KR20140142871A - Composition containing gamma-mangosteen for preventing or treating degenerative brain disease - Google Patents
Composition containing gamma-mangosteen for preventing or treating degenerative brain disease Download PDFInfo
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- KR20140142871A KR20140142871A KR20130064545A KR20130064545A KR20140142871A KR 20140142871 A KR20140142871 A KR 20140142871A KR 20130064545 A KR20130064545 A KR 20130064545A KR 20130064545 A KR20130064545 A KR 20130064545A KR 20140142871 A KR20140142871 A KR 20140142871A
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- mangosteen
- dementia
- gamma
- disease
- present
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Abstract
Description
본 발명은 감마 망고스틴을 유효성분으로 함유하는 퇴행성 뇌질환의 예방 또는 치료용 조성물에 관한 것이다.
The present invention relates to a composition for preventing or treating degenerative brain diseases containing gamma-mangosteen as an active ingredient.
퇴행성 뇌질환은 뇌의 기능이 퇴화함에 따라 발생하는 모든 뇌기능 장애 및 질병을 총칭하는 말로, 알쯔하이머병 등의 치매성 질환과 인지장애, 뇌졸중 등을 포함한다.Degenerative brain disease is a generic term for all brain dysfunctions and diseases caused by degeneration of brain function. It includes dementia such as Alzheimer's disease, cognitive disorder, and stroke.
치매는 '정신이 없어진 것'이라는 의미의 라틴어에서 유래된 말로, 정상적으로 생활을 영위하던 사람이 다양한 원인에 의해 기능이 손상되면서 이전에 비해 인지 기능이 지속적이고 전반적으로 저하되어 일상생활에 상당한 지장을 나타내게 되는 상태를 말한다. 치매는 기억력과 더불어 그외 다양한 지적능력이 감퇴되는 것으로, 노인이 되면 자연스럽게 기억력이 감퇴되는 증상과는 구별된다. 이러한 치매는 뇌의 기질적인 병변으로 인해 신경세포 및 조직이 파괴됨으로써, 뇌기능 장애 및 저하가 지속적으로 발생하여 유발되는 것으로 알려져 있다. 외과적 수술후 발생하는 혼돈 상태 등의 의식 장애는 이차적으로 인지기능의 저하를 유발하는데 이를 '섬망'이라 하며, 치매와는 구별되는 증상이다. 과거에는 치매를 망령, 노망이라고 부르면서 노인이 되면 당연히 일어나는 노화 현상이라고 생각했으나, 최근 많은 연구를 통해 뇌질환의 하나로 인식되고 있다. Dementia is a term derived from the Latin word meaning "lost in spirit." This means that a person who has been living normally has been impaired by various causes, and his or her cognitive function is continuously and generally lowered than before. It refers to the state to be represented. Dementia is characterized by memory loss and various other intellectual abilities, which distinguish it from the symptoms of naturally declining memory. It is known that such dementia is caused by continuous development of brain dysfunction and deterioration due to destruction of nerve cells and tissues due to a mild lesion of the brain. Concomitant disorders such as chaos after surgery can cause secondary deterioration of cognitive function, which is called 'delirium' and is a symptom different from dementia. In the past, dementia was called aggression and aging, and it was thought to be an aging phenomenon naturally occurring when an elderly person became an elderly person.
흔히, 치매를 하나의 질병으로 생각하고 모두 똑같으며, 별다른 치료법이 없다고 속단해버리는 경향이 있다. 그러나, 치매는 원인에 따라 세분화할 경우 70여 가지에 달한다. 치매는 크게 노인성 치매와 혈관성 치매로 구분되며, 특히 알쯔하이머병과 혈관성 치매가 가장 많이 발생하는 치매인 것으로 알려져 있다. 치매는 루이체 치매, 전측두엽 치매, 파킨슨병 치매 등을 포함하는 퇴행성 뇌질환으로, 정상압 뇌수두증, 두부 외상, 뇌종양, 대사성 질환, 결핍성 질환, 중독성 질환, 감염성 질환 등 다양한 원인 질환에 의해 유발될 수 있다.Often, they think of dementia as a disease, they all are the same, and they tend to concede that there is no cure. However, dementia is classified into more than 70 cases according to the cause. Dementia is classified into senile dementia and vascular dementia. It is known that Alzheimer's disease and vascular dementia are the most common dementia. Dementia is a degenerative brain disease that includes Lewy body dementia, anterior temporal dementia, dementia of Parkinson's disease, and is caused by various causes such as normal pressure hydrocephalus, head trauma, brain tumor, metabolic disease, .
한편, 우리나라는 출산율 저하 및 고령화 등으로 인해 노령화 사회에 진입하면서 총 인구에 대한 노인 인구의 비중이 점차 커지고 있는 실정이다. 이러한 노인 인구의 증가와 더불어 치매 환자수도 급증하고 있는 것으로 알려져 있다. "노인의 치매 실태와 대책”에 대한 한국보건사회연구소의 연구 결과에 따르면, 국내 치매 환자수는 2010년에 약 47만명, 2012년에 약 52만명으로 통계되었으며, 2030년에 약 114만명으로 예상되고 있다. 또한, 치매 유병율은 2010년에 8.76%로 통계되었으며, 2020년에 9.74%로 증대할 것으로 예상되고 있다. On the other hand, the proportion of the elderly population to the total population is gradually increasing as Korea enters the aging society due to the declining fertility rate and aging population. It is known that the number of dementia patients is increasing rapidly with the increase of the elderly population. According to a study by the Korea Institute of Health and Social Research on "the status and measures of dementia of the elderly," the number of domestic dementia patients was estimated to be about 470,000 in 2010 and about 520,000 in 2012, and about 1.14 million in 2030 In addition, the prevalence of dementia was 8.76% in 2010 and is expected to increase to 9.74% in 2020.
이러한 치매 환자수의 증가는 치매 관련 의료비의 급증을 초래하였다. 치매를 위해 소비되는 연간 의료비 총액은 2002년에 약 470억원으로 통계된 반면, 2007년에는 약 3026억원으로 통계되어 약 6배가 증가되었다. 또한, 노인 장기요양 보험 가입자 중에서 치매 환자가 22.1%의 비율을 차지하는 것으로 확인되어 이에 대한 심각성을 반영하고 있다. 국민건강보험공단에서 제공한 자료에 따르면, 건강보험 실제 진료 환자수가 매년 증가하고 있다고 한다.The increase in the number of patients with dementia led to a surge in medical costs related to dementia. The total annual amount of medical expenses spent for dementia was estimated at about 47 billion won in 2002, while in 2007 it was about 302.6 billion won, which is about 6 times higher. In addition, 22.1% of demented patients among the elderly long term care insurance members were found to account for the seriousness. According to the data provided by the National Health Insurance Corporation, the actual number of health care patients is increasing every year.
미국에서도 2010년 알쯔하이머병의 환자수는 50만명을 상회하였으며, 2050년에는 약 1,350만명에 이를 것으로 예상되고 있다고 한다. 더불어, 미국에서 2010년 알쯔하이머 및 치매로 인해 지출된 의료비는 약 1,720억 달러로 통계되었다고 알려져있다. 치매의 발병을 5년 정도 지연시킬 경우, 약 4,470억 달러의 의료비 절감이 예상된다. In the United States, the number of patients with Alzheimer's disease in 2010 is over 500,000, and it is expected to reach about 13.5 million by 2050. In addition, the cost of medical care for Alzheimer's and dementia in the United States in 2010 is estimated at about $ 172 billion. If delaying the onset of dementia by 5 years, about $ 447 billion in medical costs are expected to be saved.
치매 치료제는 현재 총 4종, 즉 콜린 에스테라아제(choline esterase) 저해제인 도네페질(donepezil), 리바스티그민(rivastigmine), 갈란타민(galantamine), 타크린(tacrine) 및 NMDA 수용체 길항제(receptor antagonist)인 메만틴(memantine)만이 제한적으로 사용되고 있는 실정이며, 이의 치료 효과 또한 광범위하게 사용될 수 없다는 문제점이 있어 새로운 치료제의 개발이 요구되고 있는 실정이다. 미국, 영국, 프랑스, 독일, 일본, 이탈리아 및 스페인 등 7개국에서의 치매 치료제 시장은 2007년 약 30억 달러로 추산되었으며, 2017년에는 90억 달러에 이를 것으로 예상되고 있다.Dementia therapies currently include four types of choline esterase inhibitors: donepezil, rivastigmine, galantamine, tacrine, and NMDA receptor antagonists. Memantine has been used only limitedly, and its therapeutic effect can not be widely used. Therefore, there is a need to develop a new therapeutic agent. The dementia market in seven countries, including the United States, the United Kingdom, France, Germany, Japan, Italy and Spain, was estimated at about $ 3 billion in 2007 and is expected to reach $ 9 billion in 2017.
한편, 베타-세크레타제(β-secretase)는 치매의 주요 원인으로 알려진 아밀로이드 베타(Aβ) 펩타이드의 생성에 관여하는 효소이다. 또한, 아스파틱 세크레타제(aspartic secretase)의 일종인 베타-세크레타제는 최근 노인성 치매를 비롯한 퇴행성 뇌신경 질환의 치료제 개발을 위한 약물 타겟으로 주목받고 있다. On the other hand, β-secretase is an enzyme involved in the production of amyloid beta (Aβ) peptide, which is known to be a major cause of dementia. In addition, beta-secretase, which is a kind of aspartic secretase, is recently attracting attention as a drug target for the development of a therapeutic agent for degenerative brain diseases including senile dementia.
한편, 망고스틴(Garcinia mangostana)은 말레이시아가 원산지인 쌍떡잎식물 무환자나무목 고추나무과의 상록교목으로, 향기가 있고 새콤달콤하여 열매 중의 여왕이라고 불리울 정도로 맛이 뛰어나다. 망고스틴의 과육에 있는 색소는 탄닌을 함유하고 있어 쉽게 색이 변하지 않아 염료로 사용할 수 있다. 망고스틴은 수정을 하지 않고 종자를 만들어 심으므로, 옛날부터 동일한 품종이 재배되었으며, 재배가 까다로워 제한된 지방에서만 자라는 것으로 알려져 있다. 망고스틴은 인도네시아, 말레이시아, 타이완, 필리핀, 인도, 스리랑카 등지에서 분포한다. 망고스틴은 살균, 항균, 항알레르기 작용이 있으며, 베타카로틴을 다량 함유하고 있어 발암물질인 니트로소아민의 생성을 저해하는 것으로 알려져 있다. 또한, 망고스틴은 골다공증 예방, 시력증진, 식욕증진, 소화촉진, 변비예방, 간기능 활성화, 결핵 예방, 심장보호 등의 효과가 있는 것으로 알려져 있다. 망고스틴의 껍질에는 크산톤(Xanthone, 또는 잔톤)이 다량 함유되어 있어, 위와 같은 우수한 약리효과를 나타내는 것으로 보고되어 있다. 크산톤은 대표적으로 알파 망고스틴, 감마 망고스틴 등이 있다.On the other hand, Mangosteen (Garcinia mangostana) is an evergreen arborescent tree of the mulberry tree, which is the origin of Malaysia, and is so sweet that it is fragrant, sour and sweet and is called the queen of the fruit. The pigment in the flesh of mangosteen contains tannin and can be used as a dye because its color does not change easily. Since mangosteen is seedless without fertilization, it is said that the same breed has been cultivated since ancient times and it grows only in a limited region because it is difficult to cultivate. Mangosteen is distributed in Indonesia, Malaysia, Taiwan, Philippines, India and Sri Lanka. Mangosteen is sterilized, has antibacterial and antiallergic action, and contains a large amount of beta carotene, which is known to inhibit the production of nitrosamine, a carcinogen. In addition, mangosteen is known to have effects such as prevention of osteoporosis, improvement of vision, promotion of appetite, promotion of digestion, prevention of constipation, activation of liver function, prevention of tuberculosis, and protection of heart. The skin of mangosteen contains a large amount of xanthone (or xanthone), which is reported to exhibit such excellent pharmacological effects. Xanthones are, for example, alpha mangosteen and gamma mangosteen.
본 발명자들은 치매를 비롯한 퇴행성 뇌질환을 치료하는 효과가 우수한 약물을 개발하기 위하여 천연물 및 이로부터 분리된 화합물에 관하여 연구하던 중, 감마 망고스틴이 신경세포의 산화적 손상을 억제하고, 세포자멸사를 억제하고, 항산화 효과가 우수하며, 흥분성 신경세포 독성을 억제하고, Aβ펩타이드-유발 신경독성을 억제하고, 베타-세크레타제의 활성을 억제함으로써, 부작용이 적으며, 신경을 보호하고 Aβ펩타이드의 생성을 억제하는 효과가 우수함을 확인하고, 본 발명을 완성하게 되었다.
The inventors of the present invention have been studying natural products and compounds separated therefrom in order to develop drugs having excellent effects for treating degenerative brain diseases such as dementia. It has been found that gamma-mangostin inhibits oxidative damage of nerve cells, Suppresses excitatory neuronal cytotoxicity, inhibits Aβ peptide-induced neurotoxicity, inhibits the activity of beta-secretase, has few side effects, protects neurons, inhibits Aβ peptide-induced neurotoxicity It is confirmed that the effect of inhibiting the formation of the compound is excellent, and the present invention has been completed.
본 발명은 감마 망고스틴을 유효성분으로 함유하는 퇴행성 뇌질환의 예방 또는 치료용 약학적 조성물을 제공한다.The present invention provides a pharmaceutical composition for preventing or treating degenerative brain diseases containing gamma-mangosteen as an active ingredient.
본 발명은 감마 망고스틴을 유효성분으로 함유하는 퇴행성 뇌질환의 예방 또는 개선용 식품 조성물을 제공한다.
The present invention provides a food composition for preventing or ameliorating a degenerative brain disease containing gamma-mangosteen as an active ingredient.
본 발명의 목적은 감마 망고스틴을 유효성분으로 함유하는 퇴행성 뇌질환의 예방 또는 치료용 약학적 조성물을 제공하는 것이다.It is an object of the present invention to provide a pharmaceutical composition for preventing or treating degenerative brain diseases containing gamma-mangosteen as an active ingredient.
본 발명의 다른 목적은 감마 망고스틴을 유효성분으로 함유하는 퇴행성 뇌질환의 예방 또는 개선용 식품 조성물을 제공하는 것이다.
Another object of the present invention is to provide a food composition for preventing or ameliorating degenerative brain diseases containing gamma-mangosteen as an active ingredient.
본 발명의 감마 망고스틴은 신경세포의 산화적 손상을 억제하고, 세포자멸사를 억제하고, 항산화 효과가 우수하며, 흥분성 신경세포 독성을 억제하고, Aβ펩타이드-유발 신경독성을 억제하고, 베타-세크레타제의 활성을 억제함으로써, 부작용이 적으며, 신경을 보호하고 Aβ펩타이드의 생성을 억제하는 효과가 우수하므로, 치매를 비롯한 퇴행성 뇌질환의 예방 또는 치료에 유용하게 사용될 수 있다.
The gamma-mangosteen of the present invention inhibits oxidative damage of nerve cells, inhibits apoptosis, has excellent antioxidative effects, inhibits excitatory neuronal cytotoxicity, inhibits A [beta] peptide-induced neurotoxicity, By inhibiting the activity of cryptase, it has few side effects, is excellent in the effect of protecting neurons and inhibiting the production of A [beta] peptide, and thus can be useful for the prevention or treatment of degenerative brain diseases including dementia.
도 1은 본 발명에 따른 감마 망고스틴의 산화적 신경세포 손상 억제활성을 현미경으로 관찰한 결과를 나타낸 도이다.
도 2는 본 발명에 따른 감마 망고스틴의 반응성 산소종 억제활성을 측정한 결과를 나타낸 도이다.
도 3은 본 발명에 따른 감마 망고스틴의 카스파제-3 억제활성을 웨스턴 블럿팅을 통해 측정한 결과를 나타낸 도이다.
도 4는 본 발명에 따른 감마 망고스틴의 DNA 단편화 억제활성을 TUNEL 법을 이용하여 위상차 현미경으로 관찰한 결과를 나타낸 도이다(a. 대조군, b. 100 μM H2O2 를 2시간 동안 처리한 실험군, c. 100 μM H2O2 및 10 μM 감마 망고스틴을 2시간 동안 처리한 실험군, d. 10 μM 감마 망고스틴을 2시간 동안 처리한 실험군/ 실험에서 10 μM 감마 망고스틴은 30분간 전처리됨).
도 5는 본 발명에 따른 감마 망고스틴의 지질과산화 억제활성 및 DPPH 라디칼 소거능을 측정한 결과를 나타낸 도이다.
도 6은 본 발명에 따른 감마 망고스틴의 흥분성 신경세포 독성 억제활성을 측정한 결과를 나타낸 도이다.
도 7은 본 발명에 따른 감마 망고스틴의 Aβ펩타이드-유발 신경세포 독성 억제활성을 측정한 결과를 나타낸 도이다.
도 8은 본 발명에 따른 감마 망고스틴의 베타-세크레타제 억제활성을 측정한 결과를 나타낸 도이다.
도 9는 본 발명에 따른 감마 망고스틴의 세포독성을 평가한 결과를 나타낸 도이다.
FIG. 1 is a graph showing microscopic observation of the inhibitory activity of oxidative neuronal cell damage of gamma-mangosteen according to the present invention.
FIG. 2 is a graph showing the results of measuring the reactive oxygen species inhibitory activity of gamma-mangosteen according to the present invention. FIG.
FIG. 3 is a graph showing the caspase-3 inhibitory activity of gamma-mangosteen according to the present invention measured by Western blotting.
Figure 4 shows the result of observation of the DNA fragmentation inhibitory activity of gamma-mangosteen according to the present invention by a phase contrast microscope using TUNEL method (a. Control group, b. Treated with 100 μM H 2 O 2 for 2 hours Experimental group, c. Experimental group treated with 100 μM H 2 O 2 and 10 μM gamma mangosteen for 2 hours, d. 10 μM gamma mangosteen treated with 10 μM gamma mangosteen for 2 hours, Processed).
FIG. 5 is a graph showing the results of measuring lipid peroxidation inhibitory activity and DPPH radical scavenging activity of gamma-mangosteen according to the present invention.
FIG. 6 is a graph showing the results of measuring the activity of inhibiting excitatory neuron cytotoxicity of gamma-mangosteen according to the present invention.
FIG. 7 is a graph showing the results of measuring the inhibitory activity of Aβ peptide-induced nerve cell cytotoxicity of gamma-mangosteen according to the present invention.
8 is a graph showing the results of measurement of beta-secretase inhibitory activity of gamma-mangosteen according to the present invention.
FIG. 9 is a graph showing the results of evaluation of cytotoxicity of gamma mangosteen according to the present invention. FIG.
본 발명은 하기 화학식 1로 표시되는 감마 망고스틴을 유효성분으로 함유하는 퇴행성 뇌질환의 예방 또는 치료용 조성물을 제공한다.The present invention provides a composition for preventing or treating degenerative brain diseases comprising gamma-mangosteen represented by the following formula (1) as an active ingredient.
상기 조성물을 약학적 조성물 및 식품 조성물을 포함한다.Such compositions include pharmaceutical compositions and food compositions.
이하 본 발명에 관하여 상세히 설명한다.Hereinafter, the present invention will be described in detail.
본 발명의 유효성분인 감마 망고스틴은 통상적인 추출 및 분획 방법에 의해 얻을 수 있고 또는 시판되는 시약을 구입하여 사용할 수도 있다. Gamma mangosteen, which is an active ingredient of the present invention, can be obtained by conventional extraction and fractionation methods, or commercially available reagents can be purchased and used.
본 발명에서는 하기와 같은 방법으로 수득하였다.In the present invention, it was obtained by the following method.
먼저, 음건한 망고스틴 과피를 물, 탄소수 1 내지 4의 알코올 또는 이들의 혼합 용매로 추출한 다음, 이를 여과 및 농축하여 조추출물을 수득한다. 이때, 탄소수 1 내지 4의 알코올은 1 내지 100%(v/v)의 메탄올, 1 내지 100%(v/v)의 에탄올이며, 1 내지 100%(v/v)의 메탄올이 더욱 바람직하다. 수득한 조추출물을 증류수에 현탁하고 헥산(hexane), 클로로포름(chloroform), 에틸아세테이트(ethyl acetate), n-부탄올(n-butanol)로 순차 분획한다. 이들 분획들 중 신경세포 손상 억제 활성이 우수한 클로로포름 분획물을 크로마토그래피하여 노란 분말형태의 감마 망고스틴을 수득한다.First, the shaded mangosteen hull is extracted with water, an alcohol having 1 to 4 carbon atoms or a mixed solvent thereof, followed by filtration and concentration to obtain a crude extract. At this time, the alcohol having 1 to 4 carbon atoms is 1 to 100% (v / v) methanol, 1 to 100% (v / v) ethanol, and more preferably 1 to 100% (v / v) methanol. The obtained crude extract is suspended in distilled water and fractionated with hexane, chloroform, ethyl acetate and n-butanol in order. Among these fractions, the chloroform fraction having excellent activity for inhibiting neuronal damage is chromatographed to obtain gamma mangosteen in the form of a yellow powder.
본 발명의 감마 망고스틴은 신경세포의 산화적 손상을 억제하고, 세포자멸사를 억제하고, 항산화 효과가 우수하며, 흥분성 신경세포 독성을 억제하고, Aβ펩타이드-유발 신경독성을 억제하고, 베타-세크레타제의 활성을 억제함으로써, 부작용이 적으며, 신경을 보호하고 Aβ펩타이드의 생성을 억제하는 효과가 우수하므로, 치매를 비롯한 퇴행성 뇌질환의 예방 또는 치료에 유용하게 사용될 수 있다.The gamma-mangosteen of the present invention inhibits oxidative damage of nerve cells, inhibits apoptosis, has excellent antioxidative effects, inhibits excitatory neuronal cytotoxicity, inhibits A [beta] peptide-induced neurotoxicity, By inhibiting the activity of cryptase, it has few side effects, is excellent in the effect of protecting neurons and inhibiting the production of A [beta] peptide, and thus can be useful for the prevention or treatment of degenerative brain diseases including dementia.
상기 퇴행성 뇌질환은 치매, 경도 인지장애, 뇌졸증, 크로이츠펠트-야콥병, 외상성 두부 손상, 매독, 후천성 면역 결핍증후군, 뇌농양, 뇌종양, 다발성경화증, 저산소증, 파킨슨병, 루게릭병, 헌팅턴병, 픽병, 근위축성 측색 경화증, 간질, 허혈, 중풍, 주의결결핍-과잉행동장애, 정신 분열증, 우울증, 조울증, 외상후스트레스장애, 척수손상 및 척수염을 포함하나, 이에 한정되는 것은 아니다.Wherein said degenerative brain disease is selected from the group consisting of dementia, mild cognitive impairment, stroke, Creutzfeldt-Jakob disease, traumatic head injury, syphilis, acquired immunodeficiency syndrome, brain abscess, brain tumor, multiple sclerosis, hypoxia, Parkinson's disease, But are not limited to, colorimetric sclerosis, epilepsy, ischemia, paralysis, deprivation of behavior - hyperactivity disorder, schizophrenia, depression, manic depression, post traumatic stress disorder, spinal cord injury and myelitis.
상기 치매는 노인성 치매, 알쯔하이머병, 혈관성 치매, 루이소체 치매, 전측두엽 치매, 정상압 뇌수두증에 의한 치매, 두부 외상으로 인한 치매, 대사성 질환에 의한 치매 및 화학 물질에 의해 유발된 치매를 포함하나, 이에 한정되는 것은 아니다.
The dementia includes dementia caused by senile dementia, Alzheimer's disease, vascular dementia, dementia of the frontal lobe, anterior temporal dementia, dementia caused by normal pressure hydrocephalus, head trauma, dementia caused by metabolic disease, But is not limited thereto.
본 발명의 조성물은 감마 망고스틴과 함께 퇴행성 뇌질환에 대하여 예방 또는 치료의 효과를 갖는 공지의 유효성분을 1종 이상 더 함유할 수 있다. The composition of the present invention, together with gamma-mangosteen, may further contain one or more known active ingredients having an effect of preventing or treating degenerative brain diseases.
본 발명의 조성물은 약학적 조성물의 제조에 통상적으로 사용하는 적절한 담체, 부형제 및 희석제를 더 포함할 수 있다. 또한, 통상의 방법에 따라 산제, 과립제, 정제, 캡슐제, 현탁액, 에멀젼, 시럽, 에어로졸 등의 경구형 제형, 외용제, 좌제 및 멸균 주사용액의 형태로 제형화하여 사용될 수 있다. 당해 기술 분야에 알려진 적합한 제제는 문헌 (Remington's Pharmaceutical Science, 최근, Mack Publishing Company, Easton PA)에 개시되어 있는 것을 사용하는 것이 바람직하다. 포함될 수 있는 담체, 부형제 및 희석제로는 락토오스, 덱스트로오스, 수크로오스, 소르비톨, 만니톨, 자일리톨, 에리스리톨, 말티톨, 전분, 아카시아 고무, 알지네이트, 젤라틴, 칼슘 포스페이트, 칼슘 실리케이트, 셀룰로오스, 메틸 셀룰로오스, 미정질 셀룰로오스, 폴리비닐 피롤리돈, 물, 메틸히드록시 벤조에이트, 프로필히드록시 벤조에이트, 탈크, 마그네슘 스테아레이트 및 광물유 등이 있다. 상기 조성물을 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 조성물에 적어도 하나 이상의 부형제 예를 들면, 전분, 칼슘카보네이트 (calcium carbonate), 수크로오스, 락토오스, 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 단순 희석제인 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, 트윈 (tween) 61, 카카오지, 라우린지, 글리세로제라틴 등이 사용될 수 있다. The compositions of the present invention may further comprise suitable carriers, excipients and diluents conventionally used in the manufacture of pharmaceutical compositions. In addition, it can be formulated in the form of powders, granules, tablets, capsules, suspensions, emulsions, oral formulations such as syrups and aerosols, external preparations, suppositories and sterilized injection solutions according to a conventional method. Suitable formulations known in the art are preferably those as disclosed in Remington ' s Pharmaceutical Science, recently, Mack Publishing Company, Easton PA. Examples of carriers, excipients and diluents which may be included include lactose, dextrose, sucrose, sorbitol, mannitol, xylitol, erythritol, maltitol, starch, acacia rubber, alginate, gelatin, calcium phosphate, calcium silicate, cellulose, methylcellulose, Cellulose, polyvinylpyrrolidone, water, methylhydroxybenzoate, propylhydroxybenzoate, talc, magnesium stearate, and mineral oil. When the composition is formulated, it is prepared using a diluent such as a filler, an extender, a binder, a wetting agent, a disintegrant, a surfactant, or an excipient 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 may also be used. Examples of the liquid preparation for oral administration 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. Examples of the suppository base include witepsol, macrogol, tween 61, cacao butter, laurin, glycerogelatin and the like.
본 발명에서 사용되는 용어 "투여"는 임의의 적절한 방법으로 개체에게 소정의 본 발명의 조성물을 제공하는 것을 의미한다.The term "administering" as used herein is meant to provide any desired composition of the invention to a subject in any suitable manner.
본 발명의 약학적 조성물의 바람직한 투여량은 개체의 상태 및 체중, 질병의 정도, 약물형태, 투여경로 및 기간에 따라 다르지만, 당업자에 의해 적절하게 선택될 수 있다. 바람직한 효과를 위해서, 본 발명의 감마 망고스틴은 1일 1 mg/ kg 내지 10000 mg/kg의 양으로 투여할 수 있으며, 하루에 한번 투여할 수도 있고, 수 회 나누어 투여할 수도 있다. The preferred dosage of the pharmaceutical composition of the present invention varies depending on the condition and the weight of the individual, the degree of disease, the type of drug, the route of administration and the period of time, but can be appropriately selected by those skilled in the art. For a desired effect, the gamma-mangosteen of the present invention may be administered in an amount of 1 mg / kg to 10000 mg / kg per day, or may be administered once a day or divided into several doses.
본 발명의 약학적 조성물은 개체에게 다양한 경로로 투여될 수 있다. 투여의 모든 방식은 예상될 수 있는데, 예를 들면, 경구, 직장 또는 정맥, 근육, 피하, 자궁 내 경막 또는 뇌혈관 내 주사에 의해 투여될 수 있다. The pharmaceutical composition of the present invention may be administered to a subject in various routes. All modes of administration may be expected, for example, by oral, rectal or intravenous, intramuscular, subcutaneous, intra-uterine dural or intracerebral injection.
본 발명의 조성물은 퇴행성 뇌질환의 예방 및 치료를 위하여 단독으로, 또는 수술, 방사선 치료, 호르몬 치료, 화학 치료 및 생물학적 반응 조절제를 사용하는 방법들과 병용하여 사용할 수 있다.
The composition of the present invention can be used alone or in combination with methods using surgery, radiation therapy, hormone therapy, chemotherapy, and biological response modifiers for the prevention and treatment of degenerative brain diseases.
본 발명에서, "건강기능식품"이란, 질병의 예방 및 개선, 생체방어, 면역, 병후의 회복, 노화 억제 등 생체조절 기능을 가지는 식품을 말하는 것으로, 장기적으로 복용하였을 때 인체에 무해해야 한다. In the present invention, the term "health functional food" refers to a food having a biological control function such as prevention and improvement of disease, bio-defense, immunity, recovery after disease and aging inhibition.
본 발명의 조성물은 퇴행성 뇌질환의 예방 또는 개선을 목적으로 건강기능식품에 첨가될 수 있다. 본 발명의 감마 망고스틴을 식품 첨가물로 사용할 경우, 상기 감마 망고스틴을 그대로 첨가하거나 다른 식품 또는 식품 성분과 함께 사용될 수 있고, 통상적인 방법에 따라 적절하게 사용될 수 있다. 유효성분의 혼합양은 사용 목적 (예방, 건강 또는 치료적 처치)에 따라 적합하게 결정될 수 있다. 일반적으로, 식품 또는 음료의 제조 시에 본 발명의 감마 망고스틴은 원료에 대하여 15중량% 이하, 바람직하게는 10 중량% 이하의 양으로 첨가된다. 그러나, 건강 및 위생을 목적으로 하거나 또는 건강 조절을 목적으로 하는 장기간의 섭취의 경우에는 상기 범위 이하일 수 있으며, 안전성 면에서 아무런 문제가 없기 때문에 유효성분은 상기 범위 이상의 양으로도 사용될 수 있다.The composition of the present invention can be added to health functional foods for the purpose of preventing or improving degenerative brain diseases. When the gamma-mangosteen of the present invention is used as a food additive, the gamma-mangosteen can be added as it is or can be used together with other food or food ingredients, and can be suitably used according to a conventional method. The amount of the active ingredient to be mixed can be suitably determined according to the intended use (prevention, health or therapeutic treatment). Generally, the gamma-mangosteen of the present invention is added in an amount of not more than 15% by weight, preferably not more than 10% by weight based on the raw material, in the production of food or beverage. However, in the case of long-term intake for the purpose of health and hygiene or for the purpose of controlling health, the amount may be less than the above range, and since there is no problem in terms of safety, the active ingredient may be used in an amount exceeding the above range.
상기 식품의 종류에는 특별한 제한은 없다. 상기 물질을 첨가할 수 있는 식품의 예로는 육류, 소시지, 빵, 초콜릿, 캔디류, 스낵류, 과자류, 피자, 라면, 기타 면류, 껌류, 아이스크림류를 포함한 낙농제품, 각종 수프, 음료수, 차, 드링크제, 알코올 음료 및 비타민 복합제 등이 있으며, 통상적인 의미에서의 건강식품을 모두 포함한다.There is no particular limitation on the kind of the food. Examples of foods to which the above substances can be added include dairy products including meat, sausage, bread, chocolate, candy, snacks, confectionery, pizza, ramen and other noodles, gums, ice cream, various soups, drinks, tea, Alcoholic beverages, and vitamin complexes, all of which include health foods in a conventional sense.
본 발명의 건강음료 조성물은 통상의 음료와 같이 여러 가지 향미제 또는 천연 탄수화물 등을 추가 성분으로서 포함할 수 있다. 상술한 천연 탄수화물은 포도당, 과당과 같은 모노사카라이드, 말토오스, 수크로오스와 같은 디사카라이드, 및 덱스트린, 사이클로덱스트린과 같은 천연 감미제나, 사카린, 아스파르탐과 같은 합성 감미제 등을 사용할 수 있다. 상기 천연 탄수화물의 비율은 본 발명의 조성물 100 ml 당 일반적으로 약 0.01 내지 10 g, 바람직하게는 약 0.01 내지 0.1 g 이다.The health beverage composition of the present invention may contain various flavors or natural carbohydrates as an additional ingredient such as ordinary beverages. The natural carbohydrates may be monosaccharides such as glucose and fructose, disaccharides such as maltose and sucrose, natural sweeteners such as dextrin and cyclodextrin, synthetic sweeteners such as saccharine and aspartame, and the like. The ratio of the natural carbohydrate is generally about 0.01 to 10 g, preferably about 0.01 to 0.1 g per 100 ml of the composition of the present invention.
상기 외에 본 발명의 조성물은 여러 가지 영양제, 비타민, 전해질, 풍미제, 착색제, 펙트산 및 그의 염, 알긴산 및 그의 염, 유기산, 보호성 콜로이드 증점제, pH 조절제, 안정화제, 방부제, 글리세린, 알코올, 탄산 음료에 사용되는 탄산화제 등을 포함할 수 있다. 그 밖에 본 발명의 조성물은 천연 과일주스, 과일주스 음료 및 야채 음료의 제조를 위한 과육을 포함할 수 있다. 이러한 성분은 독립적으로 또는 조합하여 사용할 수 있다. 이러한 첨가제의 비율은 크게 중요하진 않지만 본 발명의 조성물 100 중량부 당 0.01 내지 0.1 중량부의 범위에서 선택되는 것이 일반적이다.
In addition to the above, the composition of the present invention may further contain various nutrients, vitamins, electrolytes, flavors, colorants, pectic acid and salts thereof, alginic acid and salts thereof, organic acids, protective colloid thickeners, pH adjusters, stabilizers, preservatives, glycerin, A carbonating agent used in a carbonated beverage, and the like. In addition, the composition of the present invention may comprise flesh for the production of natural fruit juices, fruit juice drinks and vegetable drinks. These components may be used independently or in combination. Although the ratio of such additives is not critical, it is generally selected in the range of 0.01 to 0.1 parts by weight per 100 parts by weight of the composition of the present invention.
이하 본 발명의 이해를 돕기 위하여 바람직한 실시예, 실험예 및 제제예를 제시한다. 그러나 하기 실시예, 실험예 및 제제예는 본 발명을 보다 쉽게 이해하기 위하여 제공되는 것일 뿐, 실시예, 실험예 및 제제예에 의해 본 발명의 내용이 한정되는 것은 아니다.
Hereinafter, preferred examples, experimental examples, and formulation examples are provided to facilitate understanding of the present invention. However, the following examples, experimental examples and preparation examples are provided only for the purpose of easier understanding of the present invention, and the present invention is not limited by the examples, experimental examples and preparation examples.
[실시예 1. 감마 망고스틴의 제조][Example 1: Preparation of gamma mangosteen]
음건한 망고스틴 과피(1.3 kg)를 100% 메탄올(v/v %)로 8 L씩 3회 초음파 추출한 다음, 이를 여과 및 감압농축하여 메탄올 추출물 401 g을 수득하였다. 상기 수득된 메탄올 추출물 중에서 164 g의 메탄올 추출물을 증류수에 현탁시킨 후, 헥산(hexane), 클로로포름(chloroform), 에틸아세테이트(ethyl acetate), n-부탄올(n-butanol)로 순차 분획을 실시한 후, 각 용매 분획물을 얻었으며, 이들 분획물 중 클로로포름 분획물(37.9 g)에서 산화적 신경세포 손상 억제 활성이 가장 우수함을 확인하였다. 따라서, 클로로포름 분획물에 대하여 헥산 및 에틸아세테이트를 혼합용매로하는 농도기울기 실리카 겔(gradient silica gel) (593 g) 개방형 칼럼 크로마토그래피(open column chromatography)를 진행하여 총 49개의 분획물(GMC1 내지 GMC 49)을 수득하였으며, 그중 35번 분획물(3.36 g)을 선별하여 클로로포름과 아세톤 혼합용매로 농도기울기 실리카 겔(gradient silica gel) (120 g) MPLC를 실시하여 총 23개의 분획물을 수득하였다. 그중 8번 분획물(GMC35-8, 698 mg)을 메탄올과 증류수로 재결정시킴으로써, 노란색 분말인 감마 망고스틴을 수득하였다. 수득된 감마 망고스틴의 화학구조 분석은 질량분석기 및 핵자기공명분광기를 이용하여 동정하였다.
The shaded mangosteen skin (1.3 kg) was ultrasonically extracted three times with 8 L of 100% methanol (v / v%), and then filtered and concentrated under reduced pressure to obtain 401 g of methanol extract. 164 g of the methanol extract in the obtained methanol extract was suspended in distilled water and sequentially fractionated with hexane, chloroform, ethyl acetate and n-butanol, Each solvent fraction was obtained. Among these fractions, the chloroform fraction (37.9 g) showed the highest inhibitory activity against oxidative neuronal damage. Thus, the chloroform fractions were subjected to open column chromatography using gradient silica gel (593 g) using hexane and ethyl acetate as a mixed solvent to obtain a total of 49 fractions (GMC1 to GMC 49) Among them, the fraction No. 35 (3.36 g) was selected and MPLC of gradient silica gel (120 g) was performed with a mixed solvent of chloroform and acetone to obtain a total of 23 fractions. Among them, fraction 8 (GMC35-8, 698 mg) was recrystallized from methanol and distilled water to obtain a yellow powder, gamma mangosteen. The chemical structure analysis of the obtained gamma mangosteen was carried out using a mass spectrometer and a nuclear magnetic resonance spectrometer.
[실험예 1. 감마 망고스틴의 산화적 신경세포 손상 억제활성 측정][Experimental Example 1: Measurement of oxidative neuronal damage inhibitory activity of gamma-mangosteen]
1. 세포의 준비 및 배양1. Cell preparation and culture
임신 17일째의 SD(Sprague-Dawley) 흰쥐(rat)의 태자에서 얻은 대뇌피질 신경세포의 배양은 하기와 같은 방법으로 수행하였다.Cultures of cerebral cortical neurons obtained from fetuses of SD (Sprague-Dawley) rats on the 17th day of pregnancy were cultured as follows.
구체적으로, 상기 흰쥐의 뇌를 적출하여 뇌막을 제거하고 피질 부분만을 분리하여 잘게 자른 후, 순차적으로 구멍의 크기를 작게 한 3개의 파스퇴르 피펫을 사용하여 단일세포로 분리하였다. 폴리-L-라이신(poly-L-lysine)과 라미닌(laminin)으로 미리 코팅해 놓은 24-웰플레이트(well plate) 또는 35 mm 배양디시(dish)에 6×105세포/웰 또는 6×106세포/배양디시 의 밀도로 각각 상기 흰쥐의 신경세포를 이식하였다. 상기 신경세포를 5% FBS(fetal bovine serum), 5% HS(horse serum), 2 mM 글루타민 및 25 mM 포도당을 포함하는 MEM(minimum essential media, Earle's salts 함유)에 넣고 95% 공기, 5% CO2의 농도로 환경조건을 유지하는 37℃의 배양기에서 배양하였다. 배양 7일 경과후, 10 μM 시토신 아라비노사이드(cytosine arabinoside)로 처리하여 신경세포 이외의 세포에 대한 성장을 억제시킨 다음, 배양 10일 이상 경과 후 실험에 사용하였다.
Specifically, the brain of the rat was removed to remove the brain membrane, and the cortical portion was separated and cut into small pieces. Then, the cells were separated into single cells using three Pasteur pipettes each having a small hole size. Poly -L- lysine to 6 × 10 5 cells / well or 6 × 10 (poly-L- lysine) and laminin (well plate) 24- well plates coated with a preloaded (laminin) or 35 mm culture dish (dish) 6 cells / culture Dissociated densities of the rat neurons were transplanted, respectively. The neurons were placed in MEM (minimum essential medium, containing Earle's salts) containing 5% FBS (fetal bovine serum), 5% HS (horse serum), 2 mM glutamine and 25 mM glucose, 2 < / RTI > in a 37 < 0 > C incubator maintained at ambient conditions. After 7 days of incubation, the cells were treated with 10 [mu] M cytosine arabinoside to inhibit growth of cells other than neurons, and then used for experiments after 10 days or more of incubation.
2. 신경세포의 산화적 세포 손상 유발2. Oxidative Cell Damage Induced by Neuronal Cells
상기 1에서 배양된 신경세포의 산화적 세포 손상을 유발하기 위하여, 하기와 같은 실험을 수행하였다. In order to induce oxidative cell damage of the neuron cultured in the above 1, the following experiment was conducted.
구체적으로, 일차 배양한 흰쥐(rat)의 대뇌피질 신경세포를 HEPES 대조식염수(HCSS; 120 mM NaCl, 5.4 mM KCl, 1.6 mM MgCl2, 2.3 mM CaCl2, 14.9 mM 포도당, 16.8mM HEPES, 10 mM NaOH)로 세척한 후 100 μM H2O2 또는 0.5 mM/10 mU/ml X(xanthine)/XO(xanthine oxidase)를 함유한 HCSS로 각각 5분 또는 10분 동안 처리하였다. 이후, 25 mM 포도당을 함유하는 MEM 배지로 배양액을 교환하여 18-20시간 동안 95% 공기, 5% CO2의 농도로 환경조건을 유지하면서 37℃의 배양기에서 배양하여 신경세포의 산화적 세포 손상을 유발하였다.
Specifically, the cerebral cortical neurons of the primary cultured rat were suspended in HEPES-normal saline (HCSS; 120 mM NaCl, 5.4 mM KCl, 1.6 mM MgCl 2 , 2.3 mM CaCl 2 , 14.9 mM glucose, 16.8 mM HEPES, NaOH) and treated with HCSS containing 100 μM H 2 O 2 or 0.5 mM / 10 mU / ml xanthine / XO (xanthine oxidase) for 5 min or 10 min, respectively. Then, the culture medium was exchanged with MEM medium containing 25 mM glucose and cultured for 18-20 hours in an incubator at 37 ° C while maintaining the environmental conditions at 95% air and 5% CO 2 concentration, Lt; / RTI >
3. 감마 망고스틴의 산화적 신경세포 손상 억제활성 측정3. Measurement of oxidative neuronal damage inhibitory activity of gamma-mangosteen
본 발명의 감마 망고스틴에 대한 신경세포의 손상에 대한 억제활성을 측정하기 위해, 종래에 공지된 방법에 따라 MTT(3-(4,5-Dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide, a yellow tetrazole)법을 수행하여 일차배양된 흰쥐 대뇌피질 신경세포의 세포 생존율을 측정하였다.In order to measure the inhibitory activity of the gamma-mangosteen of the present invention on damage to neurons, MTT (3- (4,5-Dimethylthiazol-2-yl) -2,5-diphenyltetrazolium bromide , a yellow tetrazole method) was performed to measure cell viability of primary cultured rat cerebral cortical neurons.
구체적으로, 각 웰에 MTT 시약(2 mg/ml 농도) 250 ㎕를 분주하고, 37℃의 배양기에서 3시간 동안 배양한 후, 배양물의 상등액을 제거하고, 생존한 세포에서 생성된 포르마잔(formazan) 결정을 500 ㎕의 DMSO로 용해시켰다. 각 웰에서 수득한 시료들을 마이크로플레이트 리더(microplate reader) (SpectraMax M2 microplate reader; Molecular Devices, USA)를 이용하여 550 nm에서 흡광도를 측정하였으며, 위상차 현미경으로 신경세포의 형태학적 변화를 관찰하여 세포의 손상 정도를 확인하였다. 이의 결과를 도 1에 나타내었다. Specifically, 250 占 퐇 of MTT reagent (2 mg / ml concentration) was added to each well and cultured in a 37 占 폚 incubator for 3 hours. Then, the supernatant of the culture was removed, and formazan ) Crystals were dissolved in 500 [mu] l of DMSO. Absorbance was measured at 550 nm using a microplate reader (SpectraMax M2 microplate reader; Molecular Devices, USA). The morphological changes of the neurons were observed using a phase contrast microscope, The degree of damage was confirmed. The results are shown in Fig.
도 1에 나타난 바와 같이, 본 발명의 감마 망고스틴은 10 μM의 농도에서 H2O2와 X/XO에 의해 산화적 세포 손상이 유발된 흰쥐 대뇌피질 신경세포의 세포 생존율을 유의하게 증가시킴을 확인하였으며, 특히, H2O2 에 의해 산화적 세포 손상이 유발된 흰쥐 대뇌피질 신경세포의 세포 생존율을 107.9%로 유의하게 증가시킴을 확인하였다.As shown in FIG. 1, the gamma-mangosteen of the present invention significantly increased the cell survival rate of rat cerebral cortical neurons induced by oxidative cell damage by H 2 O 2 and X / XO at a concentration of 10 μM In particular, it was confirmed that the cell viability of rat cerebral cortical neurons induced by oxidative cell damage by H 2 O 2 was significantly increased to 107.9%.
따라서, 본 발명의 감마 망고스틴은 일차배양된 흰쥐 대뇌피질 신경세포에서 산화적 스트레스에 의해 유발되는 산화적 세포 손상을 농도의존적으로 유의하게 억제하므로, 신경세포의 산화적 손상 억제 및 신경보호 효과가 우수함을 확인하였다.
Therefore, the gamma-mangosteen of the present invention significantly inhibits oxidative cell damage induced by oxidative stress in primary cultured rat cerebral cortical neurons in a concentration-dependent manner, and thus inhibits oxidative damage and neuroprotective effect of neurons .
4. 감마 망고스틴의 반응성 산소종 억제활성 측정4. Measurement of reactive oxygen species inhibitory activity of gamma-mangosteen
본 발명의 감마 망고스틴에 대한 반응성 산소종(reactive oxygen species; ROS) 억제활성을 측정하기 위해, 상기 2에서 배양된 신경세포에서 H2O2, X/XO로 유발되는 반응성 산소종 억제활성을 DCF-DA를 사용하여 하기와 같이 측정하였다.The reactive oxygen species (ROS) for the gamma-mangosteen of the present invention In order to measure the inhibitory activity, the reactive oxygen species inhibitory activity induced by H 2 O 2 , X / XO in nerve cells cultured in the above 2 was measured using DCF-DA as follows.
구체적으로, 상기 배양된 세포를 HCSS로 세척하고 10 μM DCF-DA를 함유하는 MEM 배지로 30분 동안 배양한 후, 200 μM H2O2, 0.5 mM/10 mU/ml X/XO로 2시간 동안 처리하거나 적정 농도의 감마 망고스틴을 동시에 처리하였으며, 일정시간 경과 후 마이크로플레이트 리더(SpectraMax M2e microplate reader)를 이용하여 여기 490 nm, 방출 520 nm에서 형광을 측정하였으며, IC50값을 측정하였다. 감마 망고스틴의 반응성 산소종 억제활성은 도 2에 나타내었으며, 이의 IC50값은 하기 표 1에 나타내었다.Specifically, the cultured cells were washed with HCSS, cultured in MEM medium containing 10 μM DCF-DA for 30 minutes, and then cultured in 200 μM H 2 O 2 , 0.5 mM / 10 mU / ml X / XO for 2 hours And the appropriate concentration of gamma-mangosteen was treated at the same time. After a certain period of time, the fluorescence was measured at 490 nm and 520 nm using a microplate reader (SpectraMax M2 e microplate reader) and the IC 50 value was measured . The reactive oxygen species inhibitory activity of gamma-mangosteen is shown in FIG. 2, and the IC 50 values thereof are shown in Table 1 below.
상기 표 1에 기재된 바와 같이, 본 발명의 감마 망고스틴의 IC50값은 H2O2에서 X/XO보다 낮게 측정되어, 상기 감마 망고스틴이 H2O2에 의해 생성되는 ROS를 더 강력하게 억제하였음을 확인하였다. As shown in Table 1 above, the IC 50 values of the gamma mangosteen of the present invention were measured to be lower than X / XO in H 2 O 2 , indicating that the gamma mangosteen had a stronger ROS produced by H 2 O 2 Respectively.
도 2에 나타난 바와 같이, 본 발명의 감마 망고스틴은 H2O2와 X/XO에 의해 유발된 흰쥐 대뇌피질 신경세포의 ROS을 각각 농도 의존적으로 억제하였음을 확인하였다.As shown in FIG. 2, gamma-mangosteen of the present invention inhibited the ROS of the rat cerebral cortical neurons induced by H 2 O 2 and X / XO, respectively, in a concentration-dependent manner.
따라서, 본 발명의 감마 망고스틴은 일차배양된 흰쥐 대뇌피질 신경세포에서 산화적 스트레스에 의해 생성되는 ROS를 농도의존적으로 유의하게 억제하므로, 신경세포의 산화적 손상 억제 및 신경보호 효과가 우수함을 확인하였다.
Therefore, the gamma-mangosteen of the present invention significantly inhibits ROS produced by oxidative stress in primary cultured rat cerebral cortical neurons in a concentration-dependent manner, Respectively.
[실험예 2. 감마 망고스틴의 세포자멸사 억제활성 측정][Experimental Example 2: Measurement of inhibitory activity of gamma mangosteen on apoptosis]
1. 감마 망고스틴의 카스파제-3 억제활성 측정1. Measurement of caspase-3 inhibitory activity of gamma mangosteen
본 발명의 감마 망고스틴에 대한 세포자멸사(apoptosis) 억제활성을 알아보기 위하여, 종래에 공지된 방법에 따라 웨스턴 블롯팅(western blotting)법을 수행하였다. 상기 실험예 2의 2에서 준비된 일차배양된 흰쥐 대뇌피질 신경세포에 H2O2을 2시간 동안 처리하여 프로카스파제-3(procaspase 3)로부터 생성되는 활성형 카스파제-3을 측정하였다.In order to examine the apoptosis inhibitory activity of gamma-mangosteen of the present invention, western blotting was performed according to a conventionally known method. The primary cultured rat cerebral cortical neurons prepared in 2 of Experimental Example 2 were treated with H 2 O 2 for 2 hours to measure active caspase-3 produced from procaspase-3.
구체적으로, 상기 실험예 2의 2에서 배양된 대뇌피질 신경세포를 100 mM H2O2 또는 100 mM H2O2와 적정 농도의 감마 망고스틴을 포함하는 반응액으로 일정 시간 동안 처리하였다. 이후, PBS (pH 7.3)로 세척한 후 용해 완충액(lysis buffer) (10 mM Tris-HCl (pH 7.5), 150 mM NaCl, 2 mM EDTA, 4.5 mM 피로인산나트륨(sodium pyrophosphate), 10 mM β-글리세롤인산칼슘(β-glycerophosphate), 1 mM NaF, 1 mM Na3VO4, 1% Triton X-100, 0.5% Nonidet P-40 및 프로티아제 억제제 칵테일(protease inhibitor cocktail) (Boehringer, Indianapolis, USA))로 4℃의 온도에서 30분 동안 용해시켜 14,000 rpm에서 30분 동안 원심분리하였다. 이후 상층액을 취하여 바이오레드 Dc 단백질 에쎄이 키트(BioRad Dc protein assay kit) (BioRad, Hercules, USA)로 단백질 농도를 평가하였다. 동일한 양(30 ㎍)의 단백질을 12% SDS-폴리아크릴아미드겔(polyacrylamide gel)을 이용하여 전기영동으로 분리하고, 니트로셀룰로오즈막(nitrocellulose membrane) (Whatman, Boston, USA)으로 이동시킨 후 5% 무-지방 건조 우유(non-fat dry milk)로 1.5시간 동안 실온에서 반응시켜 비특이적 반응을 차단하였다. 이후 1차 항체(카스파제-3 (8G10) 토끼 항체(rabbit antiboby))로 4℃에서 24시간 동안 반응시킨 후 TBS(tris-buffered saline with Tween)로 세척한 다음 2차 항체(anti-rabbit secondary IgG-HRP)와 반응시켜 ECL 디텍션 시스템(detection system) (Thermo Scientific, Rockford, USA)을 사용하여 Chemi-DocTM MP 이미지 시스템(imaging System) (BioRad, Hercules, CA)을 이용하여 분석하였다. 대조군은 감마 망고스틴 대신 DMSO 용매만을 넣은 것을 설정하였으며, 양성대조군으로는 감마 망고스틴 대신 알파 망고스틴을 동일한 농도구배로 처리하여 설정하였다. 이의 결과를 도 3에 나타내었다.Specifically, the cerebral cortical neurons cultured in Experimental Example 2 were treated with a reaction solution containing 100 mM H 2 O 2 or 100 mM H 2 O 2 and an appropriate concentration of gamma-mangosteen for a predetermined period of time. The cells were washed with PBS (pH 7.3), and then lysed in a lysis buffer (10 mM Tris-HCl (pH 7.5), 150 mM NaCl, 2 mM EDTA, 4.5 mM sodium pyrophosphate, Glycerophosphate, 1 mM NaF, 1 mM Na 3 VO 4 , 1% Triton X-100, 0.5% Nonidet P-40 and protease inhibitor cocktail (Boehringer, Indianapolis, USA )) At a temperature of 4 째 C for 30 minutes and centrifuged at 14,000 rpm for 30 minutes. The supernatant was then taken and the protein concentration was assessed with BioRad Dc protein assay kit (BioRad, Hercules, USA). The same amount (30 μg) of the protein was separated by electrophoresis using a 12% SDS-polyacrylamide gel, transferred to a nitrocellulose membrane (Whatman, Boston, USA) Non-fat dry milk for 1.5 hours at room temperature to block nonspecific reactions. After incubation at 4 ° C for 24 hours with a primary antibody (rabbit antiboby), the cells were washed with TBS (tris-buffered saline with Tween) and incubated with anti-rabbit secondary antibody It is reacted with an IgG-HRP) were analyzed using the ECL detection system (detection system) (Thermo Scientific, using Rockford, USA) Chemi-Doc TM MP imaging system (imaging system) (BioRad, Hercules , CA). The control group was set to contain only DMSO solvent instead of gamma-mangosteen, and alpha-mangosteen was set to the same concentration gradient instead of gamma-mangosteen as a positive control group. The results are shown in Fig.
도 3에 나타난 바와 같이, 본 발명의 감마 망고스틴은 대조군에 비하여 활성형인 카스파제-3(cleaved caspase 3)의 생성을 유의하게 억제시킴을 확인하였다. 한편, 양성대조군인 알파 망고스틴은 카스파제-3을 유의하게 억제시켰으나, 감마 망고스틴보다는 낮은 억제활성을 가지는 것으로 확인되었다.As shown in FIG. 3, gamma-mangosteen of the present invention significantly inhibited the production of active form of caspase-3 (cleaved caspase 3) as compared with the control group. On the other hand, the positive control group, alpha mangosteen significantly inhibited caspase-3, but was found to have lower inhibitory activity than gamma mangosteen.
따라서, 본 발명의 감마 망고스틴은 세포자멸사에 관여하는 카스파제-3의 활성을 농도의존적으로 유의하게 억제하고, 다른 크산톤인 알파 망고스틴보다 더 우수한 억제 효과를 가지므로, 신경세포의 손상을 억제하는 효과가 우수함을 확인하였다.
Therefore, the gamma-mangosteen of the present invention significantly inhibits the activity of caspase-3 involved in apoptosis in a concentration-dependent manner and has a more excellent inhibitory effect than the other xanthone, alpha mangosteen, Inhibitory effect was excellent.
2. 감마 망고스틴의 DNA 단편화 억제활성 측정2. Measurement of DNA fragmentation inhibitory activity of gamma-mangosteen
본 발명의 감마 망고스틴에 대한 세포자멸사(apoptosis) 억제활성을 알아보기 위하여, 상기 실험예 2의 2에서 준비된 일차배양된 흰쥐 대뇌피질 신경세포를 H2O2로 2시간 동안 처리한 후, 종래에 공지된 방법에 따라 TUNEL 법으로 염색하여 DNA 단편화(fragmentation)를 확인하였다. In order to examine the apoptosis inhibitory activity of gamma-mangosteen of the present invention, the primary cultured rat cerebral cortical neurons prepared in Experimental Example 2 were treated with H 2 O 2 for 2 hours, And DNA fragmentation was confirmed by staining with the TUNEL method.
구체적으로, TUNEL법에 의한 세포자멸사의 측정은 DeadendTM Colorimetric TUNEL assay kit를 사용하여 제조회사에서 제시한 방법을 약간 변형하여 측정하였다. 분리한 대뇌피질 세포를 96-웰 플레이트에 각 웰당 1×105개의 밀도로 이식하여 37℃의 배양기에서 95% 공기, 5% CO2의 환경조건을 유지하면서 14-15일간 배양하였다. 상기 배양된 세포를 100 mM H2O2 또는 100 mM H2O2와 10 mM 감마 망고스틴을 함유하는 용액으로 2시간 동안 처리한 다음, 4% 파라포름알데하이드(paraformaldehyde) (methanol free)로 상온에서 25분 동안 처리하여 고정시켰다. 이후, 인산완충용액(phosphate-buffered saline) (PBS)으로 5분씩 2회 세척하고, 0.2% 트리톤(Triton) X-100로 5분간 처리한 다음 PBS로 2회 세척하였다. 평형 완충용액(Equilibration buffer)으로 10분간 처리하고 PBS로 세척한 다음 TdT reaction mix로 상온에서 60분 동안 처리하였다. 이후, PBS로 세척한 후 15분간 2X SSC(saline-sodium citrate)로 처리하고 다시 PBS로 세척하고 나서 0.3% H2O2로 5분 동안 처리하였다. PBS로 세척한 후 상온에서 30분간 겨자무과산화효소-표지된 스트렙타비딘(horseradish peroxidase-labeled streptavidin)으로 처리하고, PBS로 다시 세척한 후 10분 동안 디아미노벤지딘(diaminobenzidine)으로 처리한 다음 증류수로 3회 세척한 후 Nikon eclipse TS100 위상차 현미경으로 확인하였다. 이의 결과를 도 4에 나타내었다.Specifically, the measurement of apoptosis by the TUNEL method was performed using the Deadend TM Colorimetric TUNEL assay kit and the method proposed by the manufacturer was slightly modified. Separated cerebral cortical cells were transplanted into a 96-well plate at a density of 1 × 10 5 cells / well and cultured at 37 ° C. for 14-15 days in an incubator maintained at 95% air and 5% CO 2 . The cultured cells were treated with a solution containing 100 mM H 2 O 2 or 100 mM H 2 O 2 and 10 mM gamma-mangosteen for 2 hours, and then treated with 4% paraformaldehyde (methanol free) For 25 minutes. Then, the cells were washed twice with phosphate-buffered saline (PBS) for 5 minutes, treated with 0.2% Triton X-100 for 5 minutes, and then washed twice with PBS. The cells were treated with equilibration buffer for 10 minutes, washed with PBS, and then treated with TdT reaction mix at room temperature for 60 minutes. After washing with PBS, the cells were treated with 2X SSC (saline-sodium citrate) for 15 minutes, washed with PBS, and then treated with 0.3% H 2 O 2 for 5 minutes. After washing with PBS, the cells were treated with horseradish peroxidase-labeled streptavidin for 30 minutes at room temperature, washed again with PBS, treated with diaminobenzidine for 10 minutes, ≪ / RTI > three times and then confirmed by a Nikon eclipse TS100 phase contrast microscope. The results are shown in Fig.
도 4에 나타난 바와 같이, 산화적 세포 손상 유발인자인 H2O2와 본 발명의 감마 망고스틴 10μM을 동시에 처리한 실험군은 대조군과 거의 동일하게 염색된 세포수가 감소되었음을 확인하였다.As shown in FIG. 4, it was confirmed that the number of cells stained in the experimental group treated with H 2 O 2 , which is an oxidative cell damage inducer, and 10 μM of gamma-mangostin of the present invention, was almost the same as that of the control group.
따라서, 본 발명의 감마 망고스틴은 세포자멸사에 관여하는 DNA 단편화를 유의하게 억제하므로, 신경세포의 손상을 억제하는 효과가 우수함을 확인하였다.
Accordingly, it was confirmed that the gamma-mangosteen of the present invention significantly inhibited DNA fragmentation involved in apoptosis, and thus, it was confirmed that the effect of inhibiting damage to nerve cells was excellent.
[실험예 3. 감마 망고스틴의 항산화 활성 측정] [Experimental Example 3: Antioxidant activity measurement of gamma mangosteen]
본 발명의 감마 망고스틴에 대한 항산화 활성을 측정하기 위하여, 상기 실시예 1에서 제조된 감마 망고스틴의 지질과산화 억제활성 및 DPPH(1,1-diphenyl-2-picrylhydrazyl) 라디칼 소거능을 측정하였으며, 이를 위해 웅성 SD 흰쥐로부터 뇌균질액을 얻어 사용하였다.In order to measure the antioxidative activity of gamma-mangosteen of the present invention, the lipid peroxidation inhibitory activity and DPPH (1,1-diphenyl-2-picrylhydrazyl) radical scavenging activity of gamma mangosteen prepared in Example 1 were measured, Brain homogenate was obtained from Weinung SD rats.
감마 망고스틴의 지질과산화 억제활성의 측정은 하기와 같이 수행되었다. Measurement of lipid peroxidation inhibitory activity of gamma mangosteen was performed as follows.
먼저, 일정양의 뇌 균질액; 10 μM Fe2+; 100 μM 아스코르브산(ascorbic acid); 및 적정 농도의 감마 망고스틴;을 포함하는 반응액을 37℃에서 1시간 동안 반응시킨 다음, 트리클로로아세트산과 TBA를 순차적으로 가하여 혼합하였다. 이후 100 ℃의 온도에서 15분 동안 가열하고 원심분리한 다음, 상등액을 분리하여 마이크로플레이트리더(SpectraMax M2e microplate reader)를 이용하여 532 nm에서 흡광도를 측정하였다. 실험군과 대조군에 대한 지질과산화 억제율은 하기 수학식 1을 이용하여 산출하였다.First, a certain amount of brain homogenate; 10 μM Fe 2+ ; 100 [mu] M ascorbic acid; And gamma-mangosteen at an appropriate concentration were reacted at 37 DEG C for 1 hour, and then trichloroacetic acid and TBA were added sequentially and mixed. After heating at 100 ° C for 15 minutes and centrifugation, the supernatant was separated and the absorbance was measured at 532 nm using a microplate reader (SpectraMax M2 e microplate reader). The percent inhibition of lipid peroxidation in the experimental group and the control group was calculated using the following equation (1).
대조군은 시료를 용해시킨 용매만을 처리하여 설정하였으며, 모든 실험은 1회 2군씩 3회 이상 반복하여 얻은 결과 값으로부터 산출된 평균값±S.E.M.으로 나타내었다.
The control group was set up by treating only the solvent in which the sample was dissolved. All experiments were expressed as the average value ± SEM calculated from the results obtained by repeating at least 3 times in 2 groups at once.
감마 망고스틴의 DPPH 라디칼 소거능 측정은 하기와 같이 수행되었다. The DPPH radical scavenging activity of gamma mangosteen was measured as follows.
먼저, 메탄올에 용해시킨 150 μM 의 DPPH와 적정 농도의 감마 망고스틴을 함유하는 반응액을 37℃에서 30분 동안 반응시킨 다음, 마이크로플레이트 리더(SpectraMax M2e microplate)를 이용하여 520 nm에서 흡광도를 측정하였다. 실험군과 대조군에 대한 DPPH 라디칼 소거능은 상기 수학식 1을 이용하여 산출하였다. 이의 결과를 도 5에 나타내었다.First, the reaction solution containing 150 μM of DPPH dissolved in methanol and the appropriate concentration of gamma-mangosteen was reacted at 37 ° C. for 30 minutes, and the absorbance at 520 nm was measured using a Microplate reader (SpectraMax M2 e microplate) Respectively. The DPPH radical scavenging ability of the experimental group and the control group was calculated using the above equation (1). The results are shown in Fig.
이의 결과를 도 5에 나타내었다.The results are shown in Fig.
도 5에 나타난 바와 같이, 본 발명의 감마 망고스틴은 10 μM의 농도 이상에서부터 80%의 높은 지질과산화 억제활성이 측정되었으며, 이때, IC50 값은 5.8 μM 로 확인되었다. 한편, 본 발명의 감마 망고스틴은 10 μM에서 17.2%, 30 μM에서 51%의 DPPH 라디칼 소거능이 측정되었으며, 이때, IC50 값은 29.3 μM로 확인되었다.As shown in FIG. 5, in the gamma-mangosteen of the present invention, a high lipid peroxidation inhibitory activity of 80% was measured from a concentration of 10 μM or more, wherein the IC 50 value was 5.8 μM. Meanwhile, the gamma-mangosteen of the present invention had a DPPH radical scavenging activity of 17.2% at 10 μM and 51% at 30 μM, and the IC 50 value was 29.3 μM.
따라서, 본 발명의 감마 망고스틴은 강력한 지질과산화 억제활성을 가지며 작지만 유의한 DPPH 라디칼 소거능을 가지므로, 항산화 작용이 우수하여 신경세포의 손상 억제 및 신경보호 효과가 우수함을 확인하였다.
Therefore, the gamma-mangosteen of the present invention has a strong lipid peroxidation inhibitory activity and a small but significant DPPH radical scavenging ability, and thus it is confirmed that the antioxidant activity is excellent and the nerve cell damage inhibition and neuroprotective effect are excellent.
[실험예 4. 감마 망고스틴의 신경세포 독성 억제활성 측정][Experimental Example 4: Measurement of nerve cell toxicity inhibitory activity of gamma mangosteen]
1. 흥분성 신경세포 독성 억제활성 측정1. Measurement of excitatory nerve cell toxicity inhibitory activity
본 발명의 감마 망고스틴에 대한 흥분성 신경세포 독성 억제활성을 측정하기 위하여, 상기 실험예 2의 2에서 준비된 일차배양된 흰쥐 대뇌피질 신경세포를 300 μM NMDA(N-methyl-D-aspartate) 또는 100 μM 글루타메이트(glutamate)로 15분간 처리한 후 20 내지 24시간 동안 배양한 다음, 상기 실험예 1의 3에 기재된 방법과 동일하게 MTT 법을 수행하여 세포 생존율 및 상기 실험예 1의 4에 기재된 방법과 동일하게 DCF-DA를 사용하여 ROS를 측정하였다. In order to measure the excitatory neuron cytotoxicity inhibitory activity of gamma-mangosteen according to the present invention, the primary cultured rat cerebral cortical neurons prepared in Experimental Example 2 were suspended in 300 μM N-methyl-D-aspartate or 100 treated with glutamate for 15 minutes and then cultured for 20 to 24 hours. Then, the MTT method was performed in the same manner as described in Experimental Example 3, and the cell viability and the method described in 4 of Experimental Example 1 Similarly, ROS was measured using DCF-DA.
구체적으로, 배양한 신경세포를 HCSS로 세척한 다음 100 μM 글루탐산(glutamic acid) 또는 300 μM NMDA를 함유하는 Mg2+-free HCSS로 15분간 처리하고, 25 mM 포도당을 함유하는 MEM으로 배양액을 교환하여 20-24시간 동안 95% 공기, 5% CO2의 환경조건을 유지하면서 37℃의 배양기에서 배양하여 흥분성 신경세포 독성을 유발하였다. 유발된 신경세포 독성을 상기 측정법에 따라 측정하였으며, 이의 결과를 도 6에 나타내었다.Specifically, the cultured neurons were washed with HCSS, treated with Mg 2+ -free HCSS containing 100 μM glutamic acid or 300 μM NMDA for 15 minutes, and the culture medium was exchanged with MEM containing 25 mM glucose And incubated for 20-24 hours at 37 ° C in an incubator maintained at 95% air and 5% CO 2 environment to induce excitatory neuronal cytotoxicity. The induced nerve cell toxicity was measured according to the above measurement method, and the results are shown in FIG.
도 6에 나타난 바와 같이, 본 발명의 감마 망고스틴은 일차배양한 흰쥐 대뇌피질 신경세포에서 0.3 내지 3 μM 농도 범위의 NMDA 또는 글루타메이트에 의해 유발된 흥분성 신경세포 독성을 유의하게 억제하여 세포 생존율을 30% 증가시킴을 확인하였다. 또한, 본 발명의 감마 망고스틴은 NMDA 또는 글루타메이트에 의해 생성된 ROS를 각각 농도의존적으로 유의하게 감소시킴을 확인하였다.As shown in FIG. 6, the gamma-mangosteen of the present invention significantly inhibited NMDA or glutamate-induced excitatory neuronal cytotoxicity in primary cultured rat cerebral cortical neurons in a concentration range of 0.3 to 3 μM, %. In addition, it was confirmed that the gamma-mangosteen of the present invention significantly decreased the concentration of ROS produced by NMDA or glutamate, respectively.
따라서, 본 발명의 감마 망고스틴은 NMDA및 글루타메이트로 유발된 흥분성 신경세포 독성을 농도의존적으로 유의하게 억제시키므로, 신경세포의 손상을 억제하는 효과가 우수함을 확인하였다.
Therefore, the gamma-mangosteen of the present invention significantly inhibited NMDA and glutamate-induced excitatory neuronal cytotoxicity in a concentration-dependent manner, thus confirming that the effect of inhibiting neuronal damage is excellent.
2. Aβ펩타이드-유발 신경세포 독성 억제활성 측정2. Measurement of Aβ peptide-induced neuronal cytotoxicity inhibitory activity
본 발명의 감마 망고스틴에 대한 Aβ펩타이드-유발 신경세포 독성 억제활성을 측정하기 위하여, 상기 실험예 2의 2에서 준비된 일차배양된 흰쥐 대뇌피질 신경세포를 40 μM Aβ(25-35) (Amyloid β protein fragment (25-35))로 24시간 동안 처리한 후, 상기 실험예 1의 3에 기재된 방법과 동일하게 MTT 법을 수행하여 세포 생존율을 측정하였다.The primary cultured rat cerebral cortical neurons prepared in Experimental Example 2 were suspended in 40 [mu] M A [beta] (25-35) (Amyloid [beta] ) to measure the inhibitory activity of A [beta] peptide- protein fragment (25-35)) for 24 hours, and the cell survival rate was measured by MTT method in the same manner as described in Experimental Example 3.
구체적으로, 상기 1의 실험방법을 약간 변형하여 사용하여 Aβ(25-35)를 1 mM로 용해한 다음, 일주일 동안 37℃ 온도의 배양기에서 응집(aggregation)시킨 후 사용 하였다. 이후, 배양된 신경세포를 HCSS로 세척한 다음 40 μM Aβ(25-35)를 용해된 25 mM 포도당을 함유하는 MEM 배양액으로 첨가하여 95% 공기, 5% CO2의 환경조건을 유지하면서 37℃ 온도의 배양기에서 24시간 동안 배양하여 신경세포 독성을 유발하였다. 유발된 Aβ펩타이드-유발 신경세포 독성을 상기 측정법에 따라 측정하였으며, 이의 결과를 하기 도 7에 나타내었다.Specifically, Aβ (25-35) was dissolved at a concentration of 1 mM using a slight modification of the
도 7에 나타난 바와 같이, 본 발명의 감마 망고스틴은 대조군에 비하여 30 내지 40% 범위의 세포 생존율을 가지는 것으로 확인되었다. Aβ(25-35)와 0.3 내지 10 μM 농도의 감마 망고스틴을 함께 처리한 배지에서 미약하지만 유의하게 신경세포의 독성이 억제되는 것을 확인하였다. As shown in Fig. 7, gamma-mangosteen of the present invention was confirmed to have a cell survival ratio in the range of 30 to 40% as compared with the control group. Aβ (25-35) and gamma mangosteen at 0.3 to 10 μM concentration were treated together, but the toxicity of neurons was inhibited significantly.
따라서, 본 발명의 감마 망고스틴은 Aβ펩타이드-유발 신경세포 독성을 유의하게 억제하므로, 신경세포의 손상을 억제하는 효과가 우수함을 확인하였다.
Therefore, it was confirmed that the gamma-mangosteen of the present invention significantly inhibited A [beta] peptide-induced neuronal cell toxicity, and thus it was superior in the effect of inhibiting neuronal damage.
[실험예 5. 감마 망고스틴의 베타-세크레타제 억제활성 측정][Experimental Example 5: Measurement of beta-secretase inhibitory activity of gamma mangosteen]
본 발명의 감마 망고스틴에 대한 베타-세크레타제 억제활성을 측정하기 위하여, 종래에 방법에 따라 베타-세크레타제 FRET 에쎄이 키트(β-secretase fluorescence resonance energy transfer; BACE1 FRET)법을 수행하였다. 상기 베타-세크레타제는 아밀로이드 전구 단백질(amyloid precursor protein; APP)로부터 Aβ펩타이드를 생성하는 데 관여하는 단백질이다.In order to measure the beta-secretase inhibitory activity of the gamma-mangosteen of the present invention, beta-secretase fluorescence resonance energy transfer (BACE1 FRET) was performed according to the conventional method. The beta-secretase is a protein involved in the production of A [beta] peptide from amyloid precursor protein (APP).
구체적으로, 베타-세크레타제의 억제활성은 BACE1 FRET를 사용하여 제조회사에서 제시한 방법을 약간 변형하여 측정하였다. 즉, 96-웰 플레이트에 적정 농도의 감마 망고스틴 10 μM (대조군은 에쎄이 완충용액으로 대체)와 기질 20 μM을 가한 후 조심스럽게 섞은 다음 베타-세크레타제 10 μM을 넣고 마이크로플레이트 리더(SpectraMax M2e microplate)를 이용하여 여기 545 nm, 방출 585 nm에서 형광을 측정하였으며, 실온에서 2시간 동안 반응시킨 후 동일한 조건으로 형광을 측정하였다. 베타-세크레타제의 활성 억제율(%)은 상기 수학식 1를 이용하여 산출되었다. 이의 결과를 도 8에 나타내었다.Specifically, the inhibitory activity of the beta-secretase was measured by using a BACE1 FRET with a slight modification of the method proposed by the manufacturer. Specifically, 10 μM gamma-mangostin at an appropriate concentration was added to a 96-well plate (the control was replaced with an Esey buffer solution) and 20 μM of the substrate was added to the 96-well plate. The plate was carefully mixed with 10 μM of beta-secretase, The fluorescence was measured at 545 nm excitation and 585 nm emission using a microplate reader. After reacting at room temperature for 2 hours, fluorescence was measured under the same conditions. The inhibition rate (%) of the activity of beta-secretase was calculated using the above formula (1). The results are shown in Fig.
도 8에 나타난 바와 같이, 본 발명의 감마 망고스틴은 베타-세크레타제를 농도의존적으로 유의하게 억제하였으며, 이때, IC50 값은 0.96 μM로 확인되었다. As shown in FIG. 8, the gamma-mangosteen of the present invention significantly inhibited beta-secretase in a concentration-dependent manner, wherein the IC 50 value was 0.96 μM.
따라서, 본 발명의 감마 망고스틴은 베타-세크레타제를 농도의존적으로 유의하게 억제하여 Aβ펩타이드의 생성을 유의하게 저해하므로, 치매 유발인자를 저해하여 치매를 치료하는 효과가 우수함을 확인하였다.
Therefore, the gamma mangosteen of the present invention significantly inhibited the production of A [beta] peptide by significantly inhibiting beta-secretase in a concentration-dependent manner, and thus it was confirmed that the effect of treating dementia by inhibiting the dementia inducing factor is excellent.
[실험예 6. 감마 망고스틴의 일차배양한 대뇌피질 세포에서의 세포독성 측정][Experimental Example 6: Cytotoxicity measurement of primary cultured cortical cells of gamma-mangosteen]
본 발명의 감마 망고스틴에 대한 세포독성을 평가하기 위하여, 상기 실시예 1에서 제조된 감마 망고스틴을 상기 실험예 2의 2에서 준비된 일차배양된 흰쥐 대뇌피질 신경세포에 농도별(0.3 ~ 30 μM)로 각각 처리하였으며, 상기 실험예 1의 3에 기재된 방법과 동일하게 MTT 법을 수행하여 세포 생존율을 측정하였다. 이의 결과를 하기 도 9에 나타내었다.In order to evaluate the cytotoxicity of the gamma mangosteen of the present invention, the gamma mangosteen prepared in Example 1 was added to the primary cultured rat cerebral cortical neurons prepared in Experimental Example 2 at a concentration of 0.3 to 30 μM ), And cell viability was measured by MTT method in the same manner as described in Experimental Example 1, 3. The results are shown in FIG.
도 9에 나타난 바와 같이,본 발명의 감마 망고스틴은 0.3 ~ 10 μM 농도에서는 상기 신경세포의 세포 생존율에 유의한 영향을 미치지 않았으나 30 μM 농도이상부터 세포 생존율을 감소시켜 33.4%까지 현저히 감소된 것을 확인하였다.As shown in FIG. 9, the gamma-mangosteen of the present invention did not significantly affect the cell viability of the neuron at the concentration of 0.3-10 μM, but the cell viability was decreased from 30 μM concentration to 33.4% Respectively.
따라서, 본 발명의 감마 망고스틴은 30 μM 미만의 농도에서는 유의한 세포독성이 확인되지 않으나, 30 μM 이상의 농도부터는 유의한 세포독성이 확인되었으므로, 특정 농도 범위 내에서 부작용이 적음을 확인하였다.
Therefore, it was confirmed that the gamma-mangosteen of the present invention had no significant cytotoxicity at a concentration of less than 30 μM, but significant cytotoxicity at a concentration of 30 μM or more.
이하 본 발명의 감마 망고스틴을 함유하는 퇴행성 뇌질환의 예방 또는 치료용 약학적 조성물 및 퇴행성 뇌질환의 예방 또는 개선용 식품 조성물의 제제예를 설명하나, 본 발명을 한정하고자 함이 아닌 단지 구체적으로 설명하고자 함이다.
Hereinafter, the pharmaceutical compositions for preventing or treating degenerative brain diseases containing gamma-mangosteen according to the present invention and the pharmaceutical compositions for preventing or ameliorating degenerative brain diseases will be described. However, the present invention is not limited to the specific examples I want to explain.
[제제예 1. 약학적 제제의 제조] [Preparation Example 1: Preparation of pharmaceutical preparation]
1. 산제의 제조 1. Manufacturing of powder
감마 망고스틴 20 mg
유당 100 mg
탈크 10 mg
상기의 성분들을 혼합하고 기밀포에 충진하여 산제를 제조한다.
The above components are mixed and filled in airtight bags to prepare powders.
2. 정제의 제조2. Preparation of tablets
감마 망고스틴 10 mg
옥수수전분 100 mg
유당 100 mg
스테아린산 마그네슘 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.
3. 캡슐제의 제조3. Preparation of capsules
감마 망고스틴 10 mg
결정성 셀룰로오스 3 mg
락토오스 14.8 mgLactose 14.8 mg
마그네슘 스테아레이트 0.2 mgMagnesium stearate 0.2 mg
통상의 캡슐제 제조방법에 따라 상기의 성분을 혼합하고 젤라틴 캡슐에 충전하여 캡슐제를 제조한다.
The above components are mixed according to a conventional capsule preparation method and filled in gelatin capsules to prepare capsules.
4. 주사제의 제조4. Preparation of injections
감마 망고스틴 10 mg
만니톨 180 mg180 mg mannitol
주사용 멸균 증류수 2974 mgSterile sterilized water for injection 2974 mg
Na2HPO42H2O 26 mgNa 2 HPO 4 2H 2 O 26 mg
통상의 주사제의 제조방법에 따라 1 앰플당 (2 ml) 상기의 성분 함량으로 제조한다.
(2 ml) per 1 ampoule in accordance with the usual injection preparation method.
5. 액제의 제조5. Manufacture of liquids
감마 망고스틴 20 mg
이성화당 10 g10 g per isomer
만니톨 5 g5 g mannitol
정제수 적량Purified water quantity
통상의 액제의 제조방법에 따라 정제수에 각각의 성분을 가하여 용해시키고 레몬향을 적량 가한 다음 상기의 성분을 혼합한 다음 정제수를 가하여 전체를 정제수를 가하여 전체 100 ml로 조절한 후 갈색병에 충진하여 멸균시켜 액제를 제조한다.
Each component was added and dissolved in purified water according to the usual liquid preparation method, and the lemon flavor was added in an appropriate amount. Then, the above components were mixed, and purified water was added thereto. The whole was added with purified water to adjust the total volume to 100 ml, And sterilized to prepare a liquid preparation.
[제제예 2. 식품 제제의 제조][Formulation example 2. Preparation of food preparation]
1. 건강식품의 제조1. Manufacture of health food
감마 망고스틴 100 mg
비타민 혼합물 적량Vitamin mixture quantity
비타민 A 아세테이트 70 g 70 g of vitamin A acetate
비타민 E 1.0 mgVitamin E 1.0 mg
비타민 B1 0.13 mgVitamin B1 0.13 mg
비타민 B2 0.15 mg0.15 mg of vitamin B2
비타민 B6 0.5 mgVitamin B6 0.5 mg
비타민 B12 0.2 g 0.2 g of vitamin B12
비타민 C 10 mg
비오틴 10 g Biotin 10 g
니코틴산아미드 1.7 mgNicotinic acid amide 1.7 mg
엽산 50 g Folate 50 g
판토텐산 칼슘 0.5 mgCalcium pantothenate 0.5 mg
무기질 혼합물 적량Mineral mixture quantity
황산제1철 1.75 mg1.75 mg of ferrous sulfate
산화아연 0.82 mg0.82 mg of zinc oxide
탄산마그네슘 25.3 mgMagnesium carbonate 25.3 mg
제1인산칼륨 15 mgPotassium monophosphate 15 mg
제2인산칼슘 55 mgSecondary calcium phosphate 55 mg
구연산칼륨 90 mgPotassium citrate 90 mg
탄산칼슘 100 mg
염화마그네슘 24.8 mg
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.
2. 건강음료의 제조2. Manufacture of health drinks
감마 망고스틴 100 mg
비타민 C 15 gVitamin C 15 g
비타민 E(분말) 100 gVitamin E (powder) 100 g
젖산철 19.75 g19.75 g of ferrous lactate
산화아연 3.5 g3.5 g of zinc oxide
니코틴산아미드 3.5 gNicotinic acid amide 3.5 g
비타민 A 0.2 gVitamin A 0.2 g
비타민 B1 0.25 gVitamin B1 0.25 g
비타민 B2 0.3gVitamin B2 0.3g
물 정량
Water quantification
통상의 건강음료 제조방법에 따라 상기의 성분을 혼합한 다음, 약 1시간 동안 85℃에서 교반 가열한 후, 만들어진 용액을 여과하여 멸균된 2 l 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 stirred and heated at 85 DEG C for about 1 hour. The solution thus prepared was filtered and sterilized in a sterilized 2 liter container, It is used in the production of the health beverage composition of the invention.
상기 조성비는 비교적 기호음료에 적합한 성분을 바람직한 실시예로 혼합 조성하였지만 수요계층이나, 수요국가, 사용용도 등 지역적, 민족적 기호도에 따라서 그 배합비를 임의로 변형 실시하여도 무방하다.Although the compositional ratio is relatively mixed with a component suitable for a favorite drink, it is also possible to arbitrarily modify the compounding ratio according to the regional or national preference such as the demand class, the demanding country, and the use purpose.
Claims (8)
[화학식 1]
A pharmaceutical composition for preventing or treating degenerative brain diseases, comprising gamma-mangosteen represented by the following formula (1) as an active ingredient.
[Chemical Formula 1]
The pharmaceutical composition according to claim 1, wherein the gamma mangosteen is obtained from mangosteen hull.
The method according to claim 1, wherein the gamma mangosteen is obtained by extracting mangosteen hull with water, an alcohol having 1 to 4 carbon atoms or a mixed solvent thereof to obtain a crude extract, and then extracting the crude extract with hexane, chloroform, Wherein the composition is obtained by fractionation of the chloroform fraction obtained by successive fractionation with ethyl acetate, n-butanol, in order to prevent or treat degenerative brain diseases.
4. The method according to claim 3, wherein the alcohol having 1 to 4 carbon atoms is 1 to 100% (v / v) methanol or 1 to 100% (v / v) A pharmaceutical composition.
5. The method of any one of claims 1 to 4 wherein the degenerative brain disease is selected from the group consisting of dementia, mild cognitive impairment, stroke, Creutzfeldt-Jakob disease, traumatic head injury, syphilis, acquired immune deficiency syndrome, brain abscess, Hypersomnia, Parkinson's disease, schizophrenia, Huntington's disease, Pick's disease, amyotrophic lateral sclerosis, epilepsy, ischemia, paralysis, paresis, hyperactivity disorder, schizophrenia, depression, mania, posttraumatic stress disorder, , Wherein the compound is at least one kind of degenerative brain disease selected from the group consisting of:
6. The method according to claim 5, wherein the dementia is selected from the group consisting of senile dementia, Alzheimer's disease, vascular dementia, dementia of the frontal lobe, dementia due to normal pressure hydrocephalus, dementia caused by head trauma, dementia caused by metabolic diseases, Wherein the dementia is one or more dementia selected from the group consisting of dementia, dementia, and dementia.
[화학식 1]
1. A food composition for preventing or improving degenerative brain diseases, comprising gamma-mangosteen represented by the following formula (1) as an active ingredient.
[Chemical Formula 1]
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Cited By (2)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| KR20190044918A (en) | 2017-10-23 | 2019-05-02 | 안동대학교 산학협력단 | Pharmaceutical composition comprising the extracts of mangosteen peduncle as an effective component for prevention or treatment of thrombosis and health functional food comprising the same |
| CN109956952A (en) * | 2017-12-14 | 2019-07-02 | 浙江工业大学 | α-mangostin derivative and the preparation method and application thereof |
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2013
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Cited By (3)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| KR20190044918A (en) | 2017-10-23 | 2019-05-02 | 안동대학교 산학협력단 | Pharmaceutical composition comprising the extracts of mangosteen peduncle as an effective component for prevention or treatment of thrombosis and health functional food comprising the same |
| CN109956952A (en) * | 2017-12-14 | 2019-07-02 | 浙江工业大学 | α-mangostin derivative and the preparation method and application thereof |
| CN109956952B (en) * | 2017-12-14 | 2020-11-13 | 浙江工业大学 | Alpha-toosedarin derivative and preparation method and application thereof |
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