The present invention refers to the application of berberine, or an active metabolite thereof, or a pharmaceutically acceptable salt thereof in the preparation of a drug for preventing and/or treating phenylketonuria. It belongs to the technical field of medicinal technology.
Phenylketonuria (PKU) is a common amino acid metabolism disorder. It is caused by the defect of phenylalanine hydroxylase in the metabolic pathway of phenylalanine, making phenylalanine unable to be converted to tyrosine. This results in the accumulation of phenylalanine and phenylpyruvate and excreted in large amounts from the urine. Pediatric phenylketonuria is a common autosomal recessive disorder. The child is normal at birth, and the symptoms usually appear at 3 to 6 months after milk feeding starts. The symptoms become obvious at the age of 1 year. The main clinical features of phenylketonuria are mental retardation, mental and neurological symptoms, eczema, skin scratch marks, pigment loss, rat odor, and electroencephalographic abnormalities, etc. If early diagnosis and treatment are available, the aforementioned clinical manifestations may not occur. The intelligence will be normal, and the electroencephalographic abnormalities can be restored. At present, the most commonly used therapeutic method is to reduce the amount of phenylalanine in breast milk or infant formula. There is no drug for prevention/treatment in clinic.
Recent evidence suggests that the alterations in intestinal bacteria can affect the activities of central nervous system in animals, leading to the changes in the function and behavior of brain. The experimental results have supported the hypothesis of “gut-brain axis”. However, the molecular mechanisms and chemical basis of the dialogue between host and bacteria remain unclear. It is very likely that intestinal bacteria regulate the function of brain through the production of metabolites by themselves which affect the biosynthesis of neurotransmitters, such as serotonin, and thereby affecting the physiological functions of host. Thus, clarifying the action mode of gut-brain pathway may help us understand the new functions of intestinal bacteria and facilitate the discovery of new methods to treat central nervous system disorders.
Berberine (BBR) is a natural compound which can be isolated from different kinds of plants, such as Coptis, Berberis, Goldenseal, and Cortex Phellodendri, etc. Berberine has been used as an over-the-counter drug to treat diarrhea without significant adverse effects in patients for several decades. Since 2004, we have discovered that berberine can be used as a new drug for the treatment of hyperlipidemia and type 2 diabetes. Its clinical efficacy has been confirmed by many research groups both at home and abroad. At the meantime, berberine has been shown to improve cognitive function and increase learning and memory in rodent models. The present patent describes that oral administration of berberine can reduce the level of blood phenylpyruvate while increase the level of tyrosine in α-methylphenylalanine induced phenylketonuria models of suckling rats, resulting in a down regulated ratio of phenylalanine/tyrosine. Accordingly, the levels of dopa and dopamine in brain after treatment are significantly increased in a-methylphenylalanine induced phenylketonuria models of SD suckling rats. While the intraperitoneal injection of berberine group and pseudo-germ-free animal oral berberine group have no obvious effect. Oral administration of berberine analogs, namely jatrorrhizine and dihydroberberine, can reduce the level of phenylpyruvate and the ratio of phenylalanine/tyrosine in blood of ICR mice as well.
Dopamine is one of the most important neurotransmitters in human and oral administration of berberine can increase the expression of dopa and dopamine in the brain of phenylketonuria models of suckling rats. At present, there is a lack of effective drugs for the treatment of phenylketonuria in children in clinic. Oral administration of berberine is able to improve the metabolic pathway of phenylalanine, increasing the biosynthesis of tyrosine from phenylalanine, and reducing the biotransformation of phenylpyruvate from phenylalanine. The increased tyrosine synthesis activates the synthesis pathway of dopa-dopamine, leading to a significant increase in the expression of dopamine in brain. Thus, the present patent describes that oral administration of berberine or an active metabolite thereof, or a pharmaceutically acceptable salt thereof, can reduce the level of phenylpyruvate and the ratio of phenylalanine/tyrosine in blood of SD suckling rats or ICR mice, thereby increasing the levels of dopa and dopamine in brain, suggesting their application in preventing and/or treating phenylketonuria. The mechanisms may be related to the gut-brain axis pathway under the regulation of intestinal bacteria.
The technical problem to be solved in the present invention is to provide a new drug for preventing and/or treating phenylketonuria.
To solve the technical problem in the present invention, the technical proposal is provided in the present invention as follows.
The present invention provides the use of berberine represented by Formula (I), an active metabolite thereof, or a pharmaceutically acceptable salt thereof in the preparation of a drug for preventing and/or treating phenylketonuria,
Said active metabolite of berberine mentioned above includes jatrorrhizine represented by Formula (II), dihydroberberine represented by Formula (III), thalifendine represented by Formula (IV), berberrubine represented by Formula (V), demethyleneberberine represented by Formula (VI), palmatine represented by Formula (VII), and columbamine represented by Formula (VIII),
Said pharmaceutically acceptable salt includes hydrochloride, sulfate, hydrobromate, hydroiodate, formate, acetate, or oxalate.
Said phenylketonuria mentioned is caused by elevated phenylpyruvate in blood.
Using α-methylphenylalanine induced phenylketonuria model of suckling rats is one of the important experiments in evaluating phenylketonuria.
α-Methylphenylalanine induced suckling rats are used, in which the concentration of phenylpyruvate in blood is significantly higher than that of the normal control group, and the ratio of phenylalanine/tyrosine is significantly higher than that in the normal control group. These results indicate that the metabolism of phenylalanine in suckling rats having phenylketonuria is abnormal and a large amount of phenylpyruvate is produced from phenylalanine, rather than tyrosine. The phenylpyruvate and the ratio of phenylalanine/tyrosine in blood of the suckling rats are significantly lower than that of the model group after oral administration of berberine. The oral administration of berberine can improve the metabolism of phenylalanine, and further prevent and/or treat the phenylketonuria.
The phenylpyruvate concentration and ratio of phenylalanine/tyrosine in blood are the key indicators for evaluating the therapeutic effect in phenylketonuria model of suckling rats.
1. Experimental Animals, Instruments and Reagents
SD suckling rats (1 day old) were purchased from Beijing Vital River Laboratory Animal Technology Co., Ltd. All the animals and female rats were fed in SPF environment (21±2° C., 12-hour photoperiod) and had free access to food and water during the experiment. Berberine was purchased from the J&K Technology Co. LTD (Beijing, China). Phenylpyruvate, phenylalanine, and tyrosine were purchased from Solarbio Science&Technology Co. LTD (Beijing, China). α-Methylphenylalanine was purchased from Sinuokai Technology Co. LTD (Nanjing, China).
2. Experimental Instruments and Analysis Methods
High-performance liquid chromatography-triple quadrupole tandem mass spectrometry (LC-MS/MS 8050, Shimadzu Corporation, Japan) was used to quantitatively determine the concentration of dopa, phenylalanine, tyrosine, and phenylpyruvate. Alltima C18 (5 μm, 4.6×150 mm) chromatography column was used in the experiment, and the column temperature was maintained at 40° C. The mobile phase to measure L-dopa was water-formic acid (100: 0.2 v/v) and acetonitrile. The condition of gradient elution was as follows (A: B, 0 min, 90:10; 2.5 min, 80:20; 2.51 min, 5:95; 5 min, 5:95; 5.01 min, 90:10; 8 min 90:10). The flow rate was 0.8 mL/min. Multi-reaction monitoring mode was used for quantization, and the quantitative ion pair of dopa was 198.15→52.05 (m/z). Phenylalanine, tyrosine, and phenylpyruvate level were determined using Alltima C18 (5 μm, 4.6×150 mm) chromatography column at column temperature of 40° C. The mobile phase contained water-formic acid (100:0.1 v/v) and methanol. The condition of gradient elution was as follows (A: B, 0 min, 90:10; 1 min, 90:10; 1.01 min, 60:40; 5 min, 5:95; 7 min, 5:95; 7.01 min 90:10; 10 min 90:10). The flow rate was 0.8 mL/min. Multi-reaction monitoring mode was used for quantization. The quantitative ion pair was: phenylalanine, 165.85→120.20; tyrosine, 182.00→136.10; phenylpyruvate, 163.00→91.00.
3. Experimental Design and Animal Grouping
Experimental design: The animals were divided into 6 groups, including: the normal control group, the model group, the low-dose of oral berberine treated model group, the high-dose of oral berberine treated model group, the intraperitoneal berberine treated model group, and the oral berberine treated pseudo-germ-free model group. The establishment of model started at 2 days old of SD suckling rats, which were administrated for 10 days, and then they were treated for 7 days.
Animal grouping:
(1) Normal control group: normal saline (s.c.).
(2) Model group: a-methylphenylalanine (s.c. 50 mg/kg/d), and phenylalanine (s.c. 200 mg/kg/d);
(3) Low-dose of oral berberine treated model group: α-methylphenylalanine (s.c. 50 mg/kg/d), phenylalanine (s.c. 200 mg/kg/d), berberine (oral, 100 mg/kg/d);
(4) High-dose of oral berberine treated model group: α-methylphenylalanine (s.c. 50 mg/kg/d), phenylalanine (s.c. 200 mg/kg/d), berberine (oral, 200 mg/kg/d);
(5) Intraperitoneal berberine treated model group: α-methylphenylalanine (s.c. 50 mg/kg/d), phenylalanine (s.c. 200 mg/kg/d), berberine (i.p. 20 mg/kg/d);
(6) Oral berberine treated pseudo-germ-free model group: α-methylphenylalanine (s.c. 50 mg/kg/d), phenylalanine (s.c. 200 mg/kg/d), berberine (oral, 200 mg/kg/d); Antibiotic dose: cefadroxil (100 mg/kg/d), oxytetracycline (300 mg/kg/d), erythromycin (300 mg/kg/d).
4. Results
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The concentrations of phenylpyruvate and tyrosine in blood are the key indicators to evaluate the therapeutic effect for phenylketonuria in children.
1. Experimental Animals, Instruments and Reagents
ICR mice (male, 20±2 g) were purchased from Beijing Vital River Laboratory Animal Technology Co., Ltd. All the animals were fed in SPF environment (21±2° C., 12-hour photoperiod) and had free access to food and water during the experiment. Berberine was purchased from the J&K Technology Co. LTD (Beijing, China). Phenylpyruvate, phenylalanine, and tyrosine were purchased from Solarbio Science&Technology Co. LTD (Beijing, China).
2. Experimental Design and Animal Grouping
Experimental design: The animals were divided into three groups, including the control group, the 200 mg/kg jatrorrhizine oral treated group at 12 h, the 200 mg/kg jatrorrhizine oral treated group at 24 h.
Animal Grouping:
(1) The control group: saline 0.2 mL (oral);
(2) The 200 mg/kg jatrorrhizine singe oral treated group at 12 h: 200 mg/kg jatrorrhizine (oral);
(3) The 200 mg/kg jatrorrhizine single oral treated group at 24 h: 200 mg/kg jatrorrhizine (oral).
3. Results
As shown in
As shown in
The concentrations of phenylpyruvate and tyrosine in blood are the key indicators to evaluate the therapeutic effect for phenylketonuria.
1. Experimental Animals, Instruments and Reagents
ICR mice (male, 20±2 g) were purchased from Beijing Vital River Laboratory Animal Technology Co., Ltd. All the animals were fed in SPF environment (21±2° C., 12-hour photoperiod) and had free access to food and water during the experiment. Berberine was purchased from the J&K Technology Co. LTD (Beijing, China). Dihydroberberine was purchased from the Mansite Biology & Technology Co. LTD (Chengdu, China). Phenylpyruvate, phenylalanine, and tyrosine were purchased from Solarbio Science&Technology Co. LTD (Beijing, China).
2. Experimental Design and Animal Grouping
Experimental design: The animals were divided into three groups, including the control group, the 200 mg/kg dihydroberberine oral treated group at 12 h, the 200 mg/kg dihydroberberine oral treated group at 24 h.
Animal Grouping:
(1) The control group: saline 0.2 mL (oral);
(2) The 100 mg/kg dihydroberberine singe oral treated group at 12 h: 100 mg/kg jatrorrhizine (oral);
(3) The 100 mg/kg dihydroberberine singe oral treated group at 24 h: 100 mg/kg jatrorrhizine (oral).
3. Results
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Number | Date | Country | Kind |
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201710231436.5 | Apr 2017 | CN | national |
Filing Document | Filing Date | Country | Kind |
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PCT/CN2018/078910 | 3/14/2018 | WO | 00 |