KR101646009B1 - A composition comprising oroxylin A compound for preventing and treating the viral disease caused by enterovirus - Google Patents
A composition comprising oroxylin A compound for preventing and treating the viral disease caused by enterovirus Download PDFInfo
- Publication number
- KR101646009B1 KR101646009B1 KR1020150165528A KR20150165528A KR101646009B1 KR 101646009 B1 KR101646009 B1 KR 101646009B1 KR 1020150165528 A KR1020150165528 A KR 1020150165528A KR 20150165528 A KR20150165528 A KR 20150165528A KR 101646009 B1 KR101646009 B1 KR 101646009B1
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- KR
- South Korea
- Prior art keywords
- oroxylin
- enterovirus
- extract
- cvb3
- compound
- Prior art date
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Abstract
본 발명은 항엔테로바이러스를 갖는 조성물에 관한 것으로, 상세하게는 황금의 추출물 또는 이로부터 분리된 화합물을 유효성분으로 함유하는 본 발명의 조성물은(1) 베로(vero) 세포에서의 세포독성 및 EV71, CVB3, CVA16의 항바이러스 활성실험, 세포병변 억제실험; (2) EV71에 대한 항바이러스 활성을 확인하기 위한 enterovirus 71의 VP단백질에 대한 Western blot 분석법; (3) replicon system(pRibFluc-EV71)을 이용한 Replicon 분석법을 통한 항바이러스 활성 메카니즘 분석실험; (4) BALB/c 마우스를 이용한 CVB3 바이러스에 대한 항바이러스 활성 측정을 위한 in vivo 동물실험 등의 광범위한 시험관내 실험(in vitro test) 및 생체내 동물실험(in vivo test)를 통하여, 본 발명의 상기 시료들이 강력한 항 엔테로바이러스 활성을 나타냄을 확인함으로, 상기 조성물을 엔테로 바이러스에 기인한 질환의 예방 및 치료용 약학조성물 또는 건강기능식품으로 유용하게 이용될 수 있다.The present invention relates to a composition having an anti-enterovirus, and more particularly, to a composition comprising an extract of gold or a compound isolated therefrom as an active ingredient, which comprises (1) cytotoxicity in vero cells and EV71 , CVB3, CVA16, and cytopathic inhibition experiments; (2) Western blot analysis of the VP protein of enterovirus 71 to confirm antiviral activity against EV71; (3) Analysis of antiviral activity mechanism through replicon analysis using replicon system (pRibFluc-EV71); (4) In vitro tests and in vivo tests in vivo, such as in vivo animal experiments for the determination of antiviral activity against CVB3 virus using BALB / c mice, By confirming that the samples exhibit strong anti-enterovirus activity, the composition can be usefully used as a pharmaceutical composition or health functional food for the prevention and treatment of diseases caused by enteroviruses.
Description
본 발명은 황금 추출물로부터 분리된 화합물을 유효성분으로 함유하는 엔테로 바이러스에 기인한 질환의 예방 및 치료용 약학 조성물 또는 건강기능식품에 관한 것이다.The present invention relates to a pharmaceutical composition or health functional food for the prevention and treatment of diseases caused by enteroviruses containing a compound isolated from a golden extract as an active ingredient.
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[문헌 69] van der Linden L, van der Schaar HM, Lanke KH, Neyts J, van Kuppeveld FJ. Differential effects of the putative GBF1 inhibitors Golgicide A and AG1478 on enterovirus replication. J Virol. 2010 Aug;84(15):7535-4269.[Literature 69] van der Linden L, van der Schaar HM, Lanke KH, Neyts J, van Kuppeveld FJ. Differential effects of the putative GBF1 inhibitors Golgicide A and AG1478 on enterovirus replication. J Virol. 2010 Aug; 84 (15): 7535-4269.
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엔테로바이러스(Enterovirus)는 27~30 nm 크기의 envelope를 갖지 않는 바이러스로써 정이십면체의 형태를 이루고, 현재까지 약 68여종 이상의 혈청형이 알려져 있다. 이것은 분류학적으로 Picornaviridae과의 Enterovirus속에 속하며, 이들 속에는 3가지 혈청형의 Poliovirus (PV: 1~3)와 23가지 혈청형의 Coxsackievirus A군 (CVA: 1~22, 24), 6가지 혈청형의 Coxsackievirus B군 (CVB: 1~6), 그리고 28가지 혈청형의 Echovirus군 (ECV: 1~7, 9, 11~21, 24~27, 29~33) 및 기타 Human Enterovirus (EV: 68~116)등으로 구성되어 있다 [1-4]. 그러나 최근 enterovirus 연구자들은 RdRp (RNA dependent RNA polymerase)유전자의 염기서열을 이용한 계통분석을 통하여 enterovirus 속을 HEV (Human Enterovirus) A~D의 유전자형으로 분류하기도 한다 [1,5]. HEV-A에는 11가지 혈청형의 CVA와 EV71이 속하며, HEV-B는 모든 CVB와 ECV, EV69, EV73 및 CVA9의 38가지 혈청형이 여기에 포함된다. HEV-C는 11가지의 CVA를 포함하며, 마지막으로 HEV-D에는 EV68과 EV70의 두 가지 혈청형만이 여기에 속한다 [6]. Enteroviruses are viruses that do not have an envelope of 27 to 30 nm in size. They form a true dodecahedron, and about 68 serotypes have been known to date. It belongs to the Enterovirus genus of Picornaviridae taxonomically. Three genotypes of poliovirus (PV: 1 ~ 3), 23 serotypes of Coxsackievirus A (CVA: 1 ~ 22, 24), six serotypes (ECV: 1 ~ 7, 9, 11 ~ 21, 24 ~ 27, 29 ~ 33) and other human enteroviruses (EV: 68 ~ 116 ) And the like [1-4]. However, recently, researchers enterovirus e nterovirus through the system analysis using the nucleotide sequence of RdRp (RNA dependent RNA polymerase) gene And genotypes of HEV (human enterovirus) A to D [1,5]. There are 11 serotypes of CVA and EV71 in HEV-A, and 38 serotypes of all CVB and ECV, EV69, EV73 and CVA9 in HEV-B. HEV-C contains 11 CVAs. Finally, HEV-D contains only two serotypes, EV68 and EV70 [6].
엔테로바이러스(Enterovirus)s의 게놈은 약 7.2~7.5kb 크기의 single stranded positive sense RNA의 형태를 갖는다. 그것은 하나의 ORF (open reading frame)와 5´및 3´말단에 단백질로 발현되지 않는 NCR (non-coding region)로 구성되어 있다. ORF는 하나의 polyprotein으로 발현되는데, 약 2,185개의 아미노산으로 이루어져 있다 [7]. 이 polyprotein은 바이러스의 단백질 분해효소에 의해서 여러 개의 다른 단백질로 나누어진다. 하나의 polyprotein은 P1, P2, P3로 구분되어 있는데, P1부분은 바이러스의 캡시드 단백질의 구성요소인 VP4, VP2, VP3, VP1을 순서대로 암호화 하고 있다. P2부분은 2Apro 단백질분해효소와 현재까지 기능이 정확하게 알려지지 않은 단백질을 암호화하고 있으며, P3부분은 VPg 단백질과 3Cpro 단백질분해효소 및 RdRp가 암호화되어 있다. VPg 단백질은 primer로써 3´쪽에 작용하여, negative sense strand 게놈 형성에 관여 한다 [8]. 5´NCR은 700~800 bp로 구성되어 있고, 매우 복잡한 2차 구조를 형성한다. 이러한 RNA의 2차 구조의 기능은 첫째로 RdRp에 의해서 positive sense RNA가 합성 될 때 시작점으로 제공되고, 둘째는 cap-independent 단백질 합성이 가능하도록 해 준다 [9]. 3´NCR은 100~150 bp로 구성되어 있으며, 이것의 2차 구조는 RNA 게놈의 주형으로 제공되는 negative sense RNA가 합성될 때 primer의 기능에 관여한다고 알려져 있다 [10-14].The genome of Enterovirus s has the form of single stranded positive sense RNA of about 7.2 to 7.5kb in size. It consists of one open reading frame (ORF) and a non-coding region (NCR) that is not expressed as a protein at the 5 'and 3' ends. The ORF is expressed as a polyprotein, consisting of about 2,185 amino acids [7]. This polyprotein is divided into several different proteins by the proteolytic enzyme of the virus. One polyprotein is divided into P1, P2, and P3, which encodes VP4, VP2, VP3, and VP1, which are components of the capsid protein of the virus, in order. The P2 part is 2A pro Proteinases and proteins that are not yet known to function correctly are encoded. The P3 part encodes VPg protein and 3C pro Protease and RdRp are encoded. The VPg protein acts as a primer on the 3 'side and is involved in the formation of a negative sense strand genome [8]. The 5 'NCR consists of 700 to 800 bp, forming a very complex secondary structure. The function of the secondary structure of these RNAs is firstly provided as a starting point when positive sense RNA is synthesized by RdRp, and secondly, allowing cap-independent protein synthesis [9]. 3'NCR consists of 100-150 bp, and its secondary structure is known to be involved in primer function when negative sense RNA is provided as a template for the RNA genome [10-14].
엔테로바이러스(Enterovirus)는 주로 하절기에 유ㆍ소아 층에 침범하여 감염자의 면역학적 특성에 따라 중증감염을 초래하기도 한다. 특히 위생이 나쁜 환경에서 흔하게 전파되는 전염성 병원체로써 감염경로는 분변-구강이며, 오염된 물과 토양을 통한 경구적인 전파로 이어진다. 감염자에서 배출된 분변속의 바이러스가 오수나 폐수를 통해 지하수, 하천, 해수로 흘러들어가 다시 사람에게로 전염되는데, 드물게는 호흡기 분비물을 통해서도 감염 된다 [15,16]. Enterovirus는 소화기를 통해 감염된 후 인후두 부위나 소장의 림프절에서 일차적으로 증식한 후 신체의 각 장기로 이동 한다 [17]. 임상증상은 감기 등의 가벼운 증상부터 심각한 마비까지 매우 다양하다. 소아인 경우 비폴리오성 enterovirus 감염은 50%정도 불현성 감염으로 나타지만, 나머지 경우 상기도 감염이나, 소화기증상, 결막염, 중이염, 피부발진, 무균성수막염, 포진성구협염, 수족구병, 고환염 등의 증상을 보인다. 드물게 심근염, 뇌염, Guillian-Barre syndrome, 실조증, 말단신경염, 횡단성척수염, 사지마비, 당뇨병, 유행성출혈성 각결막염 등 치명적이거나 합병증을 남기는 경우도 보고되어 있다 [18-22]. Enterovirus에 의한 대표적인 증상은 무균성수막염이고 주로 하절기에 발생하지만 봄이나 늦가을, 그리고 겨울에도 산발적으로 발생하는 경우가 있어 일 년 내내 감염될 위험이 존재한다. 또한 주된 발생 연령층은 영유아나, 경우에 따라 소아 및 노령층에서도 발생할 수 있다 [23,24].Enterovirus (Enterovirus) mainly invades infant and childhood during summer season, and may cause severe infection according to the immunological characteristics of the infected person. It is an infectious pathogen that is commonly spread in hygiene-poor environments. The infection pathway is fecal-oral, leading to oral transmission through contaminated water and soil. Fecal viruses from infected people flow through wastewater or wastewater into groundwater, rivers, and seawater, and then again to humans, though rarely through respiratory secretions [15,16]. Enteroviruses are transmitted through the digestive tract and then propagate primarily to the lymph nodes of the larynx or small intestine and then to the organs of the body [17]. Clinical symptoms vary from mild symptoms such as colds to severe paralysis. The incidence of nonpolyposis enterovirus infection is as low as 50% in infants, but in the remaining cases the incidence of upper respiratory infection, digestive symptoms, conjunctivitis, otitis media, skin rash, aseptic meningitis, herpes zoster, . It is rarely reported to cause fatal or complications such as myocarditis, encephalitis, Guillian-Barre syndrome, ataxia, terminal neuritis, transverse myelitis, limb paralysis, diabetes mellitus, and epidemic keratoconjunctivitis [18-22]. The most common symptom of enterovirus is aseptic meningitis, which occurs mainly during the summer, but sporadically occurs in spring, late autumn, and winter, so there is a risk of infection throughout the year. In addition, the main age group can occur in infants and, in some cases, children and elderly [23,24].
현재 개발되어 있는 항바이러스제제에 대한 바이러스 내성의 증가로 인하여, 최근에는 안전성과 보다 높은 효과, 그리고 저렴한 생산비용을 갖는 항바이러스제제들이 개발 중이지만 아직도 많은 바이러스들에서 치료 효과를 갖는 제제는 없다 [25]. 그런 이유로 아시아, 유럽 그리고 미국 등지의 과학자들은 약용식물을 기반으로 한 전통의학으로부터 항바이러스 제제에 대한 자료들을 이용하고 있다 [26-28]. 약용 식물들은 종종 여러 항바이러스 효과를 나타내는데, 이들은 부작용과 내성의 잠재성이 적고 생산비용이 낮다. 이미 많은 약용 식물들은 바이러스에 감염된 사람이나 동물들에 적용되어 강력한 항바이러스 효과를 나타내고 있다 [29,30]. Although antiviral agents with safety, higher efficacy, and lower production cost are currently under development due to increased viral resistance to currently developed antiviral agents, there are still no agents that have therapeutic effects in many viruses [ ]. For this reason, scientists in Asia, Europe and the United States are using data on antiviral agents from traditional medicinal plant-based medicines [26-28]. Medicinal plants often exhibit several antiviral effects, which have low potential for side effects and tolerance and low production costs. Many medicinal plants have already been shown to have potent antiviral effects in viral infected individuals or animals [29,30].
엔테로바이러스(Enterovirus)에 속하는 많은 바이러스의 경우, 적절한 마우스 모델이 없어 항바이러스제 연구에 있어서 큰 걸림돌이 되고 있다. 최근 EV71에 대한 세포 수용체가 규명되고, 인간 수용체를 가지고 있는 형질도입 마우스가 개발되어 연구가 진행되고 있으나, 아직까지 널리 사용되고 있지 못하고 있는 실정이다 [31, 32]. 반면에, Enterovirus 중 CVB3는 인간 뿐 아니라 마우스에서도 감염이 되는 것으로 알려져 있으며, 간, 심장, 뇌, 척수 및 췌장에 감염되는 것으로 알려져 있다 [33, 34]. CVB3 감염의 경우, 앞서 설명한 것과 같이 사람에 감염된 경우 대부분 특이한 증상이 없이 지나가는 것으로 알려져 있지만, 일부 제1형 당뇨병의 발병과 연관이 있음이 보고되었다 [35]. 또한, 췌장에 존재하는 Acinar 세포와 베타세포가 CVB3 에 감염되는 것이 보고되었으며, 마우스 모델에 있어서도 CVB3에 의한 췌장 감염이 일어나는 것이 잘 알려져 있다 [36, 37].For many viruses belonging to enteroviruses, there is no appropriate mouse model, which is a major obstacle to antiviral research. Recently, a cell receptor for EV71 has been identified, and a transgenic mouse having a human receptor has been developed and studied, but it has not been widely used yet [31,32]. CVB3, on the other hand, is known to infect not only humans but also mice, and is known to infect liver, heart, brain, spinal cord, and pancreas [33, 34]. In the case of CVB3 infection, as described above, it is reported that most people infected with the disease pass through without any specific symptoms, but it has been reported to be associated with the development of some type 1 diabetes [35]. In addition, it has been reported that the Acinar cells and beta cells present in the pancreas are infected with CVB3, and in the mouse model, CVB3-induced pancreatic infections are well known [36, 37].
Picornaviridae과에 속하는 EV71, CVB3, CVA16은 외피 비보유 positive-sense, single-stranded RNA viruses이다 [38, 39]. 영유아와 어린이에게서 EV71 및 CVA16 감염은 감염 초기 단계에서 발열, 두통, 인후통 등의 가벼운 감기증상과 함께 수족구병을 유발한다. EV71 및 CVA16 감염 후 수일이 지나면 손, 발, 입안에 궤양과 발진을 유발할 뿐만 아니라 호흡기, 장, 심장, 중추 신경 시스템도 감염을 유발한다 [38, 39]. 또한, EV71는 종종 소아마비와 같은 급성 이완성 마비와 뇌염을 일으킬 수 있다. CVB3는 소아 및 청소년층에서 가벼운 복통에서 본격적인 심낭염 및 심근염에 이르기까지 다양한 질병을 유발 한다고 알려져 있다 [40]. 그러나, 최근 여러 나라에서 EV71, CVB3 및 CV16의 반복적인 발생에도 불구하고, 사용 가능한 백신 또는 효과적인 항 바이러스 치료제의 개발이 어려운 실정이다. 따라서, EV71, CVB3 및 CVA16 감염을 치료하는 효과적인 항바이러스 치료제의 개발이 시급한 실정이다. EV71, CVB3 and CVA16 belonging to the Picornaviridae family are positive-sense, single-stranded RNA viruses [38, 39]. In infants and children, EV71 and CVA16 infections cause early onset infections with mild cold symptoms such as fever, headache, and sore throat. EV71 and CVA16 In addition to causing ulcers and rashes in the hands, feet and mouth within days after infection, respiratory, intestinal, cardiac, and central nervous systems also cause infections [38, 39]. In addition, EV71 can often cause acute relaxation paralysis, such as polio, and encephalitis. CVB3 is known to cause a variety of diseases in children and adolescents, ranging from mild abdominal pain to full pericarditis and myocarditis [40]. However, despite the repeated occurrence of EV71, CVB3 and CV16 in many countries, it is difficult to develop a vaccine or an effective antiviral agent. Therefore, it is urgent to develop an effective antiviral therapeutic agent for treating EV71, CVB3 and CVA16 infection.
엔테로바이러스(Enterovirus)에 대한 항바이러스제 개발은 지속적으로 연구되어져 왔다. 플레코나릴(Pleconaril)은 감수성이 있는 세포의 수용체와 결합을 하는 바이러스의 캡시드 단백질에 결합하여 바이러스가 세포내로 들어가는 것을 방해함으로써 항바이러스 활성을 나타낸다고 보고되어 있다 [41]. Pleconaril은 임상적으로는 78%, 바이러스학적으로는 92%, 실험적으로는 88%에서 enterovirus 감염 환자에게서 바이러스를 억제하는 활성을 나타낸 것으로 보고되고 있으나, 부작용으로 인해 FDA의 승인을 받지 못하였고 이것의 사용은 대부분 생명이 위험한 상황에 한정되며, 이것에 대한 내성 바이러스 또한 보고되고 있는 실정이다 [42-44]. 또한 RNA 바이러스 및 DNA 바이러스에 광범위한 항바이러스 활성을 나타내는 항바이러스제인 리바비린(Ribavirin) 역시 다양한 바이러스에서 약제내성을 나타내는 것으로 보고 되어있다 [45].The development of antiviral agents against Enterovirus has been continuously studied. Pleconaril has been reported to exhibit antiviral activity by binding to the capsid protein of a virus that binds to receptors in susceptible cells, thereby preventing the virus from entering the cell [41]. Pleconaril has been reported to have a viral suppressive activity in enterovirus infections in 78% of clinically, 92% of virologically, and 88% of experimental cases, but has not been approved by the FDA for its side effects. Most uses are limited to life-threatening situations, and resistant viruses have also been reported [42-44]. Ribavirin, an antiviral agent that exhibits extensive antiviral activity against RNA viruses and DNA viruses, has also been reported to exhibit drug resistance in a variety of viruses [45].
황금 (Scutellaria baicalensis Georgi)은 꿀풀과에 속하는 여러해살이 식물로 중국, 일본, 한국에서 약용식물로 널리 사용되고 있다. 황금의 주요 효능은 염증, 호흡기 감염, 소화기 감염에 효과가 있다고 알려져 있다 [46]. 황금의 주요 성분으로는 바이칼레인(baicalein), 바이칼린(baicalin), 우고닌(wogonin), 노르우고닌(norwogonin), 오록실린(oroxylin) A, β-시토스테롤(sitosterol), 모슬로플라본(mosloflavone) 등이 알려져 있다 [47]. Oroxylin A는 항암효과[48], 항미생물[49] 효과, 인식강화[50] 등 많은 생물학적 활성을 가지고 있다고 알려져 있다. Oroxylin A의 항암 효과는 가장 활발히 연구되는 분야로 세포자살 [51], 전이억제 [52], 세포주기 억제 [53]등 다양한 메커니즘으로 항암효과를 나타낸다고 알려져 있다. Golden ( Scutellaria baicalensis Georgi ) is a perennial plant belonging to the family Lamiaceae and is widely used as a medicinal plant in China, Japan and Korea. The main efficacy of gold is known to be effective in inflammation, respiratory infections, and gastrointestinal infections [46]. The main ingredients of gold are baicalein, baicalin, wogonin, norwogonin, oroxylin A, sitosterol, mosloflavone, ) Are known [47]. Oroxylin A is known to have many biological activities including anticancer effects [48], antimicrobial effects [49], and cognitive enhancement [50]. The anticancer effect of Oroxylin A is the most actively studied area, and it is known that it has anticancer effect by various mechanisms such as cell suicide [51], metastasis inhibition [52] and cell cycle inhibition [53].
오록실린(Oroxylin) A는 O-methyl기를 가지고 있는 flavone으로 황금에서 발견되었으며, 황금은 바이칼레인(baicalein) 및 우고닌(wogonin) 등의 생리활성 물질을 가지고 있는 유용한 약용 식물이다 [54]. Oroxylin A 는 다양한 약리작용을 나타내는 것으로 알려져 있으며, 항염, 항암, 항혈전 작용을 타나내는 것이 보고되었다 [55]. 또한 최근 연구를 통해 황금 추출물과 에틸아세테이트 및 클로로포름 분획물이 influenza virus [56], RSV [57], HBV [58, 59], 및 HIV-1 [60]에 항바이러스 활성을 나타내는 것이 보고되었으며, 이러한 항바이러스 활성이 wogonin, oroxylin 또는 baicalein등에 의해 나타나는 것으로 보고되었다. 이와 더불어 최근 황금의 수용성 추출물 및 baicalein이 dengue virus의 복제를 억제하여 항바이러스 활성을 나타냄이 보고되었다 [61, 62]. Oroxylin A is a flavone with an O-methyl group found in gold and gold is a useful medicinal plant with bioactive substances such as baicalein and wogonin [54]. Oroxylin A is known to exhibit various pharmacological actions and has been reported to exhibit anti-inflammatory, anti-cancer, and anti-thrombotic effects [55]. Recent studies have also shown that gold extracts, ethyl acetate and chloroform fractions exhibit antiviral activity against influenza virus [56], RSV [57], HBV [58, 59], and HIV-1 [60] Antiviral activity has been reported to be caused by wogonin, oroxylin, or baicalein. In addition, it has recently been reported that water-soluble extracts of gold and baicalein inhibit the replication of dengue virus and exhibit antiviral activity [61, 62].
그러나, 아직까지 오록실린(oroxylin) A, 노르우고닌(norwogonin), 모슬로플라본(mosloflavone) 및 이들을 포함하는 황금 추출물과 분획물이 엔테로바이러스(enterovirus)에 대한 항바이러스 활성을 가지고 있음은 보고된 바 없다. However, it has been reported that oroxylin A, norwogonin, mosloflavone, and gold extracts and fractions containing them have antiviral activity against enteroviruses none.
이에 본 발명에서는 황금 추출물 및 클로로포름 분획물, 그리고 클로로포름 분획물 중 포함된 오록실린(oroxylin) A, 노르우고닌(norwogonin), 모슬로플라본(mosloflavone)이 CVB3, CVA16 및 EV71에 대한 광범위 항바이러스 활성을 나타냄을 Vero세포에서 세포병변 억제 효과실험 및 세포독성 실험 등의 in vitro과 in vivo 동물실험을 통해 증명하고, 본 연구를 통해 황금 추출물, 분획물 및 황금에 포함된 norwogonin, oroxylin A, mosloflavone의 enterovirus 감염치료 효과를 최초로 규명하였다. In the present invention, oroxylin A, norwogonin, and mosloflavone contained in the gold extract and chloroform fractions and the chloroform fractions exhibit broad antiviral activity against CVB3, CVA16 and EV71 In vitro and in vivo animal experiments such as cell-lesion inhibitory effect and cytotoxicity test in Vero cells. In this study, enterovirus infection treatment of norwogonin, oroxylin A and mosloflavone contained in gold extract, fraction and gold Effect was first identified.
본 연구에서는 엔테로바이러스(enterovirus)속에 속하는 EV71, CVB3 및 CVA16에 대하여 황금 추출물 및 이로부터 분리된 오록실린(oroxylin) A, 노르우고닌(norwogonin), 모슬로플라본(mosloflavone) 화합물 시료를 대상으로 (1) Vero 세포에서의 세포독성 및 EV71, CVB3, CVA16의 항바이러스 활성실험, 세포병변 억제실험(실험예 1); (2) EV71에 대한 항바이러스 활성을 확인하기 위한 enterovirus 71의 VP단백질에 대한 Western blot 분석법 (실험예 2); (3) replicon system (pRibFluc-EV71)을 이용한 Replicon 분석법을 통한 항바이러스 활성 메카니즘 분석실험 (실험예 3); (4) BALB/c 마우스를 이용한 CVB3 바이러스에 대한 항바이러스 활성 측정을 위한 in vivo 동물실험(실험예 4) 등의 광범위한 시험관내 실험(in vitro test) 및 생체내 동물실험(in vivo test)를 통하여, 본 발명의 상기 시료들이 강력한 항 엔테로바이러스(enterovirus) 활성을 나타냄을 확인하여 본 발명을 완성하였다.In this study, the gold extracts and the oroxylin A, norwogonin and mosloflavone compounds isolated from the enterovirus (EV71, CVB3, and CVA16) 1) cytotoxicity in Vero cells and antiviral activity tests of EV71, CVB3 and CVA16, experiments for inhibiting cell lesion (Experimental Example 1); (2) Western blot analysis of the VP protein of enterovirus 71 to confirm antiviral activity against EV71 (Experimental Example 2); (3) Experiment for analysis of antiviral activity mechanism by replicon analysis using replicon system (pRibFluc-EV71) (Experimental Example 3); (4) in vitro test and in vivo test such as in vivo animal experiment (Example 4) for the antiviral activity measurement of CVB3 virus using BALB / c mouse The inventors of the present invention confirmed that the samples of the present invention exhibited strong enter enterovirus activity, thereby completing the present invention.
상기한 목적을 달성하기 위하여, 본 발명은 황금 추출물 또는 이로부터 분리된 노르우고닌(norwogonin), 오록실린(oroxylin) A, 및 모슬로플라본(mosloflavone)으로 구성된 군으로부터 선택된 화합물을 유효성분으로 함유하는 엔테로 바이러스에 기인한 감염증의 예방 및 치료용 약학조성물을 제공한다.In order to accomplish the above object, the present invention provides a pharmaceutical composition containing, as an active ingredient, a compound selected from the group consisting of gold extract or norwogonin, oroxylin A, and mosloflavone isolated therefrom The present invention provides a pharmaceutical composition for preventing and treating infectious diseases caused by enteroviruses.
또한, 본 발명은 황금 추출물 또는 이로부터 분리된 노르우고닌(norwogonin), 오록실린(oroxylin) A, 및 모슬로플라본(mosloflavone)으로 구성된 군으로부터 선택된 화합물 및 기존 항엔테로 바이러스제와의 조합을 유효성분으로 함유하는 엔테로 바이러스에 기인한 감염증의 예방 및 치료를 위한 약학 조성물을 제공한다.The present invention also relates to a pharmaceutical composition comprising a combination of a compound selected from the group consisting of gold extract or isolated therefrom, such as norwogonin, oroxylin A, and mosloflavone, A pharmaceutical composition for the prevention and treatment of infectious diseases caused by enteroviruses.
또한, 황금 추출물 또는 이로부터 분리된 노르우고닌(norwogonin), 오록실린(oroxylin) A, 및 모슬로플라본(mosloflavone)으로 구성된 군으로부터 선택된 화합물을 유효성분으로 함유하는 항엔테로 바이러스제를 제공한다.The present invention also provides an anti-enteroviral agent containing, as an active ingredient, a compound selected from the group consisting of a gold extract or isolated therefrom, norwogonin, oroxylin A, and mosloflavone.
본 발명은 황금 추출물 또는 이로부터 분리된 노르우고닌(norwogonin), 오록실린(oroxylin) A, 및 모슬로플라본(mosloflavone)으로 구성된 군으로부터 선택된 화합물을 유효성분으로 함유하는 엔테로 바이러스에 기인한 감염증의 예방 및 개선용 건강기능식품을 제공한다.The present invention relates to a method for the treatment of an infectious disease caused by an enterovirus comprising, as an active ingredient, a compound selected from the group consisting of gold extracts or isolated from them, norwogonin, oroxylin A, and mosloflavone. And a health functional food for prevention and improvement.
본원에서 정의되는 황금 추출물은 황금의 줄기, 엽 및 뿌리줄기를 포함하는 전초의 조추출물, 극성용매 가용 추출물 또는 비극성용매 가용 추출물임을 특징으로 한다.The gold extract as defined herein is characterized by being a crude extract, a polar solvent-soluble extract or a non-polar solvent-soluble extract of a plant including golden stem, leaf and root stem.
본원에서 정의되는 조추출물은 정제수를 포함한 물, 메탄올, 에탄올, 부탄올 등의 탄소수 1 내지 4의 저급알코올 또는 이들의 혼합용매로부터 선택된 용매, 바람직하게는 메탄올 또는 물 및 메탄올 혼합용매, 보다 바람직하게는 메탄올에 가용한 추출물임을 특징으로 한다.The crude extract as defined herein may be dissolved in a solvent selected from water including purified water, a lower alcohol having 1 to 4 carbon atoms such as methanol, ethanol, and butanol, or a mixed solvent thereof, preferably methanol or water and a methanol mixed solvent, And is an extract which is soluble in methanol.
본원에서 정의되는 비극성용매 가용 추출 분획물은 본원의 조추출물로부터 헥산, 메틸렌 클로라이드, 클로로포름, 또는 에틸아세테이트, 바람직하게는 헥산, 또는 클로로포름 용매에 가용한 추출물만을 정제한 비극성 용매에 가용한 추출 분획물들을 포함한다.The nonpolar solvent-soluble extract fractions defined herein contain extract fractions soluble in nonpolar solvents purified from the crude extract of the present invention in hexane, methylene chloride, chloroform, or ethyl acetate, preferably hexane, or chloroform solvent alone do.
본원에서 정의되는 극성용매 가용 추출물은 상기 조추출물로부터 비극성용매 가용분획물들을 제거하고 남은 물, 메탄올, 부탄올 또는 이들의 혼합용매로부터 선택되어진 용매, 바람직하게는 물 또는 부탄올, 보다 바람직하게는 부탄올에 가용한 추출 분획물을 포함한다.The polar solvent-soluble extract as defined herein is prepared by removing the non-polar solvent-soluble fractions from the crude extract and washing with water, methanol, butanol or a mixed solvent thereof, preferably water or butanol, more preferably, And one extracted fraction.
본원에서 정의되는 엔테로바이러스(enterovirus)는 3가지 혈청형의 Poliovirus (PV: 1~3); 23가지 혈청형의 Coxsackievirus A군 (CVA: 1~22, 24); 6가지 혈청형의 Coxsackievirus B군 (CVB: 1~6); 28가지 혈청형의 Echovirus군 (ECV: 1~7, 9, 11~21, 24~27, 29~33) 및 기타 인체 Enterovirus (EV: 68~116)으로 구성된 군으로부터 선택된 혈청형, 보다 바람직하게는 EV71, CVB3, 또는 CVA16 혈청형을 가짐을 특징으로 한다.Enteroviruses as defined herein include three serotypes of Poliovirus (PV: 1-3); Coxsackievirus A group of 23 serotypes (CVA: 1 to 22, 24); Six serotypes of Coxsackievirus B (CVB: 1 to 6); A serotype selected from the group consisting of 28 serotypes of Echovirus (ECV: 1-7, 9, 11-21, 24-27, 29-33) and other human enteroviruses (EV: 68-111) Is characterized by having an EV71, CVB3, or CVA16 serotype.
본원에서 정의되는 엔테로바이러스(enterovirus)에 기인한 질환은 수족구병, 상기도 감염증, 소화기증상, 결막염, 중이염, 피부발진, 무균성수막염, 포진성구협염, 고환염, 심근염, 뇌염, 길라안-바레 증후군 (Guillian-Barre syndrome), 실조증, 말단신경염, 횡단성척수염, 사지마비, 당뇨병, 유행성출혈성 각결막염, 궤양, 발진, 소아마비와 같은 급성 이완성 마비, 심낭염, 제1형 당뇨병, 또는 췌장 감염증, 바람직하게는, 상기도 감염증, 결막염, 무균성수막염, 포진성구협염, 심근염, 뇌염, 제1형 당뇨병, 또는 췌장 감염증을 포함한다.The diseases caused by enteroviruses as defined herein include those caused by enteroviruses, such as, but not limited to, those caused by atopic diseases, gastrointestinal tract infections, gastrointestinal symptoms, conjunctivitis, otitis media, skin rash, aseptic meningitis, herpetic sinusitis, Acute atonic paralysis such as Guillian-Barre syndrome, ataxia, terminal neuritis, transverse myelitis, limb paralysis, diabetes mellitus, epidemic hemorrhagic keratoconjunctivitis, ulcers, rashes, polio, pericarditis, type 1 diabetes, or pancreatic infections, preferably Include conjunctivitis, conjunctivitis, aseptic meningitis, herpetic sinusitis, myocarditis, encephalitis, type 1 diabetes, or pancreatic infections.
본원에서 정의되는 기존 항엔테로바이러스(enterovirus)제는 플레코나릴(Pleconaril), 루핀트리비르(Rupintrivir), 타미플루(Oseltamivir; Tamiflu), 렐렌자(Zanamivir, Relenza), 페라미비르(Peramivir), 아만타딘(Amantadine, Symmetrel), 리만타딘(Rimantadine), 리바비린(Rivabirin), 또는 타리바비린(Taribavirin)으로부터 선택된 항바이러스제이며, 바람직하게는 플레코나릴(Pleconaril), 루핀트리비르(Rupintrivir) 또는 리바비린(Rivabirin)을 포함한다.Existing anti-enterovirus agents as defined herein are selected from the group consisting of Pleconaril, Rupintrivir, Oseltamivir (Tamiflu), Zanamivir, Relenza, Peramivir, Amantadine Preferably selected from the group consisting of Pleconaril, Rupintrivir or Rivabirin, which is an antiviral selected from Amantadine, Symmetrel, Rimantadine, Rivabirin, or Taribavirin. do.
상기 질환은 사람을 포함한 포유동물에 발생하는 것을 특징으로 한다. The disease is characterized in that it occurs in mammals including humans.
본 발명의 황금 추출물 또는 이로부터 분리된 화합물을 유효성분으로 함유하는 조성물은, 조성물 총 중량에 대하여 상기 추출물 또는 이로부터 분리된 화합물을 0.1 ~ 50 중량% 포함한다. The composition comprising the gold extract of the present invention or a compound isolated therefrom as an active ingredient comprises 0.1 to 50% by weight of the extract or the compound isolated therefrom based on the total weight of the composition.
본 발명의 화합물은 당해 기술분야에서 통상적인 방법에 따라 약학적으로 허용 가능한 염 및 용매화물로 제조될 수 있다.The compounds of the present invention may be prepared into pharmaceutically acceptable salts and solvates by methods conventional in the art.
본원에서 정의되는 약학적으로 허용 가능한 염으로는 유리산(free acid)에 의해 형성된 산부가염이 유용하다. 산부가염은 통상의 방법, 예를 들면 화합물을 과량의 산 수용액에 용해시키고, 이 염을 메탄올, 에탄올, 아세톤 또는 아세토니트릴과 같은 수혼화성 유기 용매를 사용하여 침전시켜서 제조한다. 동일한 몰량의 화합물 및 물 중의 산 또는 알코올(예, 글리콜 모노메틸에테르)을 가열하고 이어서 상기 혼합물을 증발시켜서 건조시키거나, 또는 석출된 염을 흡인 여과시킬 수 있다.Pharmaceutically acceptable salts as defined herein are acid addition salts formed by free acids. The acid addition salt is prepared by a conventional method, for example, by dissolving the compound in an excess amount of an acid aqueous solution, and precipitating the salt using a water-miscible organic solvent such as methanol, ethanol, acetone or acetonitrile. The same molar amount of the compound and the acid or alcohol (e.g., glycol monomethyl ether) in water may be heated and then the mixture may be evaporated to dryness, or the precipitated salt may be filtered by suction.
이 때, 유리산으로는 유기산과 무기산을 사용할 수 있으며, 무기산으로는 염산, 인산, 황산, 질산, 주석산 등을 사용할 수 있고 유기산으로는 메탄술폰산, p-톨루엔술폰산, 아세트산, 트리플루오로아 세트산, 시트르산, 말레인산(maleic acid), 숙신산, 옥살산, 벤조산, 타르타르산, 푸마르산, 만데르산, 프로피온산(propionic acid), 구연산(citric acid), 젖산(lactic acid), 글리콜산(glycollic acid), 글루콘산(gluconic acid), 갈락투론산, 글루탐산, 글루타르산(glutaric acid), 글루쿠론산(glucuronic acid), 아스파르트산, 아스코르빈산, 카본산, 바닐릭산 및 히드로 아이오딕산 등을 사용할 수 있다.As the free acid, organic acids and inorganic acids can be used. As the inorganic acids, hydrochloric acid, phosphoric acid, sulfuric acid, nitric acid, tartaric acid and the like can be used. Examples of the organic acids include methanesulfonic acid, p -toluenesulfonic acid, acetic acid, trifluoroacetic acid Citric acid, lactic acid, glycollic acid, gluconic acid, maleic acid, succinic acid, oxalic acid, benzoic acid, tartaric acid, fumaric acid, manderic acid, propionic acid, citric acid, gluconic acid, galacturonic acid, glutamic acid, glutaric acid, glucuronic acid, aspartic acid, ascorbic acid, carbonic acid, vanillic acid and hydroiodic acid can be used.
또한, 염기를 사용하여 약학적으로 허용 가능한 금속염을 만들 수 있다. 알칼리 금속 또는 알칼리토 금속염은, 예를 들면 화합물을 과량의 알칼리 금속 수산화물 또는 알칼리토 금속 수산화물 용액 중에 용해하고, 비 용해 화합물염을 여과한 후 여액을 증발, 건조시켜 얻는다. 이때, 금속염으로서는 특히 나트륨, 칼륨 또는 칼슘염을 제조하는 것이 제약상 적합하며, 또한 이에 대응하는 은염은 알칼리 금속 또는 알칼리토 금속염을 적당한 은염(예, 질산은)과 반응시켜 얻는다.In addition, bases can be used to make pharmaceutically acceptable metal salts. The alkali metal or alkaline earth metal salt is obtained, for example, by dissolving a compound in an excess amount of an alkali metal hydroxide or alkaline earth metal hydroxide solution, filtering the non-soluble compound salt, and evaporating and drying the filtrate. At this time, it is preferable for the metal salt to produce sodium, potassium or calcium salt in particular, and the corresponding silver salt is obtained by reacting an alkali metal or alkaline earth metal salt with a suitable silver salt (for example, silver nitrate).
본 발명의 화합물의 약학적으로 허용 가능한 염은, 달리 지시되지 않는 한, 본 발명의 화합물에 존재할 수 있는 산성 또는 염기성기의 염을 포함한다. 예를 들면, 약학적으로 허용 가능한 염으로는 히드록시기의 나트륨, 칼슘 및 칼륨염이 포함되며, 아미노기의 기타 약학적으로 허용 가능한 염으로는 하이드로브로마이드, 황산염, 수소 황산염, 인산염, 수소 인산염, 이수소 인산염, 아세테이트, 숙시네이트, 시트레이트, 타르트레이트, 락테이트, 만델레이트, 메탄설포 네이트(메실레이트) 및 p-톨루엔설포네이트(토실레이트) 염이 있으며, 당업계에서 알려진 염의 제조 방법이나 제조과정을 통하여 제조될 수 있다. Pharmaceutically acceptable salts of the compounds of the present invention include, unless otherwise indicated, salts of acidic or basic groups that may be present in the compounds of the present invention. For example, pharmaceutically acceptable salts include sodium, calcium and potassium salts of hydroxy groups, and other pharmaceutically acceptable salts of amino groups include hydrobromide, sulfate, hydrogen sulfate, phosphate, hydrogen phosphate, dihydrogen phosphate phosphate, acetate, succinate, citrate, tartrate, lactate, mandelate rate, methane sulfonate (mesylate) and p - toluene sulfonate (tosylate) and a salt, the salt manufacturing method or manufacturing process known in the art ≪ / RTI >
이하, 본 발명을 더욱 상세히 설명한다. Hereinafter, the present invention will be described in more detail.
본 발명의 추출물 및 화합물들은 하기와 같은 제조방법으로 수득될 수 있다. The extracts and compounds of the present invention can be obtained by the following production methods.
예를 들어, 이하, 본 발명을 상세히 설명한다.For example, the present invention will be described in detail below.
본 발명의 황금 추출물은 하기와 같이 제조될 수 있다. 건조된 황금 전초를 세척 및 세절 후 정제수를 포함한 물, 메탄올, 에탄올, 부탄올 등의 탄소수 1 내지 4의 저급알코올 또는 이들의 혼합용매로부터 선택된 용매, 바람직하게는 물, 메탄올, 에탄올 및 이의 혼합용매를 수회 섞은 다음에 30℃ 내지 150℃, 바람직하게는 실온에서 12시간 내지 30일, 바람직하게는 1일 내지 7일 동안 초음파 추출법, 열수 추출법, 상온 추출법 또는 환류추출법, 바람직하게는 상온 추출법을 약 1 내지 20회, 바람직하게는 2 내지 10회 반복 수행하여 얻은 추출액을 여과, 감압 농축, 및 건조하여 본 발명의 조추출물을 얻을 수 있다.The gold extract of the present invention can be prepared as follows. After drying and finishing the dried gold outpoule, it is mixed with a solvent selected from water, a low alcohol having 1 to 4 carbon atoms such as methanol, ethanol, and butanol, or a mixed solvent thereof, preferably water, methanol, ethanol and a mixed solvent thereof And then subjected to ultrasonic extraction, hot water extraction, room temperature extraction or reflux extraction, preferably room temperature extraction, at about 30 ° C to 150 ° C, preferably at room temperature for about 12 hours to 30 days, preferably for 1 day to 7 days, To 20 times, preferably 2 to 10 times. The extract obtained by filtration, concentration under reduced pressure, and dried can be used to obtain the crude extract of the present invention.
또한, 본 발명의 극성용매 또는 비극성용매 가용 추출물은 상기에서 얻은 조추출물, 바람직하게는 30 내지 90% 에탄올 조추출물 중량의 약 0.0005 내지 5배, 바람직하게는 0.05 내지 0.5배 부피 (v/w%)의 물을 가한 후, n-헥산, 메틸렌 클로라이드, 에틸 아세테이트 및 부탄올을 이용한 통상적인 분획과정을 수행하여 n-헥산, 메틸렌 클로라이드, 에틸 아세테이트 등의 비극성 용매에 가용한 비극성 용매 가용 추출 분획물; 및 부탄올, 물 등의 극성용매에 가용한 극성용매 가용 추출 분획물을 수득할 수 있다.The polar solvent or the non-polar solvent soluble extract of the present invention may further contain about 0.0005 to 5 times, preferably 0.05 to 0.5 times the volume (v / w%) of the crude extract, preferably 30 to 90% ), Followed by fractionation using n-hexane, methylene chloride, ethyl acetate and butanol to obtain non-polar solvent-soluble extract fractions, which are dissolved in a nonpolar solvent such as n-hexane, methylene chloride or ethyl acetate; And polar solvent-soluble extract fractions soluble in polar solvents such as butanol and water can be obtained.
상기에서 수득한 n-헥산, 메틸렌 클로라이드, 에틸 아세테이트 등의 비극성 용매에 가용한 비극성 용매 가용 추출 분획물, 바람직하게는 헥산 가용분획물을 헥산 및 메틸렌클로라이드 혼합용매를 극성을 증가시키는 방법을 이용하여 플래쉬 컬럼크로마토그래피, RP C18 컬럼크로마토그래피 또는 실리카겔 오픈 컬럼크로마토그래피 등의 크로마토그래피를 이용한 정제방법을 선택적으로 수회 반복 수행하여 본 발명의 화합물인 레이노우디올(reynoudiol)을 각각 정제 및 수득할 수 있다. The non-polar solvent-soluble fraction extracted in the non-polar solvent, such as n-hexane, methylene chloride or ethyl acetate, obtained in the above, is dissolved in hexane and methylene chloride mixed solvent in a flash column The purification method using chromatography such as chromatography, RP C18 column chromatography or silica gel open column chromatography may be repeated several times to selectively purify and obtain reynoudiol, which is a compound of the present invention.
본 발명자들은 상기 제조방법으로 수득되는 추출물 및 화합물들을 대상으로 한, (1) 베로(vero) 세포에서의 세포독성 및 EV71, CVB3, CVA16의 항바이러스 활성실험, 세포병변 억제실험(실험예 1); (2) EV71에 대한 항바이러스 활성을 확인하기 위한 enterovirus 71의 VP단백질에 대한 Western blot 분석법 (실험예 2); (3) replicon system(pRIBFluc-EV71)을 이용한 Replicon 분석법을 통한 항바이러스 활성 메카니즘 분석실험 (실험예 3); (4) BALB/c 마우스를 이용한 CVB3 바이러스에 대한 항바이러스 활성 측정을 위한 in vivo 동물실험(실험예 4) 등의 광범위한 시험관내 실험(in vitro test) 및 생체내 동물실험(in vivo test)를 통하여, 본 발명의 상기 시료들이 강력한 항 엔테로바이러스 활성을 나타냄을 확인함으로, 상기 조성물을 엔테로 바이러스에 기인한 질환의 예방 및 치료용 약학조성물 또는 건강기능식품으로 유용함을 확인하였다.(1) cytotoxicity in vero cells and antiviral activity tests of EV71, CVB3 and CVA16, experiments for inhibition of cell lesion (Experimental Example 1), and ; (2) Western blot analysis of the VP protein of enterovirus 71 to confirm antiviral activity against EV71 (Experimental Example 2); (3) Analysis of antiviral activity mechanism through replicon analysis using replicon system (pRIBFluc-EV71) (Experimental Example 3); (4) in vitro test and in vivo test such as in vivo animal experiment (Example 4) for the antiviral activity measurement of CVB3 virus using BALB / c mouse Through confirming that the samples of the present invention exhibit strong anti-enteroviral activity, it is confirmed that the composition is useful as a pharmaceutical composition or health functional food for the prevention and treatment of diseases caused by enteroviruses.
따라서, 본원 발명은 상기의 제조방법으로 얻어진 황금 추출물 또는 이로부터 분리된 화합물을 유효성분으로 함유하는 엔테로 바이러스에 기인한 질환의 예방 및 치료를 위한 약학 조성물 및 건강기능식품을 제공한다.Accordingly, the present invention provides a pharmaceutical composition and a health functional food for the prevention and treatment of diseases caused by enterovirus containing the gold extract or the compound isolated therefrom as an active ingredient.
본 발명의 약학 조성물은, 조성물 총 중량에 대하여 상기 추출물 또는 화합물을 0.1 내지 50 중량%로 포함한다. The pharmaceutical composition of the present invention contains 0.1 to 50% by weight of the above extract or compound, based on the total weight of the composition.
또한, 황금의 줄기, 엽 및 뿌리줄기는 오랫동안 식용되거나 생약으로 사용되어 오던 약재로서 본 발명의 황금 추출물로부터 분리된 화합물 역시 독성 및 부작용 등의 문제가 없다. In addition, the stem, leaf and stem of gold have been used for a long time as a medicinal herb or as a herbal medicine, and the compounds isolated from the gold extract of the present invention are also free from toxicity and side effects.
본 발명의 추출물 또는 화합물을 함유하는 약학 조성물의 제조에 통상적으로 사용하는 적절한 담체, 부형제 및 희석제를 더 포함할 수 있다.Excipients and diluents conventionally used in the preparation of pharmaceutical compositions containing the extracts or compounds of the present invention.
본 발명의 추출물 또는 화합물의 약학적 투여 형태는 이들의 약학적 허용 가능한 염의 형태로도 사용될 수 있고, 또한 단독으로 또는 타 약학적 활성 화합물과 결합뿐만 아니라 적당한 집합으로 사용될 수 있다. The pharmaceutical dosage forms of the extracts or compounds of the present invention may be used in the form of their pharmaceutically acceptable salts and may be used alone or in combination with other pharmacologically active compounds as well as in suitable aggregates.
본 발명에 따른 추출물 또는 화합물을 함유하는 조성물은, 각각 통상의 방법에 따라 산제, 과립제, 정제, 캡슐제, 현탁액, 에멀젼, 시럽, 에어로졸 등의 경구형 제형, 외용제, 좌제 및 멸균 주사용액의 형태로 제형화하여 사용될 수 있다. 추출물 또는 화합물을 함유하는 조성물에 함유될 수 있는 담체, 부형제 및 희석제로는 락토즈, 덱스트로즈, 수크로스, 솔비톨, 만니톨, 자일리톨, 에리스리톨, 말티톨, 전분, 아카시아 고무, 알지네이트, 젤라틴, 칼슘 포스페이트, 칼슘 실리케이트, 셀룰로즈, 메틸 셀룰로즈, 미정질 셀룰로스, 폴리비닐 피롤리돈, 물, 메틸히드록시벤조에이트, 프로필히드록시벤조에이트, 탈크, 마그네슘 스테아레이트 및 광물유를 들 수 있다. 제제화할 경우에는 보통 사용하는 충진제, 증량제, 결합제, 습윤제, 붕해제, 계면활성제 등의 희석제 또는 부형제를 사용하여 조제된다. 경구투여를 위한 고형제제에는 정제, 환제, 산제, 과립제, 캡슐제 등이 포함되며, 이러한 고형제제는 상기 화합물에 적어도 하나 이상의 부형제 예를 들면, 전분, 칼슘카보네이트(calcium carbonate), 수크로스(sucrose) 또는 락토오스(lactose), 젤라틴 등을 섞어 조제된다. 또한 단순한 부형제 이외에 마그네슘 스테아레이트, 탈크 같은 윤활제들도 사용된다. 경구를 위한 액상 제제로는 현탁제, 내용액제, 유제, 시럽제 등이 해당되는데 흔히 사용되는 단순희석제인 물, 리퀴드 파라핀 이외에 여러 가지 부형제, 예를 들면 습윤제, 감미제, 방향제, 보존제 등이 포함될 수 있다. 비경구 투여를 위한 제제에는 멸균된 수용액, 비수성용제, 현탁제, 유제, 동결건조 제제, 좌제가 포함된다. 비수성용제, 현탁제로는 프로필렌글리콜(propylene glycol), 폴리에틸렌 글리콜, 올리브 오일과 같은 식물성 기름, 에틸올레이트와 같은 주사 가능한 에스테르 등이 사용될 수 있다. 좌제의 기제로는 위텝솔(witepsol), 마크로골(macrogol), 트윈 (tween) 61, 카카오지, 라우린지, 글리세롤젤라틴 등이 사용될 수 있다.The composition containing the extract or the compound according to the present invention can be administered orally or parenterally in the form of oral, granule, tablet, capsule, suspension, emulsion, syrup, aerosol or the like, external preparation, Can be used. Examples of carriers, excipients and diluents that may be contained in the composition containing the extract or compound include lactose, dextrose, sucrose, sorbitol, mannitol, xylitol, erythritol, maltitol, starch, acacia rubber, alginate, gelatin, calcium phosphate , Calcium silicate, cellulose, methylcellulose, microcrystalline cellulose, polyvinylpyrrolidone, water, methylhydroxybenzoate, propylhydroxybenzoate, talc, magnesium stearate and mineral oil. In the case of formulation, a diluent or excipient such as a filler, an extender, a binder, a wetting agent, a disintegrant, or a surfactant is usually used. Solid formulations for oral administration include tablets, pills, powders, granules, capsules and the like, which may contain at least one excipient such as starch, calcium carbonate, sucrose ), Lactose, gelatin and the like. In addition to simple excipients, lubricants such as magnesium stearate and talc are also used. Examples of the liquid preparation for oral use include suspensions, solutions, emulsions, and syrups. In addition to water and liquid paraffin, simple diluents commonly used, various excipients such as wetting agents, sweeteners, fragrances, preservatives and the like may be included . Formulations for parenteral administration include sterilized aqueous solutions, non-aqueous solutions, suspensions, emulsions, freeze-dried preparations, and suppositories. Examples of the suspending agent include propylene glycol, polyethylene glycol, vegetable oil such as olive oil, injectable ester such as ethyl oleate, and the like. As a suppository base, witepsol, macrogol, tween 61, cacao butter, laurin, glycerol gelatin and the like can be used.
본 발명의 추출물 또는 화합물의 바람직한 투여량은 환자의 상태 및 체중, 질병의 정도, 약물형태, 투여경로 및 기간에 따라 다르지만, 당업자에 의해 적절하게 선택될 수 있다. 그러나 바람직한 효과를 위해서, 본 발명의 추출물 또는 화합물은 1일 0.0001 내지 100 ㎎/kg으로, 바람직하게는 0.001 내지 10 ㎎/kg으로 투여하는 것이 좋다. 투여는 하루에 한번 투여할 수도 있고, 수회 나누어 투여할 수도 있다. 상기 투여량은 어떠한 면으로든 본 발명의 범위를 한정하는 것은 아니다.The preferred dose of the extract or compound of the present invention varies depending on the condition and the weight of the patient, the degree of disease, the type of drug, the administration route and the period of time, but can be appropriately selected by those skilled in the art. However, for the desired effect, the extract or the compound of the present invention is preferably administered at 0.0001 to 100 mg / kg, preferably 0.001 to 10 mg / kg per day. The administration may be carried out once a day or divided into several times. The dose is not intended to limit the scope of the invention in any way.
본 발명의 추출물 또는 화합물은 쥐, 생쥐, 가축, 인간 등의 포유동물에 다양한 경로로 투여될 수 있다. 투여의 모든 방식은 예상될 수 있는데, 예를 들면, 경구, 직장 또는 정맥, 근육, 피하, 자궁내 경막 또는 뇌혈관 내(intracerebroventricular) 주사에 의해 투여될 수 있다.The extract or compound of the present invention can be administered to mammals such as rats, mice, livestock, humans, and the like in various routes. All modes of administration may be expected, for example, by oral, rectal or intravenous, intramuscular, subcutaneous, intra-uterine or intracerebroventricular injections.
또한, 본 발명은 황금 추출물 또는 이로부터 분리된 노르우고닌(norwogonin), 오록실린(oroxylin) A, 및 모슬로플라본(mosloflavone)으로 구성된 군으로부터 선택된 화합물을 유효성분으로 함유하는 엔테로 바이러스에 기인한 질환의 예방 및 개선용 건강기능식품을 제공한다.The present invention also relates to a method for the treatment or prevention of diseases caused by enteroviruses containing, as an active ingredient, a compound selected from the group consisting of gold extracts or isolated therefrom, norwogonin, oroxylin A, and mosloflavone A health functional food for preventing and improving diseases is provided.
본 발명의 추출물 또는 화합물을 첨가할 수 있는 식품으로는, 예를 들어, 각종 식품류, 음료, 껌, 차, 비타민 복합제, 건강 기능성 식품류 등이 있다.Examples of foods to which the extract or compound of the present invention can be added include various foods, beverages, gums, tea, vitamin complexes, and health functional foods.
또한, 엔테로 바이러스로 인한 질환의 예방 효과를 목적으로 식품 또는 음료에 첨가될 수 있다. 이 때, 식품 또는 음료 중의 상기 추출물의 양은 전체 식품 중량의 0.01 내지 15 중량%로 가할 수 있으며, 건강 음료 조성물은 100 ㎖를 기준으로 0.02 내지 5 g, 바람직하게는 0.3 내지 1 g의 비율로 가할 수 있다. It may also be added to foods or beverages for the purpose of preventing diseases caused by enteroviruses. In this case, the amount of the extract in the food or drink may be 0.01 to 15% by weight of the total food, and the health beverage composition may be added in a proportion of 0.02 to 5 g, preferably 0.3 to 1 g, .
본 발명의 건강기능식품은 정제, 캡슐제, 환제, 액제 등의 형태를 포함한다.The health functional food of the present invention includes forms such as tablets, capsules, pills, and liquids.
본 발명의 건강 기능성 음료 조성물은 지시된 비율로 필수 성분으로서 상기 추출물 또는 화합물을 함유하는 외에는 다른 성분에는 특별한 제한이 없으며 통상의 음료와 같이 여러 가지 향미제 또는 천연 탄수화물 등을 추가 성분으로서 함유할 수 있다. 상술한 천연 탄수화물의 예는 모노사카라이드, 예를 들어, 포도당, 과당 등; 디사카라이드, 예를 들어 말토스, 슈크로스 등; 및 폴리사카라이드, 예를 들어 덱스트린, 시클로덱스트린 등과 같은 통상적인 당, 및 자일리톨, 소르비톨, 에리트리톨 등의 당알콜이다. 상술한 것 이외의 향미제로서 천연 향미제(타우마틴, 스테비아 추출물(예를 들어 레바우디오시드 A, 글리시르히진등))및 합성 향미제(사카린, 아스파르탐 등)를 유리하게 사용할 수 있다. 상기 천연 탄수화물의 비율은 본 발명의 조성물 100㎖당 일반적으로 약 1 내지 20g, 바람직하게는 약 5 내지 12g이다.The health functional beverage composition of the present invention is not particularly limited to the ingredients other than the above-mentioned extract or compound as an essential ingredient in the indicated ratios and may contain various flavors or natural carbohydrates as an additional ingredient have. Examples of the above-mentioned natural carbohydrates include monosaccharides such as glucose, fructose and the like; Disaccharides such as maltose, sucrose and the like; And polysaccharides, for example, conventional sugars such as dextrin, cyclodextrin and the like, and sugar alcohols such as xylitol, sorbitol and erythritol. As natural flavors other than those described above, natural flavors (such as tau martin, stevia extract (e.g., rebaudioside A, glycyrrhizin)) and synthetic flavors (saccharin, aspartame, etc.) have. The ratio of the natural carbohydrate is generally about 1 to 20 g, preferably about 5 to 12 g per 100 ml of the composition of the present invention.
또한, 본 발명은 엔테로 바이러스에 기인한 질환의 개선을 위한 황금 추출물 또는 이로부터 분리된 노르우고닌(norwogonin), 오록실린(oroxylin) A, 및 모슬로플라본(mosloflavone)으로 구성된 군으로부터 선택된 화합물을 주성분으로 함유하는 건강보조식품을 제공한다.The present invention also relates to a method for the treatment of diseases caused by enterovirus, comprising the step of administering a compound selected from the group consisting of a gold extract for the improvement of diseases caused by enterovirus or isolated therefrom, norwogonin, oroxylin A, and mosloflavone Provide health supplements containing the main ingredient.
또한, 본 발명은 엔테로 바이러스에 기인한 질환의 개선을 위한 황금 추출물 또는 이로부터 분리된 노르우고닌(norwogonin), 오록실린(oroxylin) A, 및 모슬로플라본(mosloflavone)으로 구성된 군으로부터 선택된 화합물을 주성분으로 함유하는 식품 또는 식품첨가물을 제공한다.The present invention also relates to a method for the treatment of diseases caused by enterovirus, comprising the step of administering a compound selected from the group consisting of a gold extract for the improvement of diseases caused by enterovirus or isolated therefrom, norwogonin, oroxylin A, and mosloflavone And a food or food additive containing the main ingredient.
또한 상기 건강기능식품은 식품첨가물을 추가로 포함할 수 있으며, "식품첨가물"로서의 적합여부는 다른 규정이 없는 한 식품의약품 안정청에 승인된 식품첨가물공전의 총칙 및 일반시험법 등에 따라 해당 품목에 관한 규격 및 기준에 의하여 판정한다. In addition, the health functional food may further include food additives, and the suitability of the food functional food as a "food additive" Standards and standards.
상기 "식품첨가물공전"에 수재된 품목으로 예를 들어, 케톤류, 글리신, 구연산칼륨, 니코틴산, 계피산 등의 화학적 합성품, 감색소, 감초추출물, 결정셀롤로오스, 구아검 등의 천연첨가물, L-글루타민산나트륨제제, 면류첨가알칼리제, 보존료제제, 타르색소제제 등의 혼합 제제류들을 들 수 있다.Examples of the products listed in the above-mentioned "food additives" include natural products such as ketones, chemical products such as glycine, potassium citrate, nicotinic acid and cinnamic acid, coloring matter, licorice extract, crystalline cellulose, guar gum, Sodium laurate, sodium glutamate preparation, noodles-added alkaline agent, preservative agent, tar pigment preparation and the like.
본 발명의 추출물 또는 화합물이 포함된 기능성 식품으로는 빵, 떡류, 건과류, 캔디류, 초콜릿류, 츄잉껌, 쨈류와 같은 과자류 아이스크림류, 빙과류, 아이스크림 분말류와 같은 아이스크림 제품류 우유류, 저지방 우유류, 유당분해우유, 가공유류, 산양유, 발효유류, 버터유류, 농축유류, 유크림류, 버터유, 자연치즈, 가공치즈, 분유류, 유청류와 같은 유가공품류 식육가공품, 알가공품, 햄버거와 같은 식육제품류 어묵, 햄, 소세지, 베이컨 등의 어육가공품과 같은 어육제품류 라면류, 건면류, 생면류, 유탕면류, 호화건먼류, 개량숙면류, 냉동면류, 파스타류와 같은 면류 과실음료, 채소류음료, 탄산음료, 두유류, 요구르트 등의 유산균음료, 혼합음료와 같은 음료 간장, 된장, 고추장, 춘장, 청국장, 혼합장, 식초, 소스류, 토마토케첩, 카레, 드레싱과 같은 조미식품 마가린, 쇼트닝 및 피자를 들 수 있으나, 이에 제한되는 것은 아니다. Examples of the functional food containing the extract or the compound of the present invention include confectionery ice cream such as bread, rice cake, dried fruit, candy, chocolate, chewing gum and confectionery, ice cream such as ice cream, ice cream powder, low- Dairy products such as cracked milk, processed oil, goat milk, fermented oil, butter oil, concentrated oil, yogurt cream, butter oil, natural cheese, processed cheese, powdered milk, milk products, meat products such as egg products and hamburgers Fish noodles such as ham, sausage, and bacon; noodle products such as ramen noodles, noodle noodles, fresh noodles, noodle noodles, luxury noodles, improved sleep noodles, frozen noodles, noodles such as pasta, Such as beverages, bean paste, red pepper paste, chunks, chonggukjang, mixed berries, vinegar, sauces, tomato ketchup, curry, dressing, etc. US food but are margarine, shortening and pizza, without being limited thereto.
본 발명의 건강 기능성 음료 조성물은 지시된 비율로 필수 성분으로서 상기 추출물 또는 화합물을 함유하는 외에는 다른 성분에는 특별한 제한이 없으며 통상의 음료와 같이 여러 가지 향미제 또는 천연 탄수화물 등을 추가 성분으로서 함유할 수 있다. 상술한 천연 탄수화물의 예는 모노사카라이드, (예를 들어, 포도당, 과당 등); 디사카라이드, (예를 들어 말토스, 슈크로스 등); 및 폴리사카라이드, (예를 들어 덱스트린, 시클로덱스트린 등)과 같은 통상적인 당, 및 자일리톨, 소르비톨, 에리트리톨 등의 당알콜이다. 상술한 것 이외의 향미제로서 천연 향미제(타우마틴, 스테비아 추출물(예를 들어 레바우디오시드 A, 글리시르히진 등)) 및 합성 향미제(사카린, 아스파르탐 등)를 유리하게 사용할 수 있다. 상기 천연 탄수화물의 비율은 본 발명의 조성물 100 ㎖ 당 일반적으로 약 1~20 g, 바람직하게는 약 5~12 g이다.The health functional beverage composition of the present invention is not particularly limited to the ingredients other than the above-mentioned extract or compound as an essential ingredient in the indicated ratios and may contain various flavors or natural carbohydrates as an additional ingredient have. Examples of the above-mentioned natural carbohydrates include monosaccharides (e.g., glucose, fructose, etc.); Disaccharide, (e.g., maltose, sucrose, etc.); And polysaccharides (for example, dextrin, cyclodextrin and the like), and sugar alcohols such as xylitol, sorbitol and erythritol. As natural flavors other than those described above, natural flavors (such as tau martin, stevia extract (e.g., rebaudioside A, glycyrrhizin)) and synthetic flavors (saccharin, aspartame, etc.) have. The ratio of the natural carbohydrate is generally about 1 to 20 g, preferably about 5 to 12 g per 100 ml of the composition of the present invention.
상기 외에 본 발명의 추출물 또는 화합물은 여러 가지 영양제, 비타민, 광물(전해질), 합성 풍미제 및 천연 풍미제 등의 풍미제, 착색제 및 중진제(치즈, 초콜릿 등), 펙트산 및 그의 염, 알긴산 및 그의 염, 유기산, 보호성 콜로이드 증점제, pH 조절제, 안정화제, 방부제, 글리세린, 알코올, 탄산음료에 사용되는 탄산화제 등을 함유할 수 있다. 그밖에 본 발명의 추출물 또는 화합물은 천연 과일 쥬스 및 과일 쥬스 음료 및 야채 음료의 제조를 위한 과육을 함유할 수 있다. 이러한 성분은 독립적으로 또는 조합하여 사용할 수 있다. 이러한 첨가제의 비율은 그렇게 중요하진 않지만 본 발명의 추출물 100 중량부 당 0 내지 약 20 중량부의 범위에서 선택되는 것이 일반적이다.In addition to the above, the extract or the compound of the present invention can be used as a flavoring agent such as various nutrients, vitamins, minerals (electrolytes), synthetic flavors and natural flavors, coloring agents and intermediates (cheese, chocolate etc.), pectic acid and its salts, And salts thereof, organic acids, protective colloid thickeners, pH adjusting agents, stabilizers, preservatives, glycerin, alcohols, carbonating agents used in carbonated drinks, and the like. In addition, the extract or the compound of the present invention may contain natural fruit juice and pulp for the production of fruit juice drinks and vegetable drinks. These components may be used independently or in combination. The proportion of such additives is not so critical, but is generally selected in the range of 0 to about 20 parts by weight per 100 parts by weight of the extract of the present invention.
상기에 언급한 바와 같이, 본 발명의 황금 추출물 및 이로부터 분리된 화합물은 (1) 베로(vero) 세포에서의 세포독성 및 EV71, CVB3, CVA16의 항바이러스 활성실험, 세포병변 억제실험(실험예 1); (2) EV71에 대한 항바이러스 활성을 확인하기 위한 enterovirus 71의 VP단백질에 대한 Western blot 분석법 (실험예 2); (3) replicon system(pRIBFluc-EV71)을 이용한 Replicon 분석법을 통한 항바이러스 활성 메카니즘 분석실험 (실험예 3); (4) BALB/c 마우스를 이용한 CVB3 바이러스에 대한 항바이러스 활성 측정을 위한 in vivo 동물실험(실험예 4) 등의 광범위한 시험관내 실험(in vitro test) 및 생체내 동물실험(in vivo test)를 통하여, 본 발명의 상기 시료들이 강력한 항 엔테로바이러스 활성을 나타냄을 확인함으로, 상기 조성물을 엔테로 바이러스에 기인한 질환의 예방 및 치료용 약학조성물 또는 건강기능식품으로 유용하다.As mentioned above, the gold extract of the present invention and the compounds isolated therefrom are (1) cytotoxicity in vero cells and antiviral activity tests of EV71, CVB3 and CVA16, One); (2) Western blot analysis of the VP protein of enterovirus 71 to confirm antiviral activity against EV71 (Experimental Example 2); (3) Analysis of antiviral activity mechanism through replicon analysis using replicon system (pRIBFluc-EV71) (Experimental Example 3); (4) in vitro test and in vivo test such as in vivo animal experiment (Example 4) for the antiviral activity measurement of CVB3 virus using BALB / c mouse By confirming that the samples of the present invention exhibit strong anti-enterovirus activity, the composition is useful as a pharmaceutical composition or health functional food for the prevention and treatment of diseases caused by enteroviruses.
도 1는 본 발명의 시료의 EV71 감염에 의한 세포 독성에 미치는 효과를 나타낸 도이며(여기에서, (A) 비감염 세포(Noninfected cells); (B) norwogonin 시료 처치 비감염 세포(noninfected cells treated with norwogonin); (C) oroxylin A 시료 처치 비감염세포(noninfected cells treated with oroxylin A); (D) mosloflavone 시료 처치 비감염세포(noninfected cells treated with mosloflavone); (E) 리바비린 처치 비감염세포(noninfected cells treated with ribavirin); (F) EV71-감염 세포(EV71-infected cells); (G) norwogonin 시료 EV71-감염 세포 (EV71-infected cells treated with norwogonin); (H) oroxylin A 시료 EV71-감염 세포 (EV71-infected cells treated with oroxylin A); (I) mosloflavone 시료 EV71-감염 세포 (EV71-infected cells treated with mosloflavone); (J) 리바비린 처치 EV71-감염 세포 (EV71-infected cells treated with ribavirin)을 각각 나타냄);
도 2는 본 발명의 시료의 CVB3 감염에 의한 세포 독성에 미치는 효과를 나타낸 도이며(여기에서, (A) 비감염 세포(Noninfected cells); (B) norwogonin 시료 처치 비감염 세포(noninfected cells treated with norwogonin); (C) oroxylin A 시료 처치 비감염세포(noninfected cells treated with oroxylin A); (D) mosloflavone 시료 처치 비감염세포(noninfected cells treated with mosloflavone); (E) 리바비린 처치 비감염세포(noninfected cells treated with ribavirin); (F) CB3-감염 세포(CB3-infected cells); (G) norwogonin 시료 CB3-감염 세포 (CB3-infected cells treated with norwogonin); (H) oroxylin A 시료 CB3-감염 세포 (CB3-infected cells treated with oroxylin A); (I) mosloflavone 시료 CB3-감염 세포 (CB3-infected cells treated with mosloflavone); (J) 리바비린 처치 CB3-감염 세포 (CB3-infected cells treated with ribavirin)을 각각 나타냄);
도 3는 본 발명의 시료의 CVA16 감염에 의한 세포 독성에 미치는 효과를 나타낸 도이며(여기에서, (A) 비감염 세포(Noninfected cells); (B) norwogonin 시료 처치 비감염 세포(noninfected cells treated with norwogonin); (C) oroxylin A 시료 처치 비감염세포(noninfected cells treated with oroxylin A); (D) mosloflavone 시료 처치 비감염세포(noninfected cells treated with mosloflavone); (E) 리바비린 처치 비감염세포(noninfected cells treated with ribavirin); (F) CVA16-감염 세포(CVA16-infected cells); (G) norwogonin 시료 CVA16-감염 세포 (CVA16-infected cells treated with norwogonin); (H) oroxylin A 시료 CVA16-감염 세포 (CVA16-infected cells treated with oroxylin A); (I) mosloflavone 시료 CVA16-감염 세포 (CVA16-infected cells treated with mosloflavone); (J) 리바비린 처치 CVA16-감염 세포 (CVA16-infected cells treated with ribavirin)을 각각 나타냄);
도 4는 본 발명의 시료의 EV71에 대한 항바이러스 활성을 나타낸 도이며(결과는 독립적인 삼중 실험치의 백분율 수치의 형균(mean) ± S.D.로 나타냄);
도 5는 본 발명의 시료의 CVB3에 대한 항바이러스 활성을 나타낸 도이며(결과는 독립적인 삼중 실험치의 백분율 수치의 형균(mean) ± S.D.로 나타냄);
도 6는 본 발명의 시료의 CVA16에 대한 항바이러스 활성을 나타낸 도이며(결과는 독립적인 삼중 실험치의 백분율 수치의 형균(mean) ± S.D.로 나타냄);
도 7는 본 발명의 시료의 EV71 바이러스 Capside 단백질 발현에 미치는 영향을 나타낸 도이며;
도 8는 본 발명의 시료의 EV71 바이러스 복제(replication) 및 번역(translation)에 미치는 영향을 나타낸 도이며;
도 9는 CVB3 감염된 BALB/c 마우스에서 황금 추출물 및 oroxylin A 투여에 의한 마우스 체중 변화를 측정한 도이며;
도 10은 CVB3 감염된 BALB/c 마우스에서 황금 추출물 및 oroxylin A 투여에 의한 췌장 조직 분석를 수행한 도이며; (A) A : 비감염군; B : 바이러스 감염군; C : 황금 methanol 추출물 처치 바이러스 감염군; D : oroxylin A 시료 처치 바이러스 감염군 (B) 췌장의 acini cell 수를 나타냄.1 is a graph showing the effect of a sample of the present invention on cytotoxicity caused by EV71 infection, wherein (A) noninfected cells, (B) norwogonin noninfected cells treated with norwogonin, ; (C) nonoxed cells treated with oroxylin A; (D) noninfected cells treated with oroxylin A; (D) noninfected cells treated with mosloflavone; (E) ribavirin treated with ribavirin; (EV71-infected cells treated with norwogonin) (EV71-infected cells) (EV71-infected cells) (EV71-infected cells treated with norwogonin) (I) EV71-infected cells treated with mosloflavone; (J) EV71-infected cells treated with ribavirin);
FIG. 2 shows the effect of the present invention on cytotoxicity by CVB3 infection (A) noninfected cells; (B) noninfected cells treated with norwogonin (B) ; (C) nonoxed cells treated with oroxylin A; (D) noninfected cells treated with oroxylin A; (D) noninfected cells treated with mosloflavone; (E) ribavirin treated with ribavirin; CB3-infected cells (CB3-infected cells); (G) norwogonin CB3-infected cells treated with norwogonin; (H) oroxylin A sample CB3-infected cells (J) CB3-infected cells treated with ribavirin, respectively); (iii) moxifloxacin, oroxylin A; (i) mosloflavone CB3-infected cells treated with mosloflavone;
FIG. 3 is a graph showing the effect of the present invention on cytotoxicity caused by CVA16 infection (A) noninfected cells; (B) noninfected cells treated with norwogonin (B) ; (C) nonoxed cells treated with oroxylin A; (D) noninfected cells treated with oroxylin A; (D) noninfected cells treated with mosloflavone; (E) ribavirin treated with ribavirin; (F) CVA16-infected cells (G) norwogonin sample CVA16-infected cells treated with norwogonin; (H) oroxylin A sample CVA16-infected cells (J) CVA16-infected cells treated with ribavirin, respectively); (iv) moxifloxacin, oroxylin A; (I) mosloflavone sample CVA16-infected cells treated with mosloflavone;
Figure 4 shows the antiviral activity of the sample of the present invention against EV71 (the results are expressed as the mean ± SD of the percentage values of the independent triplicate experiments);
Figure 5 shows the antiviral activity of the samples of the present invention against CVB3 (the results are expressed as the mean ± SD of percentages of independent triplicate experiments);
Figure 6 is a graph depicting the antiviral activity of the samples of the invention against CVA16 (the results are expressed as the mean ± SD of percentages of independent triplicate experiments);
7 is a graph showing the effect of the sample of the present invention on the expression of EV71 virus Capside protein;
Figure 8 shows the effect of the sample of the present invention on EV71 viral replication and translation;
FIG. 9 is a graph showing changes in mouse body weight by administration of gold extract and oroxylin A in CVB3-infected BALB / c mice;
FIG. 10 shows pancreatic tissue analysis by gold extract and oroxylin A administration in CVB3-infected BALB / c mice; (A) A: Non-infected group; B: Virus infected group; C: Golden methanol extract treatment Virus infected group; D: Oroxylin A Sample treatment Virus infection group (B) Number of acini cells in the pancreas.
이하, 본 발명을 하기의 실시예 및 실험예에 의해 상세히 설명한다. Below, The present invention will be described in detail by the following examples and experimental examples.
단, 하기 실시예 및 실험예는 본 발명을 예시하는 것일 뿐, 본 발명의 내용이 하기 실시예 및 실험예에 의해 한정되는 것은 아니다.However, the following examples and experimental examples are illustrative of the present invention, and the content of the present invention is not limited by the following examples and experimental examples.
실시예 1. 황금 추출물 및 분획Example 1. Gold extract and fraction
1-1. 황금의 조추출물의 제조1-1. Preparation of crude extract of gold
청주시 상당구에 위치한 대림건재약업사로부터 구입한 건조한 황금 1.2kg에 메탄올(methanol) 6.0 L를 가하여 실온에서 24시간 침지하여 추출하고 감압농축기를 이용하여 농축하여 메탄올(methanol) 추출물 66.3 g을 (이하, SBM이라 함) 얻어 CVB3에 대한 항바이러스 활성을 측정하였다.6.0 L of methanol was added to 1.2 kg of dry gold purchased from Daelim Construction Materials Co., Ltd. located in Cheongju City, and the mixture was immersed at room temperature for 24 hours. The mixture was concentrated using a vacuum concentrator to obtain 66.3 g of methanol extract (hereinafter referred to as SBM , And the antiviral activity against CVB3 was measured.
1-2. 극성 용매 및 비극성용매 가용 추출물의 분획1-2. Fractions of polar solvent and non-polar solvent soluble extract
실시예 1-1에서 얻은 메탄올 추출물 (66.3 g)을 증류수에 현탁(suspension)하고, 당 업계에 통상적인 분획방법에 따라 클로로포름(chloroform), 에틸아세테이트(ethyl acetate), n-부탄올(BuOH)로 차례대로 분획하고 감압 건조하여 클로로포름 가용 분획물 (15.0g, 이하, SBC라 함),에틸아세테이트 가용 분획물 (18.2 g, 이하, SBE라 함), n-BuOH 가용 분획물 (13.6g, 이하, SBB라 함)을 얻은 후 물 분획(이하, SBW라 함)로 분획하였고 각 분획물들의 항바이러스 활성을 실험한 결과 클로로포름층에서 유의적인 항바이러스 활성을 나타내는 것을 확인 하였다 (표 1).The methanol extract (66.3 g) obtained in Example 1-1 was suspended in distilled water and purified by using chloroform, ethyl acetate and n-butanol (BuOH) according to a conventional fractionation method (15.6 g, hereinafter referred to as SBC), ethyl acetate soluble fraction (18.2 g, hereinafter referred to as SBE) and n-BuOH soluble fraction (13.6 g, hereinafter referred to as SBB) ), And then fractionated into a water fraction (hereinafter referred to as SBW). The antiviral activity of each fraction was examined to find that the chloroform layer showed significant antiviral activity (Table 1).
a Concentration required to reduce cell growth by 50% (μg/mL).
b Concentration required to inhibit virus-induced CPE by 50% (μg/mL).
c Therapeutic index = CC50/IC50
d Not determinedResults are presented as the mean IC 50 values ± SD obtained from three independent experiments carried out in triplicate.
a Concentration required to reduce cell growth by 50% (μg / mL).
b Concentration required to inhibit virus-induced CPE by 50% (μg / mL).
c Therapeutic index = CC 50 / IC 50
d Not determined
1-3. 활성 화합물의 분리1-3. Isolation of active compounds
실시예 1-2에서 항바이러스 활성을 나타낸 chloroform층을 C18 실리카 겔 컬럼 흡착 크로마토그래피 (C-18 silica gel column adsorption chromatography, 2.5 × 25 cm)에 methanol과 water 3:7, 4:6, 6:4, 8:2, 10:0 비율의 혼합용매를 500ml 각각 두 번 용출용매로 이용하여 11개의 분획으로 분리하였다. Fraction 6에서 13번 분획물을 sephadex LH-20 컬럼(25-100 μm, Sigma-Aldrich, Steinheim, Germany)컬럼 크로마토그래피 (2.5 × 170 cm)에 100% methanol을 이용하여 분리 정제하였으며, 활성이 확인된 물질들은 ESI-MS, 1HNMR과 13C NMR 분석을 실시하여 문헌에 기재된 물성티와 비교하여 norwogornin (표 2), oroxylin A (표 3), 그리고 mosloflavone (표 4)으로 각각 그 구조를 동정하였다 [63-65]The chloroform layer exhibiting antiviral activity in Example 1-2 was subjected to C18 silica gel column chromatography (C-18 silica gel column, adsorption chromatography, 2.5 x 25 cm) with methanol and water at 3: 7, 4: 6, 6: 4, 8: 2, and 10: 0 ratios were separated into 11 fractions using two 500 ml elution solvents. Fractions 6 to 13 were isolated and purified by column chromatography (2.5 × 170 cm) on a sephadex LH-20 column (25-100 μm, Sigma-Aldrich, Steinheim, Germany) using 100% methanol. The structures were identified by norwogornin (Table 2), oroxylin A (Table 3), and mosloflavone (Table 4), respectively, by comparing ESI-MS, 1 HNMR and 13 C NMR analysis [63-65]
Norwogornin의Norwogornin's 구조 rescue
OroxylinOroxylin A의 구조 Structure of A
Mosloflavone의Mosloflavone 구조 rescue
a Concentration required to reduce cell growth by 50% (μg/mL).
b Concentration required to inhibit virus-induced CPE by 50% (μg/mL).
c Therapeutic index = CC50/IC50
d Not determinedResults are presented as the mean IC 50 values ± SD obtained from three independent experiments carried out in triplicate.
a Concentration required to reduce cell growth by 50% (μg / mL).
b Concentration required to inhibit virus-induced CPE by 50% (μg / mL).
c Therapeutic index = CC 50 / IC 50
d Not determined
참조예 1. 바이러스와 세포주 및 시약Reference Example 1. Viruses, cell lines and reagents
Enterovirus는 충청남도 보건환경연구원 미생물검사과에서 제공받았으며 37℃에서 vero 세포(CCL-81, ATCC)에서 증식시켰다. Vero 세포는 DMEM media에 10% FBS와 0.01% 항생제를 첨가하여 유지하였다. 항생제와 trypsinEDTA (15400-054), FBS (16000-044) 그리고 DMEM media (12491-015)는 Gibco사 제품을 사용 하였다. Tissue culture dish (353003)는 Falcon사 제품을 사용하였고 sulforhodamine B (SRB(S9012-25G))는 SigmaAldrich에서 구매하였다. Ribavirin (R0182)은 DUCHEFA (Netherlands)사에서 구입하였고 항바이러스 화합물의 용해용액은 DMSO를 사용하였으며, DMEM media에 희석하였다. DMSO의 최종 농도는 세포배양에 전혀 영향이 없는 최대 농도인 0.1%로 사용하였다. 또한 0.1% DMSO는 세포대조군으로 사용하였다.Enterovirus was obtained from the Microbiology Section of the Institute of Health and Environment, Chungnam Province and was propagated in vero cells (CCL-81, ATCC) at 37 ℃. Vero cells were maintained in DMEM medium supplemented with 10% FBS and 0.01% antibiotics. Antibiotics, trypsin EDTA (15400-054), FBS (16000-044) and DMEM media (12491-015) were purchased from Gibco. Tissue culture dish (353003) was purchased from Falcon and sulforhodamine B (SRB (S9012-25G)) was purchased from SigmaAldrich. Ribavirin (R0182) was purchased from DUCHEFA (Netherlands). DMSO was used as a solution for the antiviral compound and diluted in DMEM media. The final concentration of DMSO was used as the maximum concentration of 0.1%, which had no effect on cell culture. 0.1% DMSO was used as a cell control.
실험예 1. 항바이러스 활성 시험Experimental Example 1. Antiviral activity test
상기 실시예 시료의 항바이러스 활성과 세포독성의 측정은 바이러스에 의해 일어나는 세포 병변을 억제시키는 능력에 대하여 SRB assay로 확인하기 위하여 문헌에 기재된 방법을 응용하여 하기와 같이 실험을 수행하였다 [66, 67]. In order to confirm the antiviral activity and cytotoxicity of the sample of the above example by the SRB assay for the ability to inhibit the cell lesion caused by the virus, experiments were conducted as described below by using the method described in the literature [66, 67 ].
1-1. 항바이러스 활성 시험1-1. Antiviral activity test
즉, 96-well culture plate (Nunc, Denmark) 각각의 well에 각 바이러스에 감수성을 갖는 세포를 2 X 104의 수로 준비하였다. 24시간 후 96-well culture plate에 각각의 세포가 90%정도 자랐을 때 실험에 이용하였다. 각 well에 media를 제거한 후, 각 세포에 대하여 PBS로 1회 세척하였다. 그 후, 1% FBS와 각각의 바이러스가 포함된 90μL의 DMEM에 적합한 농도의 norwogonin, oroxylin A, mosloflavone 10μL를 첨가하였다. Norwogonin, oroxylin A, mosloflavone 의 항바이러스 활성은 0.4 μg/mL, 2 μg/mL, 10 μg/mL, 및 50 μg/mL 4개의 농도에서 확인하였다. Namely, each virus-susceptible cell was prepared in each well of a 96-well culture plate (Nunc, Denmark) in a number of 2 × 10 4 . After 24 h, each cell was grown in a 96-well culture plate at 90%. Media was removed from each well and each cell was washed once with PBS. After that, Norwogonin, oroxylin A, and 10 μL of mosloflavone were added to 90 μL of DMEM containing 1% FBS and each virus. Antiviral activity of Norwogonin, oroxylin A, and mosloflavone was determined at four concentrations of 0.4 μg / mL, 2 μg / mL, 10 μg / mL, and 50 μg / mL.
4개의 well은 화합물을 처리하지 않고 바이러스만 처리한 세포대조구로 사용하였고, 또 다른 4개의 well은 바이러스와 화합물을 모두 처리하지 않은 세포 대조구로 사용하였다. CO2 배양기 (VS-9108MS, Vision, Korea)에서 37℃, 5% CO2의 조건으로 2일 동안 배양 후 세포의 형태를 위상차현미경 (Axiovert 10; Zeiss, Wetzlar, Germany)에서 4 X 10배율로 관찰 한 후 이미지를 기록하였다. Four wells were used as the cell control without virus treatment and the other four wells were used as the cell control without virus and compound treatment. A CO 2 incubator (VS-9108MS, Vision, Korea ) a phase contrast microscope in the form of after incubation for 2 days by 37 ℃, conditions of 5% CO 2 cells; in (Axiovert 10 Zeiss, Wetzlar, Germany ) with 4 X 10 magnification After observation, images were recorded.
1-2. 세포독성 시험1-2. Cytotoxicity test
96 well plates에 배양한 각각의 세포는 바이러스를 처리한 well 옆에 0.4 μg/mL, 2 μg/mL, 10 μg/mL, 및 50 μg/mL 4개의 농도의 norwogonin, oroxylin A, 및 mosloflavone 를 처리 한 후 37℃에서 2일 동안 CO2 배양기에 배양 한 후 SRB assay로 세포독성을 평가하였다.Each cell cultured in 96-well plates was treated with four concentrations of norwogonin, oroxylin A, and mosloflavone at concentrations of 0.4 μg / mL, 2 μg / mL, 10 μg / mL, and 50 μg / mL, After incubation at 37 ° C for 2 days in a CO 2 incubator, cytotoxicity was evaluated by SRB assay.
1-3. 실험 결과1-3. Experiment result
황금 methanol 추출물 및 분획물들의 CVB3에 대한 항바이러스 활성 및 세포독성Antiviral Activity and Cytotoxicity of Gold Methanol Extracts and Fractions on CVB3
황금 methanol 추출물을 이용하여 chloroform, ethyl acetate, butanol, water층으로 분획하였고 황금 methanol 추출물 및 각 분획층을 이용하여 CVB3에 대하여 항바이러스 활성을 실험을 진행하였다. 황금 methanol 추출물 및 각 분획층의 활성 실험 농도는 50 μg/mL, 10 μg/mL, 2 μg/mL 및 0.4 μg/mL을 사용 하였다. 각각의 추출물 및 분획층의 세포독성은 실험에 사용한 최대 약제 농도인 50 μg/mL에서 water 분획층을 제외한 모든 분획층에서 세포독성을 나타내었다. 그러나 10 μg/mL의 약제 농도에서는 추출물 및 각각의 분획층에서 모두 세포독성을 나타내지 않았다. 항바이러스 활성 실험결과 CVB3에 대하여 10 μg/mL 농도의 황금 methanol 추출물 및 chloroform 분획층에서는 약 50%의 항바이러스 활성을 나타내었으나 ethyl acetate, butanol, water 분획층에서는 항바이러스 활성을 나타내지 않았다. CVB3에 대하여 황금 methanol 추출물 및 chloroform 분획층의 IC50 (약제의 50% 억제농도) 값은 각각 9.35 μg/mL, 9.76 μg/mL 값을 나타내었다 (표 1). The methanol extracts were fractionated into chloroform, ethyl acetate, butanol and water. The anti - viral activity of CVB3 was examined by using golden methanol extract and each fraction. The concentrations of 50 μg / mL, 10 μg / mL, 2 μg / mL and 0.4 μg / mL of gold methanol extract and each fraction were used. The cytotoxicity of each extract and fraction layer was cytotoxic in all the fraction layers except the water fraction layer at the maximum drug concentration of 50 μg / mL used in the experiment. However, at the concentration of 10 μg / mL, neither the extract nor the respective fraction layers showed cytotoxicity. Antiviral activity The antiviral activity of CVB3 was about 50% in the golden methanol extract and chloroform fraction at the concentration of 10 μg / mL, but did not show any antiviral activity in the ethyl acetate, butanol and water fractions. The IC 50 (50% inhibitory concentration) values of the golden methanol extract and the chloroform fraction of CVB3 were 9.35 μg / mL and 9.76 μg / mL, respectively (Table 1).
EV71, CVB3, CVA16에 대한 norwogonin, oroxylin A 와 mosloflavone의 항바이러스 활성과 세포독성Antiviral activity and cytotoxicity of norwogonin, oroxylin A and mosloflavone against EV71, CVB3, and CVA16
Norwogonin, oroxylin A 및 mosloflavone에 대하여 세포독성과 EV71, CVB3, CVA16의 항바이러스 활성을 측정하였다. 사용된 Vero 세포에 대하여 norwogonin, oroxylin A 와 mosloflavone 모두의 CC50은 실험한 최대 농도인 50 μg/mL에서는 나타나지 않았다. 바이러스 활성을 50% 억제하는 항바이러스 효과를 나타내는 IC50은 EV71에 대하여 norwogonin은 31.9 μg/mL, oroxylin A는 20.6 μg/mL, mosloflavone은 27.8 μg/mL의 값을 보였고 CVB3에는 norwogonin은 13.5 μg/mL, oroxylin A는 3.17 μg/mL, mosloflavone은 3.92 μg/mL 보였다. 그러나 CVA16에 대하여 oroxylin A는 17.5 μg/mL의 IC50 값을 나타내었으나 norwogonin, mosloflavone은 50%이상의 항바이러스 활성을 나타내지 않았다. 또한 양성대조군으로 사용한 ribavirin에서는 EV71, CVB3, CVA16 모든 바이러스에 대하여 50%이상의 항바이러스 활성을 나타내지 않았다 (표 4). Norwogonin, oroxylin A and mosloflavone were measured for cytotoxicity and antiviral activities of EV71, CVB3 and CVA16. The CC 50 of norwogonin, oroxylin A, and mosloflavone were not shown at the maximum concentration of 50 μg / mL in the Vero cells used. The IC 50 values showing antiviral effects that inhibit viral activity by 50% were 31.9 μg / mL for norwogonin, 20.6 μg / mL for oroxylin A, 27.8 μg / mL for mosloflavone, and 13.5 μg / mL, oroxylin A and mosloflavone were 3.17 μg / mL and 3.92 μg / mL, respectively. However, for the CVA16, oroxylin A showed an IC 50 value of 17.5 μg / mL, while norwogonin and mosloflavone showed no antiviral activity of more than 50%. In addition, ribavirin used as a positive control did not show more than 50% antiviral activity against all viruses of EV71, CVB3, and CVA16 (Table 4).
Norwogonin, oroxylin A 와 mosloflavone의 EV71, CVB3, CVA16에 대한 세포병변 억제 효과Cellular lesion inhibition effect of Norwogonin, oroxylin A and mosloflavone on EV71, CVB3, and CVA16
Vero 세포에 EV71 (도 1), CVB3 (도 2), CVA16 (도 3)를 감염 시키고 2일 후 세포병변을 현미경을 이용하여 이미지화 하였다. 세포에 바이러스를 감염시키지 않고 약제도 처리 한지 않은 정상대조군(도 1A, 도 2A 및 도 3A)과 바이러스 감염 없이 norwogonin 50μg/mL을 처리한 군 (도 4B, 도 5B 및 도 6B), oroxylin A 50μg/mL을 처리한 군 (도 1C, 도 2C 및 도 3C), mosloflavone 50μg/mL을 처리한 군 (도 1D, 도 2D 및 도 3D)과 ribavirin 50μg/mL을 처리한 군 (도 1E, 도 2E 및 도 3E)에서 정상대조군과 같이 정상적인 세포의 모양을 보여 주었다. Vero cells were infected with EV71 (Fig. 1), CVB3 (Fig. 2), and CVA16 (Fig. 3). After 2 days, cell lesions were imaged using a microscope. (FIG. 1A, FIG. 2A, and FIG. 3A) and the group treated with 50 μg / mL norwogonin without virus infection (FIG. 4B, FIG. 5B and FIG. 6B), 50 μg of oroxylin A (Fig. 1C, Fig. 2C and Fig. 3C) treated with 50 袖 g / mL of mosloflavone and the group treated with 50 袖 g / mL ribavirin And Fig. 3E) showed normal cell shapes as in the normal control group.
이 결과로 Norwogonin, oroxylin A, mosloflavone과 ribavirin은 세포독성을 나타내지 않는다는 것을 확인하였다. EV71, CVB3, CVA16을 감염시키고 약제를 처리하지 않은 감염대조군 (도 1F, 도 2F 및 도 3F), EV71, CVB3, CVA16을 감염시키고 norwogonin 50μg/mL을 처리한 군 (도 1G, 도 2G 및 도 3G), oroxylin A 50μg/mL을 처리한 군 (도 1H, 도 2H 및 도 3H), mosloflavone 50μg/mL을 처리한 군 (도 1I, 도 2I 및 도 3I)과 ribavirin 50μg/mL을 처리한 군 (도 1J, 도 2J 및 도 3J)에서 감염대조군과 ribavirin 처리군은 각각의 바이러스에 의한 세포병변을 나타내었다. Norwogonin, oroxylin A, mosloflavone은 EV71, CVB3 모두에 세포병변을 억제하여 정상적인 세포모양을 보여 주었다. As a result, Norwogonin, oroxylin A, mosloflavone and ribavirin were not cytotoxic. (Fig. 1F, Fig. 2F and Fig. 3F) infected with EV71, CVB3 and CVA16 and treated with 50 μg / ml of norwogonin (Fig. 1H, Fig. 2H and Fig. 3H) treated with 50 μg / mL of oroxylin A and 50 μg / mL of ribavirin treated with 50 μg / mL of mosloflavone (Fig. 1J, Fig. 2J and Fig. 3J), the infection control group and the ribavirin treatment group showed cell lesions caused by each virus. Norwogonin, oroxylin A, and mosloflavone inhibited cell lesions in both EV71 and CVB3, and showed normal cell morphology.
그러나 CVA16에 대하여 oroxylin A는 세포병변을 억제하였으나 norwogonin, mosloflavone은 세포병변을 억제하지 못하였다. 각각의 군을 이미지화한 후 microplate reader를 이용하여 cell viability를 측정하였다. EV71에 대하여 Norwogonin, oroxylin A, mosloflavone은 모두 60% 이상의 cell viability 보였고 (도 4), CVB3에는 각각의 compound가 50% 이상의 cell viability를 보였다 (도 5). 그러나 CVA16에는 oroxylin A만 50% 이상의 cell viability를 보였다 (도 6).However, for CVA16, oroxylin A inhibited cell lesion, but norwogonin and mosloflavone did not inhibit cell lesion. Each group was imaged and cell viability was measured using a microplate reader. Norwogonin, oroxylin A, and mosloflavone showed more than 60% cell viability for EV71 (FIG. 4), and each compound showed more than 50% cell viability for CVB3 (FIG. 5). In CVA16, however, only oroxylin A showed cell viability of more than 50% (Fig. 6).
실험예 2. VP-Western blot 분석 시험Experimental Example 2. VP-Western blot analysis test
EV71에 대하여 norwogonin, oroxylin A, 및 mosloflavone의 항바이러스 활성을 확인하기 위하여 문헌에 기재된 enterovirus 71의 VP단백질에 대한 Western blot분석법을 응용하여 하기와 같이 실험을 수행하였다 [68]. In order to confirm the antiviral activity of norwogonin, oroxylin A, and mosloflavone against EV71, Western blot analysis of the VP protein of enterovirus 71 described in the literature was applied as follows [68].
2-1. 실험과정2-1. Experimental course
Vero 세포는 6-well culture plate에 well당 5 X 105 개의 세포농도로 배양하였다. 24시간 후에 배양용액을 제거한 후 PBS로 세척하였다. 그 후 1% FBS가 포함된 900μL의 바이러스 배양액 (media)에 norwogonin, oroxylin A, 및 mosloflavone 과 ribavirin을 50μg/mL농도가 되게 100μL 첨가하였다. 그 후 37℃, 5% CO2 배양기에 48시간 동안 배양 후 RIPA lysis buffer(Cat. Number 89900, Pierce)를 이용하여 세포를 용해시켰다. 그리고 용해된 세포를 원심분리하여 단백질이 포함된 상층액만 분리하였다. 단백질이 포함된 상층액을 10분 동안 100℃ 에서 가열한 후 12% 아크릴아미드 겔 (acrylamide gel, Cat. Number 456-1043, BIO-RAD)을 이용하여 100V 에서 1시간 동안 전기영동을 실시하였다. 그 후 기기 (iBlotGel Transfer Device, Invitrogen, Carlsbad, CA)를 이용하여 20V에서 7분 동안 acrylamide gel에 있는 단백질을 iBlotTransfer Stack, PVDF, regular-size(IB401001, invitrogen)으로 옮겨 주었다. membrane은 5 % skim milk (232100, Difco)에 상온에서 1시간 동안 반응 시킨 후 PBST(Phosphate buffer saline Tween-20)로 3번 세척해 주었다. 그 후 mouse anti-enterovirus 71 monoclonal antibody (MAB 979, Millipore)를 5% skim milk에 1:1000의 비율로 희석한 1차 항체를 상온에서 2시간동안 membrane에 반응시킨 후 다시 PBST로 3번 세척해 주었다. 이 실험에서 대조군으로 사용한 α-Tubulin은 mouse monoclonal IgG1 (SC-32293, Santa Cruz) 항체를 1차 항체로 사용하여 같은 방법으로 수행하였다. Enterovirus 71의 VP단백질과 대조군인 α-Tubulin을 확인하기 위한 2차 항체는 polyclonal goat anti-mouse IgG(H+L) HRP (SA001-500, GenDEPOT)를 사용하였다. polyclonal goat anti-mouse IgG(H+L) HRP를 5% skim milk에 1:5000의 비율로 희석한 후 상온에서 1시간동안 membrane에 반응 시킨 후, PBST로 3번 세척하고 측정기기(ChemiDoc XRS Plus Imaging System, BIO-RAD,Hercules, CA, USA)을 이용하여 측정하였다. Vero cells were cultured in 6-well culture plates at 5 × 10 5 cells per well. After 24 hours, the culture solution was removed and washed with PBS. Then, 100 μL of norwogonin, oroxylin A, and mosloflavone and ribavirin were added to 900 μL of virus culture medium containing 1% FBS at a concentration of 50 μg / mL. Cells were then lysed in RIPA lysis buffer (Cat. No. 89900, Pierce) at 37 ° C in a 5% CO 2 incubator for 48 h. The dissolved cells were centrifuged to separate only the supernatant containing the protein. The protein-containing supernatant was heated at 100 ° C. for 10 minutes and then electrophoresed at 100 V for 1 hour using 12% acrylamide gel (Cat No. 456-1043, BIO-RAD). The protein in acrylamide gel was then transferred to iBlotTransfer Stack, PVDF, and regular-size (IB401001, Invitrogen) at 20V for 7 min using a device (iBlotGel Transfer Device, Invitrogen, Carlsbad, CA). The membrane was incubated in 5% skim milk (232100, Difco) for 1 hour at room temperature and then washed three times with PBST (Phosphate buffer saline Tween-20). The primary antibody diluted 1: 1000 in 5% skim milk was reacted with the mouse anti-enterovirus 71 monoclonal antibody (MAB 979, Millipore) for 2 hours at room temperature and then washed three times with PBST gave. In this experiment, α-tubulin, which was used as a control, was subjected to the same method using mouse monoclonal IgG1 (SC-32293, Santa Cruz) as a primary antibody. The secondary antibody to identify the VP protein of Enterovirus 71 and α-Tubulin as the control group was polyclonal goat anti-mouse IgG (H + L) HRP (SA001-500, GenDEPOT). polyclonal goat anti-mouse IgG (H + L) HRP was diluted in 5% skim milk at a ratio of 1: 5000 and reacted at room temperature for 1 hour. Then, the cells were washed 3 times with PBST, Imaging System, BIO-RAD, Hercules, CA, USA).
2-2. Norwogonin, oroxylin A 와 mosloflavone의 EV71 VP 단백질 발현 억제 효과2-2. Inhibitory Effect of Norwogonin, oroxylin A and mosloflavone on EV71 VP Protein Expression
Norwogonin, oroxylin A 와 mosloflavone의 EV71에 대한 항바이러스 활성을 Western blot분석을 통하여 확인 하였다. EV71 감염 48시간 후 EV71의 VP 단백질을 확인하였다. Norwogonin, oroxylin A 와 mosloflavone은 EV71 감염 48시간 후 각각의 바이러스 VP 단백질의 발현을 억제하였다. 그러나 대조약제로 사용한 ribavirin은 50μg/mL의 농도에서 각각의 바이러스 VP단백질의 발현을 억제하지 못하였다 (도 7).Antiviral activity of norwogonin, oroxylin A and mosloflavone against EV71 was confirmed by Western blot analysis. After 48 hours of EV71 infection, the VP protein of EV71 was identified. Norwogonin, oroxylin A and mosloflavone inhibited the expression of the respective viral VP proteins 48 hours after EV71 infection. However, ribavirin used as a control agent did not inhibit the expression of each viral VP protein at a concentration of 50 μg / mL (FIG. 7).
결국, 세포내에서 CPE 억제 실험과 western blot을 통하여 norwogonin, oroxylin A 및 mosloflavone이 EV71, CVB3, CVA16에 대한 항바이러스 활성을 확인하였다.Finally, norwogonin, oroxylin A and mosloflavone showed antiviral activity against EV71, CVB3 and CVA16 through CPE inhibition experiments and western blot.
실험예 3. 항바이러스 활성 메카니즘 분석 시험Experimental Example 3. Antiviral Activity Mechanism Analysis Test
Norwogonin, oroxylin A 와 mosloflavone의 항바이러스 활성 메카니즘을 분석하기 위해 Frank J. M. van Kuppeveld 그룹으로부터 제공 받은 replicon system(pRibFluc-EV71)을 이용하여 문헌에 기재된 Replicon 분석법을 응용하여 하기와 같이 실험을 수행하였다 [69]. To analyze the antiviral activity mechanism of norwogonin, oroxylin A and mosloflavone, replicon analysis method described in the literature was applied using the replicon system (pRibFluc-EV71) provided by Frank JM van Kuppeveld group as follows [69 ].
3-1.실험과정3-1. Experimental Process
pRibFluc-EV71은 EV71의 P1 capside coding 부위가 firefly luciferase gene으로 대체되어서 세포내에서 virus의 life cycle중 entry, penetration, uncoating, assembly, release등을 제외한 replication, translation에 대한 효과만 명확하게 관찰할 수 있는 system이다 [69].pRibFluc-EV71 replaces the P1 capside coding region of EV71 with a firefly luciferase gene, which can clearly observe the effects of replication and translation except entry, penetration, uncoating, assembly, and release in the virus life cycle system [69].
pRibFluc-EV71 plasmid를 MluI enzyme(1071A, TaKaRa)을 이용하여 linearize하고, T7 RNA polymerase(P1280, promega)에 의해 in vitro transcription을 수행 하였다. Transcription된 RNA를 vero cell에 x-treme(04476093001, Roche))을 이용하여 2μg trasfection한 후 norwogonin, oroxylin A, mosloflavone를 10μg/mL농도로 8시간 처리하였다. 그 후 one-glo(E6120, Promega)를 이용하여 firefly luciferase activity를 측정하다.Plasmid pRibFluc-EV71 was linearized with MluI enzyme (1071A, TaKaRa) and in vitro transcription was performed with T7 RNA polymerase (P1280, promega). Transcribed RNA was transfected into vero cells by 2 μg of x-treme (04476093001, Roche) and treated with norwogonin, oroxylin A, and mosloflavone at a concentration of 10 μg / mL for 8 hours. Then, one-glo (E6120, Promega) is used to measure firefly luciferase activity.
3-2. Norwogonin, oroxylin A 와 mosloflavone의 EV71 replication과 traslation 억제 효과3-2. Effects of Norwogonin, oroxylin A and mosloflavone on EV71 replication and traslation
Norwogonin, oroxylin A 와 mosloflavone의 EV71에 대한 replication과 traslation 억제 효과를 replicon system을 이용하여 분석하였다. pRibFluc-EV71을 trasfection한 후 8시간 후에 firefly luciferase activity를 확인하였다. Norwogonin은 8시간 후에 firefly luciferase activity를 약 50% 억제 하였으나, oroxylin A 와 mosloflavone은 firefly luciferase activity를 억제하지 못하였다 (도 8). 반면에 엔테로바이러스 protease 억제제로 알려진 rupintrivir는 동일조건에서 95%이상 firefly luciferase activity를 억제하였다. The replication and traslation inhibitory effects of Norwogonin, oroxylin A and mosloflavone on EV71 were analyzed using a replicon system. The firefly luciferase activity was confirmed 8 hours after trasfection of pRibFluc-EV71. Norwogonin inhibited firefly luciferase activity by about 50% after 8 h, while oroxylin A and mosloflavone did not inhibit firefly luciferase activity (Fig. 8). On the other hand, rupintrivir, known as an enterovirus protease inhibitor, inhibited more than 95% of firefly luciferase activity under the same conditions.
norwogonin, oroxylin A 및 mosloflavone 활성기전을 알아보기 위하여 세포내에서 EV71 replicon system (pRIBFluc-EV71)을 이용하여 이 화합물들의 활성기전을 분석한 결과, norwogonin은 세포내에서 바이러스의 replication 또는 translation에 일정부분 관여 하여 항바이러스 활성을 나타내는 것을 확인하였다. 하지만 이러한 효과가 바이러스 감염 vero세포에서 확인된 항바이러스 효과에 비해서 상대적으로 약한 것을 감안하면 norwogonin이 replication/translation외에 다른 기전을 통해서 항바이러스효과를 나타낼 가능성을 배제할수 없다. 반면에 oroxylin A 및 mosloflavone은 바이러스의 replication 또는 translation에는 관여하지 않는 것을 확인하였다.To investigate the activity of norwogonin, oroxylin A and mosloflavone, we investigated the activation mechanism of these compounds using EV71 replicon system (pRIBFluc-EV71) in cells. As a result, norwogonin was involved in replication or translation of virus Indicating that it exhibits antiviral activity. However, considering that these effects are relatively weak compared to the antiviral effects confirmed in viral infected vero cells, it is not possible to exclude the possibility that norwogonin exhibits antiviral effects through other mechanisms besides replication / translation. Whereas oroxylin A and mosloflavone were not involved in the replication or translation of the virus.
실험예 4. in vivo 항바이러스 활성 시험Experimental Example 4: In vivo antiviral activity test
상기 실시예 시료들의 CVB3 바이러스에 대한 항바이러스 활성을 in vivo 동물실험 상에서 확인하기 위하여 문헌에 기재된 방법을 응용하여 하기와 같이 실험을 수행하였다 [70]. 이 실험에서는 norwogonin, oroxylin A 및 mosloflavone 중에서 세포실험을 통해서 가장 높은 항바이러스 효과를 보이는 것으로 확인된 oroxylin A와 황금 methoanl 추출물을 사용하였다. In order to confirm the antiviral activity against the CVB3 virus of the above-mentioned samples in vivo in an animal experiment, the following experiment was conducted by applying the method described in the literature [70]. In this experiment, oroxylin A and gold methoanl extracts, which were found to have the highest antiviral effect among norwogonin, oroxylin A and mosloflavone, were used in cell experiments.
4-1.실험과정4-1. Experimental Process
CVB3에 대한 황금 methanol 추출물 및 oroxylin A의 항바이러스 활성을 in vivo에서 확인하기 위하여 BALB/c 마우스를 이용하여 실험하였다. In order to confirm the antiviral activity of the golden methanol extract and oroxylin A against CVB3 in vivo , the experiment was carried out using BALB / c mouse.
Male BALB/c 마우스(4주령, 15g)는 ㈜코아텍에서 구입하였다. 구입한 BALB/c 마우스는 1주일 동안 적응시킨 후 정상대조군, 바이러스감염대조군, 바이러스감염 후 황금추출물 투여군, 바이러스 감염 후 oroxylin A 투여군 등 4개의 군으로 군당 5마리씩 분리 하였다. CVB3는 1 × 106 TCID50/100 μL로 복강에 감염 시켰다. 황금 methanol 추출물은 0.5% CMC (Carboxymethyl cellulose) 에 30 mg/kg의 농도로 녹여 경구투여 하였고, oroxylin A는 PBS에 10 mg/kg의 농도로 녹여 복강투여 하였다. 약제 투여는 실험기간인 5일 동안 매일 같은 시간에 투여 하였고, 체중 측정 역시 실험기간 동안 매일 측정 하였다. 실험 종료 후 마우스의 췌장 조직을 이용하여 조직염색 (H&E staining)을 통하여 바이러스에 의한 Acinar cell을 포함한 조직 손상 정도를 확인하였다. Male BALB / c mice (4 weeks old, 15 g) were purchased from Coatec Co., BALB / c mice were divided into four groups: normal control group, virus control group, gold extract group after virus infection, and oroxylin A group after virus infection. CVB3 was infected into the abdominal cavity to 1 × 10 6 TCID 50/100 μL. The golden methanol extract was orally administered to 0.5% CMC (carboxymethyl cellulose) at a concentration of 30 mg / kg, and oroxylin A was dissolved in PBS at a concentration of 10 mg / kg. The drug administration was administered at the same time every day for 5 days, and the body weight was also measured daily during the experiment. After the end of the experiment, the tissue damage (H & E staining) using the pancreas tissue of the mouse was confirmed and the degree of tissue damage including the Acinar cell caused by the virus was confirmed.
4-2. 4-2. In In vivovivo 실험을 통한 Through experiments CVB3에On CVB3 대한 황금 methanol 추출물과 The golden methanol extract and oroxylinoroxylin A의 항바이러스 활성 Antiviral activity of A
세포실험을 통하여 EV71, CVB3, 및 CVA16에 대한 Norwogonin, oroxylin A, mosloflavone의 항바이러스 활성을 확인한 후, In vivo에서의 항바이러스 활성을 확인하기 위하여 CVB3에 감염된 BALB/c 마우스를 이용하여 CVB3에 대한 황금 methanol 추출물과 oroxylin A의 항바이러스 활성을 측정하였다. 현재 enterovirus속에 포함되어 있는 coxsackievirus A, B, 및 enterovirus 중 마우스에 감염을 일으키는 type은 coxsackievirus B가 유일하다. 그러므로 CVB3를 이용하여 마우스 실험을 통해 in vitro에서 EV71, CVB3, 및 CVA16 등 Enterovirus에 대한 광범위 항바이러스 활성을 나타내는 황금 추출물 및 Oroxylin A 등이 실제로 in vivo에서도 활성을 나타내는 지 확인해 보았다. After confirming antiviral activity of Norwogonin, oroxylin A, and mosloflavone against EV71, CVB3, and CVA16 through cell experiments, CVB3-infected BALB / c mice were used to examine the antiviral activity against CVB3 The antioxidant activities of golden methanol extract and oroxylin A were measured. Currently coxsackievirus B is the only type of coxsackievirus A, B, and enterovirus in enterovirus that causes infection in mice. Therefore, we conducted a mouse experiment using CVB3 to examine whether gold extracts and Oroxylin A, which exhibit broad-spectrum antiviral activity against Enteroviruses such as EV71, CVB3, and CVA16 in vitro, are actually active in vivo.
본 실험 결과, 체중은 정상대조군은 정상적으로 증가 하였으나 바이러스감염군은 정상대조군에 비하여 약 10% 정도 감소하였다. 황금 methanol 추출물 투여군과 oroxylin A 투여군 역시 정상대조군에 비하여 약 10% 정도 체중이 감소하였고 바이러스 감염대조군과 유의적인 차이를 보이지 않았다 (도 9). As a result, body weight was increased normally in the normal control group, but the viral infection group was decreased by about 10% as compared with the normal control group. The methanol extract group and the oroxylin A treated group showed a decrease of about 10% in body weight and no significant difference from the virus-infected control group as compared with the normal control group (FIG. 9).
체중에서 두드러진 회복효과가 없음에도 불구하고 조직손상에서 개선효과가 나타나는지를 확인하기 위해서 CVB3 감염에 의해서 가장 두드러지게 나타나는 것으로 잘 알려진 췌장의 조직손상을 분석하였다. 마우스의 췌장을 이용하여 조직 염색을 통하여 바이러스에 의한 조직 손상 정도를 확인한 결과 정상대조군에서는 췌장의 acinal cell이 정상적인 형태를 보였으나 바이러스감염 대조군에서는 바이러스 감염에 의하여 acinal cell이 대부분 손상 되었다. 그러나 황금 methanol 추출물과 oroxylin A를 투여한 군에서는 바이러스 감염 대조군 보다 acinal cell이 덜 손상 받은 것을 확인 할 수 있었다 (도 10). We analyzed the tissue damage of the pancreas, which is most known to be the most prominent by CVB3 infection, in order to confirm the improvement effect of tissue damage, even though there is no significant recovery effect on body weight. The pancreas of the pancreas was used for tissue staining. The acinar cells of the pancreas were normal in the normal control group, but most of the acinar cells were damaged by the viral infection in the viral infection control group. However, in the group treated with golden methanol extract and oroxylin A, acinal cells were less damaged than the virus-infected control group (FIG. 10).
본 연구 결과로 황금 추출물과 황금 chloroform 분획물에서 CVB3에 항바이러스 활성을 나타내었고 황금 chloroform 분획물에서 분리한 norwogonin, oroxylin A 및 mosloflavone의 EV71, CVB3, CVA16에 대한 항바이러스 활성을 확인 하였다. 특히 oroxylin A와 황금추출물의 경우 CBV3 감염 마우스 수준에서도 췌장의 조직손상 개선효과가 나타났다. 그러므로 norwogonin, oroxylin A 및 mosloflavone은 enterovirus에 대한 새로운 항바이러스 후보물질로 사용이 가능할 것으로 기대된다.As a result of this study, antiviral activity of CVB3 was observed in gold extract and gold chloroform fraction, and antiviral activity of norwogonin, oroxylin A and mosloflavone isolated from golden chloroform fractions were confirmed for EV71, CVB3 and CVA16. Especially in the case of oroxylin A and gold extracts, CBV3-infected mice showed improvement of pancreatic tissue damage. Therefore, norwogonin, oroxylin A and mosloflavone are expected to be used as novel antiviral candidates for enteroviruses.
실험예 5. 독성검정Experimental Example 5. Toxicity Test
식약청의 예규에 따라 ICR 마우스 (male, 6 weeks, 오리에트사로부터 구입)를 대상으로 급성독성을 검정하였다. 그 결과, 황금 추출물, 은 300 mg/kg의 경구투여까지 급성독성 (마우스가 죽지 않았다는 것인가)을 보이지 않았다.Acute toxicity was tested in ICR mice (male, 6 weeks, purchased from Aruet) according to KFDA specifications. As a result, the gold extract did not show acute toxicity (the mouse did not die) until oral administration of 300 mg / kg.
이상의 실험예의 결과 황금 추출물은 안전하게 엔테로 바이러스 (influenza virus) 감염증에 사용이 가능함을 확인하였다.As a result of the above experiment, it was confirmed that the gold extract can be safely used for the infection of influenza virus.
본 발명의 추출물 또는 화합물을 아래와 같은 제형으로 투여할 수 있으며, 아래의 제제 실시예는 본 발명을 예시하는 것일 뿐, 이에 의해 본 발명의 내용이 제한되는 것은 아니다.The extract or compound of the present invention can be administered in the form of the following formulation, and the following formulation examples are illustrative of the present invention, and the contents of the present invention are not limited thereto.
제제예 1. 산제의 제조Preparation Example 1. Preparation of powder
SBM 추출물 --------------------------------------- 20 mgSBM extract --------------------------------------- 20 mg
유당 -------------------------------------------- 100 mgLactose -------------------------------------------- 100 mg
탈크 --------------------------------------------- 10 mgTalc --------------------------------------------- 10 mg
상기의 성분들을 혼합하고 기밀포에 충진하여 산제를 제조한다.The above components are mixed and filled in airtight bags to prepare powders.
제제예 2. 정제의 제조Formulation Example 2. Preparation of tablets
SBB 추출물 --------------------------------------- 10 mgSBB extract --------------------------------------- 10 mg
옥수수전분 -------------------------------------- 100 mgCorn starch -------------------------------------- 100 mg
유당 -------------------------------------------- 100 mgLactose -------------------------------------------- 100 mg
스테아린산 마그네슘 ------------------------------- 2 mgMagnesium stearate ------------------------------- 2 mg
상기의 성분들을 혼합한 후 통상의 정제의 제조방법에 따라서 타정하여 정제를 제조한다.After mixing the above components, tablets are prepared by tableting according to the usual preparation method of tablets.
제제예 3. 캡슐제의 제조Formulation Example 3. Preparation of capsules
norwogonin 화합물 -------------------------------- 10 mgnorwogonin compound -------------------------------- 10 mg
결정성 셀룰로오스 --------------------------------- 3 mgCrystalline cellulose --------------------------------- 3 mg
락토오스 --------------------------------------- 14.8 mgLactose --------------------------------------- 14.8 mg
마그네슘 스테아레이트 --------------------------- 0.2 mgMagnesium stearate 0.2 mg < RTI ID = 0.0 >
통상의 캡슐제 제조방법에 따라 상기의 성분을 혼합하고 젤라틴 캡슐에 충진하여 캡슐제를 제조한다.The above components are mixed according to a conventional capsule preparation method and filled in gelatin capsules to prepare capsules.
제제예 4. 주사제의 제조Formulation Example 4. Preparation of injection
SBC 추출물 --------------------------------------- 10 mgSBC extract --------------------------------------- 10 mg
만니톨 ------------------------------------------ 180 mgMannitol ------------------------------------------ 180 mg
주사용 멸균 증류수 ----------------------------- 2974 mgSterile sterile distilled water for injection ----------------------------- 2974 mg
Na2HPO412H2O -------------------------------------- 26 mgNa 2 HPO 4 12H 2 O -------------------------------------- 26 mg
통상의 주사제의 제조방법에 따라 1 앰플당 (2㎖) 상기의 성분 함량으로 제조한다.(2 ml) per 1 ampoule according to the usual injection preparation method.
제제예 5. 액제의 제조Formulation Example 5. Preparation of a liquid preparation
oroxylin A -------------------------------------- 10 mgoroxyline -------------------------------------- 10 mg
이성화당 ----------------------------------------- 10 gIsing Party ----------------------------------------- 10 g
만니톨 -------------------------------------------- 5 gMannitol -------------------------------------------- 5 g
정제수 ------------------------------------------- 적량Purified water -------------------------------------------
통상의 액제의 제조방법에 따라 정제수에 각각의 성분을 가하여 용해시키고 레몬향을 적량 가한 다음 상기의 성분을 혼합한 다음 정제수를 가하여 전체를 100 ㎖로 조절한 후 갈색병에 충진하여 멸균시켜 액제를 제조한다.Each component was added to purified water in accordance with the conventional liquid preparation method and dissolved, and the lemon flavor was added in an appropriate amount. Then, the above components were mixed and then purified water was added thereto to adjust the whole volume to 100 ml. The solution was filled in a brown bottle and sterilized, .
제제예 6. 건강 식품의 제조Formulation Example 6. Preparation of Healthy Foods
SBW 추출물 ----------------------------------- 1000 ㎎SBW Extract ----------------------------------- 1000 mg
비타민 혼합물 ----------------------------------- 적량Vitamin mixture -----------------------------------
비타민 A 아세테이트 ---------------------------- 70 ㎍Vitamin A Acetate ---------------------------- 70 g
비타민 E -------------------------------------- 1.0 ㎎Vitamin E -------------------------------------- 1.0 mg
비타민 B1 ------------------------------------ 0.13 ㎎Vitamin B1 ------------------------------------ 0.13 mg
비타민 B2 ------------------------------------ 0.15 ㎎Vitamin B2 ------------------------------------ 0.15 mg
비타민 B6 ------------------------------------- 0.5 ㎎Vitamin B6 ------------------------------------- 0.5 mg
비타민 B12 ------------------------------------ 0.2 ㎍Vitamin B12 ------------------------------------ 0.2 g
비타민 C --------------------------------------- 10 ㎎Vitamin C --------------------------------------- 10 mg
비오틴 ----------------------------------------- 10 ㎍Biotin ----------------------------------------- 10 μg
니코틴산아미드 -------------------------------- 1.7 ㎎Nicotinic acid amide 1.7 mg
엽산 ------------------------------------------- 50 ㎍Folic acid ------------------------------------------- 50 μg
판토텐산 칼슘 --------------------------------- 0.5 ㎎Calcium pantothenate --------------------------------- 0.5 mg
무기질 혼합물 ----------------------------------- 적량Inorganic mixture -----------------------------------
황산제1철 ------------------------------------ 1.75 ㎎Ferrous sulfate 1.75 mg < RTI ID = 0.0 >
산화아연 ------------------------------------- 0.82 ㎎Zinc oxide - 0.82 mg
탄산마그네슘 --------------------------------- 25.3 ㎎Magnesium carbonate --------------------------------- 25.3 mg
제1인산칼륨 ------------------------------------ 15 ㎎Potassium phosphate monohydrate 15 mg
제2인산칼슘 ------------------------------------ 55 ㎎Secondary calcium phosphate ------------------------------------ 55 mg
구연산칼륨 ------------------------------------- 90 ㎎Potassium citrate ------------------------------------- 90 mg
탄산칼슘 -------------------------------------- 100 ㎎Calcium carbonate -------------------------------------- 100 mg
염화마그네슘 --------------------------------- 24.8 ㎎Magnesium Chloride --------------------------------- 24.8 mg
상기의 비타민 및 미네랄 혼합물의 조성비는 비교적 건강식품에 적합한 성분을 바람직한 실시예로 혼합 조성하였지만, 그 배합비를 임의로 변형 실시하여도 무방하며, 통상의 건강식품 제조방법에 따라 상기의 성분을 혼합한 다음, 과립을 제조하고, 통상의 방법에 따라 건강식품 조성물 제조에 사용할 수 있다.Although the composition ratio of the above-mentioned vitamin and mineral mixture is comparatively mixed with a composition suitable for health food as a preferred embodiment, the compounding ratio may be arbitrarily modified, and the above ingredients are mixed according to a conventional method for producing healthy foods , Granules can be prepared and used in the manufacture of health food compositions according to conventional methods.
제제예 7. 건강 음료의 제조Formulation Example 7. Preparation of health drink
mosloflavone 화합물 -------------------------- 1000 ㎎mosloflavone compound 1000 mg
구연산 --------------------------------------- 1000 ㎎Citric acid --------------------------------------- 1000 mg
올리고당 --------------------------------------- 100 gOligosaccharides --------------------------------------- 100 g
매실농축액 --------------------------------------- 2 gPlum concentrate --------------------------------------- 2 g
타우린 ------------------------------------------- 1 gTaurine ------------------------------------------- 1 g
정제수를 가하여 -------------------------- 전체 900 ㎖Add purified water - 900 ml total
통상의 건강음료 제조방법에 따라 상기의 성분을 혼합한 다음, 약 1시간동안 85℃에서 교반 가열한 후, 만들어진 용액을 여과하여 멸균된 2ℓ 용기에 취득하여 밀봉 멸균한 뒤 냉장 보관한 다음 본 발명의 건강음료 조성물 제조에 사용한다.The above components were mixed according to a conventional health drink manufacturing method, and the mixture was heated at 85 DEG C for about 1 hour with stirring, and the solution thus prepared was filtered to obtain a sterilized 2-liter container, which was sealed and sterilized, ≪ / RTI >
Claims (4)
상기 건강기능식품은 식품류, 분말, 과립, 정제, 캡슐, 시럽제, 음료, 껌, 차, 비타민 복합제, 또는 건강기능성 식품류 형태인 건강기능식품. The method of claim 3, wherein
The health functional food is a health functional food in the form of a food, a powder, a granule, a tablet, a capsule, a syrup, a beverage, a gum, a tea, a vitamin complex, or a health functional food.
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