactured by Cappel, catalog number 55676) was reacted as a secondary antibody, and the PVDF membrane was immersed in a reaction solution for detection of ECL-Plus Western blotting (manufactured by Amersham Pharmacia Biotech) for 5 minutes. . Thereafter, hyperfilm ECL (manufactured by Amersham Pharmacia Biotech) was exposed using a PVDF membrane, and the density of the exposed band (IFN-α) was quantified with a densitometer.

(3) Test results The results of this test are as shown in FIG. FIG. 1 shows Western blotting, and Table 2 shows the results of quantifying the density of the exposed band (IFN-α) with a densitometer. As a result, in the lactoferrin group, the amount of IFN-α produced in the Peyer's patch of the mouse increased about 16 times compared to the control group. Therefore, administration of lactoferrin markedly enhanced the IFN-α production. It was found that

[Test Example 3]
This test was performed to examine interferon-β production by oral administration of lactoferrin by Western blotting.

(1) Preparation of Samples Seven 7-week-old C57BL / 6 mice (purchased from Japan Charles River) were acclimated for 1 week, and then each of them was lactoferrin (LF) group, 3 physiological saline (control) group 2 The mice were divided into two groups of bovine serum albumin (BSA) groups. In mice in the LF group, 200 μl of bovine lactoferrin solution dissolved in physiological saline (manufactured by Otsuka Pharmaceutical Co., Ltd.) so that the dose of bovine lactoferrin (manufactured by Morinaga Milk Industry Co., Ltd.) is 300 mg / kg body weight, Used for 7 consecutive days. In the BSA group of mice, 200 μl of BSA solution dissolved in physiological saline was continuously used for 7 days using an oral sonde so that the dose of bovine serum albumin (manufactured by Sigma) was 300 mg / kg body weight. Administered. In addition, 200 μl of physiological saline was administered to the control group mice continuously for 7 days using an oral sonde. After the administration was completed, Peyer's patch tissue scattered in the small intestine of each mouse in each administration group was collected, and a sample solution for each administration group was prepared in the same manner as in Test Example 2.

(2) Test method The protein concentration of each sample solution is quantified, and an amount corresponding to 30 μg is taken as an electrophoresis sample, and recombinant IFN-β (rIFN-β: manufactured by PBL Biomedical Laboratories, catalog number 12400) -1) was used as a positive control sample, and each was subjected to SDS polyacrylamide gel electrophoresis. After electrophoresis, the proteins separated in the gel were transferred to a polyvinylidene difluoride (PVDF) membrane filter (Amersham Pharmacia Biotech), and the PVDF membrane was blocked with Block Ace (Snow Brand Milk Products). An IFN-β anti-rabbit antibody (PBL Biomedical Laboratories, catalog number 32400-1) solution was reacted as a primary antibody. Furthermore, an anti-rabbit IgG-anti-goat antibody (manufactured by Cappel, catalog number 55676) was reacted as a secondary antibody, and the PVDF membrane was immersed in a reaction solution for detection of ECL-Plus Western blotting (manufactured by Amersham Pharmacia Biotech) for 5 minutes. . Thereafter, hyperfilm ECL (manufactured by Amersham Pharmacia Biotech) was exposed using a PVDF membrane, and the density of the exposed band (IFN-β) was quantified with a densitometer.

(3) Test results The results of this test are as shown in FIG. FIG. 2 shows Western blotting, and Table 3 shows the result of quantifying the density of the exposed band (IFN-β) with a densitometer. As a result, in the lactoferrin group, the amount of IFN-β produced in the Peyer's patch of the mouse was about 4.4 times, about 1.8 times, and about 11 times, respectively, compared with the control group. Since IFN-β increased, it was found that administration of lactoferrin significantly exerted an IFN-β production enhancing effect. In the BSA group, no IFN-β production enhancing effect was confirmed.

  EXAMPLES Next, although an Example is shown and this invention is demonstrated further in detail, this invention is not limited to a following example.

(Preparation of tablets containing lactoferrin)
A tablet interferon production enhancer having the following composition was produced by the following method.
Bovine lactoferrin (Morinaga Milk Industry Co., Ltd.) 40.0 (%)
Lactose (Morinaga Milk Industry Co., Ltd.) 18.5
Corn starch (Nisshin Flour Milling) 30.7
Magnesium stearate (manufactured by Taihei Chemical Industry Co., Ltd.) 1.4
Carboxymethylcellulose calcium (Gotoku Pharmaceutical Co., Ltd.) 9.4
To the mixture of bovine lactoferrin, lactose, corn starch and carboxymethylcellulose calcium, knead uniformly while adding sterilized purified water as appropriate, dry at 50 ° C for 3 hours, and add magnesium stearate to the resulting dried product And mixed and compressed into tablets by a conventional method.

(Preparation of encapsulated lactoferrin)
A 50 mesh sieve (Yamato) was prepared by using 600 g of lactose (manufactured by Wako Pure Chemical Industries, Ltd.), 400 g of corn starch (manufactured by Nisshin Flour Milling Co., Ltd.), 400 g of crystalline cellulose (manufactured by Wako Pure Chemical Industries, Ltd.) and 600 g of bovine lactoferrin (manufactured by Morinaga Milk Industry Co., Ltd.). Sifted into a polyethylene bag with a thickness of 0.5 mm, mixed by inversion, and the powder was encapsulated using a fully automatic capsule filling machine (Cesere Pedini, press type) (Elanco Japan) No.1 gelatin capsule, Op.Yellow No.6 Body, empty weight is 75mg) filled with 275mg content, capsule containing 82mg bovine lactoferrin and having an effect of enhancing production of interferon-α and / or interferon-β 7,000 pieces were obtained.

(Preparation of beverage with added bovine lactoferrin)
90 g of skim milk powder (Morinaga Milk Industry Co., Ltd.) is dissolved in 800 ml of hot water at 50 ° C., 30 g of sugar (Nisshin Sugar Co., Ltd.), 14 g of instant coffee powder (Nestlé Co., Ltd.), 2 g of caramel (made by Showa Kako Co., Ltd.), and coffee 0.01 g of flavor (manufactured by Sanei Chemical Co., Ltd.) is added and dissolved sequentially with stirring, cooled to 10 ° C., 1 g of bovine lactoferrin (manufactured by Morinaga Milk Industry Co., Ltd.) is added, and contains about 0.1% bovine lactoferrin. A milk drink having an effect of enhancing production of interferon-α and / or interferon-β was prepared.

(Preparation of enteral nutritional powder supplemented with bovine lactoferrin)
10.8 kg of whey protein enzyme degradation product (manufactured by Morinaga Milk Industry Co., Ltd.), 36 kg of dextrin (manufactured by Showa Sangyo Co., Ltd.), and a small amount of water-soluble vitamins and minerals were dissolved in 200 kg of water, and an aqueous phase was prepared in the tank. Separately, soybean salad oil (manufactured by Taiyo Yushi Co., Ltd.) 3 kg, palm oil (manufactured by Taiyo Yushi Co., Ltd.) 8.5 kg, safflower oil (manufactured by Taiyo Yufu Co., Ltd.) 2.5 kg, lecithin (manufactured by Ajinomoto Co., Inc.) 0.2 kg, An oil phase was prepared by mixing and dissolving 0.2 kg of a fatty acid monoglyceride (manufactured by Kao Corporation) and a small amount of a fat-soluble vitamin. The oil phase was added to the aqueous phase in the tank, stirred and mixed, then heated to 70 ° C. and further homogenized with a homogenizer at a pressure of 14.7 MPa. Then, after sterilizing at 90 ° C. for 10 minutes, it was concentrated and spray-dried to prepare about 59 kg of intermediate product powder. To 50 kg of this intermediate product powder, 6.8 kg of sucrose (manufactured by Hokuren Co., Ltd.), 167 g of amino acid mixed powder (manufactured by Ajinomoto Co., Inc.), and 60 g of bovine lactoferrin (manufactured by Morinaga Milk Industry Co., Ltd.) are added and mixed uniformly to obtain bovine lactoferrin. About 57 kg of enteral nutrition food powder having an effect of enhancing production of interferon-α and / or interferon-β containing about 0.1% was produced.

  The interferon production-enhancing agent and food and drink of the present invention are suitable for diseases that have not been clinically applied to IFN-α and / or IFN-β by enhancing production of IFN-α and IFN-β induced by oral administration or ingestion. For patients who need to administer the IFN-α preparation directly, they can also be used as adjuvants with few side effects for drug treatment.

  In addition, multiple sclerosis, psoriasis, hepatocellular carcinoma, melanoma, SARS (Severe Acute Respiratory Syndrome), myelin exfoliative multiple, which are known to have therapeutic effects by IFN-α and IFN-β Treatment aids for radiculitis (Guillan-Barre syndrome) and cancer cells (myeloma, non-Hodgkin lymphoma, malignant lymphoma, breast cancer, osteosarcoma, melanoma, oral papilloma, acute leukemia, etc.) and viruses (herpes simplex virus) , Cytomegalovirus, SARS virus, and the like) and is useful as a therapeutic or prophylactic agent for various diseases and complications resulting from the growth.

It is the western blotting which measured the interferon- (alpha) produced with the Peyer's board of a mouse | mouth. It is the western blotting which measured the interferon-beta produced with the Peyer's board of a mouse | mouth.

Claims (8)

An interferon-α production enhancer containing lactoferrin as an active ingredient. The interferon-α production enhancer according to claim 1, wherein the lactoferrin is one or a mixture of two or more selected from the group consisting of a metal saturated type, a metal partially saturated type, and an apo type. A food or drink comprising the interferon-α production enhancer according to claim 1 or 2. A food or beverage product comprising lactoferrin and having an interferon-α production enhancing action, and having a label indicating that it is used for enhancing interferon-α production. An interferon-beta production enhancer containing lactoferrin as an active ingredient. The interferon-β production enhancer according to claim 5, wherein the lactoferrin is one or a mixture of two or more selected from the group consisting of a metal saturated type, a metal partially saturated type, and an apo type. A food or drink comprising the interferon-β production enhancer according to claim 5 or 6. A food or beverage product comprising lactoferrin and having an interferon-β production enhancing action and having a label indicating that it is used for enhancing interferon-β production.

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