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Resumen La palta (Persea americana) es uno de los frutos con bastante abundancia en Bolivia, esto se debe a su capacidad de producirse en climas templados y cálidos, lo que trae consigo múltiples beneficios para la salud, pues hay evidencia cientifica que sugiere que la palta podría tener efectos para inhibir o destruir el desarrollo de múltiples microorganismos. Así mismo se pudo evidenciar que los extractos Clorofórmicos y Etanólicos de la semilla de la palta si tiene un efecto bacteriostático y bactericida contra cepas de M. tuberculosis, por inducir la liberación de radicales libres, sin embargo estos extractos también han demostrado tener eficacia contra otras cepas bacterianas, micóticas y parasitarias y algunos virus.
Abstract The avocado (Persea americana) is one of the most abundant fruits in Bolivia, due to its capacity to be produced in temperate and warm climates, bringing multiple health benefits, as scientific evidence suggests the avocado may have effects in inhibiting or destroying the growth of multiple microorganisms. Likewise, it has been shown that the chlorophormic and ethanolic extracts of avocado seed have a bacteriostatic and bactericidal effect against strains of M. tuberculosis, by inducing the release of free radicals; furthermore, these extracts have also been shown to be effective against other bacterial, fungal and parasitic strains and some viruses.
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OBJECTIVE:To study the chemical constituents in the chloroform extract of Fructus Canarii. METHODS:The chloroform extract of Fructus Canarii was isolated and purified by MCI,Toyopearl HW-40F,reverse-phase C18,Sephadex LH-20 column. The structure of compounds was analyzed and identified by physicochemical properties and spectral data(mass spectrum, hydrogen spectrum and carbon spectrum). RESULTS:Eight compounds were isolated from chloroform extract of Fructus Canarii, namely Dihydrophaseicacid-3′-O-β-D-glucopyranoside(1),3,4-Dihydroxybenzoic acid(2),3-O-galloylquinic acid(3),Gallic acid (4), Ethyl gallate(5), Scopoletin(6), Dllagic acid-4-O-α-L-rhamnopyranoside(7) and Isocorilagin(8). CONCLUSIONS:Compounds 1,2 and 7 were firstly obtained from Fructus Canarii. The study lays foundation for quality evaluation of Fructus Canarii.
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Objective: To set up an analysis method of fingerprints for analgesic and anti-inflammatory effective parts from crude and processed roots of Aconitum sinomontanum (AS), and to discuss the chemical composition changes after processing that enhance the analgesic and anti-inflammatory effect. Methods: HPLC gradient elution method was developed to establish fingerprints for 10 batches of chloroform extract from crude and processed the roots of AS in different areas. And the fingerprint were analyzed and compared by Chinese Materia Medica (CMM) Fingerprint Similarity Evaluation System (2012 edition). Results: The fingerprints of chloroform extract from crude and processed the roots of AS were set up by HPLC. The gained 3 and 15 common peaks from crude and processed roots of AS, respectively. processed product added 12 peaks, including 1 peak, 2 peak, 7 peak increase were significant, accounting for the new peak area of 72.3%-84.5%. And determination of lappacontine and ranaconitine of chloroform extract from crude and proceed products, after processing the content were reduced, ranaconitine content reduced to the original one-third. Conclusion: This method with good reproducibility, and strong characteristic, and could be used for the full quality evaluation of analgesic and anti-inflammatory effect parts from crude and processed the roots of AS. To provide scientific basis for elucidating the chemical substance base and processing principle of crude and processed roots of AS.
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To predict the mechanism of liver injury induced by Genkwa Flos, we investigated the effect of chloroform extract on UGTs and UGT1A1 activities of the liver microsomes in rat and human. In the present study, 4-nitrophenol(4-NP) and β-estradiol were elected as substrates to determine activities of UGTs and UGT1A1 by UV and HPLC. The results showed that there were 1.00% of apigenin, 6.40% of hydroxygenkwanin and 18.38% of genkwanin in chloroform extract; and total diterpene mass fraction was 31.40%. Compared with the control group, chloroform extract could significantly inhibit the activity of UGTs in rat liver microsomes(RLM) system, while the inhibitory effect was not obvious in human liver microsomes(HLM) system. UGT1A1 activity was inhibited by chloroform extract in rat liver microsomes and human liver microsomes (based on genkwanin, IC₅₀=8.76, 10.36 μmol•L⁻¹). The inhibition types were non-competitive inhibition(RLM) and uncompetitive inhibition(HLM). In conclusion, the results indicated that chloroform extract showed different inhibitory effects on UGTs and UGT1A1 activity, which may be one of the mechanisms of liver injury induced by Genkwa Flos.
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Objective To evaluate the protective effects of Rosemary's chloroform extract on cerebral ischemia in mice and acute toxicity.Methods The protective of rosemary's chloroform extract on cerebral ischemia was observed and compared by the mice models of cerebral anoxia and ischemia,thrombus formation in vivo,and chloroform induced arrhythmias.Rosemary's Chloroform Extract was given orally to mice to evaluate acute toxicity.Results Rosemary's chloroform extract had different degrees of inhibition of collagen-the adrenaline induced thrombus formation,and prolonged acute ischemic mice brains off mouth breathing time and increase the number of mouth breathing (P <0.05 or P <0.01);Chloroform extract significantly reduced the incidence of chloroform induced ventricular arrhythmias.Acute toxicity results suggested that a female rat died in the next day of chloroform extract group,no additional toxicity was observed.Conclusion Rosemary's chloroforrm extract has significant protective effect on cerebral ischemia and hypoxia in mice.
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The acute toxicity of chloroform extract of Artemisia maciverae Linn was studied in Swiss albino mice. The mice were randomly distributed into four groups of three animals each. The groups were respectively administered both intraperitoneally and orally chloroform extract of Artemisia maciverae at 0, 10, 100 and 1000mg/kg in a single dose and monitored frequently for 24h and daily for 13 days in the first phase of the experiment. In the second phase of the experiment, the animals were administered single doses of the extract at 0, 200, 400 and 800mg/kg both intraperitoneally and orally and monitored frequently for 24h and 13 days respectively. The number of deaths in a group was recorded. The results of the second phase experiment were used to calculate the LD50 of the plant extract. All surviving animals were sacrificed after 14 days. Selected organs of the animals i.e. heart, lungs, liver, kidney, spleen, stomach and intestine of both the dead and sacrificed animals were removed and stored in 10% formal saline ready for histopathological analysis. Tissue specimens of the organs were examined histopathologically after processing and staining with haematoxylin and eosin. Lesions were observed in the liver, kidney and intestine of mice administered 800 and 1000mg/kg of chloroform extract of Artemisia maciverae. From this result, the LD50 of the chloroform extract of Artemisia maciverae was calculated to be 566 mg/kg. The results indicate that the extract may be toxic at a high dose and short term exposure.
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Aims: To evaluate the anthelminthic activity of Annona reticulata seeds extracts against Pheretima posthuma. Study Design: Helminth infections have tormented humans and animals for thousands of years. The indiscriminate uses of the anthelminthic drugs have lead to the emergence of resistant helminths against many anthelminthic agents. Thus the need for the treatment of helminthic infections and the prevention of the emergence of resistant strains has led to the screening medicinal plants for their anthelminthic activity. Place and Duration of Study: Department of Biotechnology, The Oxford College of Science, Bangalore, Karnataka, India, between January 2012 and March 2012. Methodology: The main aim of the present exploratory study is to evaluate the anthelminthic activity of A. reticulata seeds extracts. The in vitro studies revealed that the anthelminthic effects of crude chloroform and ethanolic extracts of A. reticulata on Pheretima posthuma was evident from induction of paralysis and mortality. Piperazine citrate was used as the standard reference drug and normal saline as a control group. Results: Among all the concentrations of chloroform and ethanolic extracts tested, 12.5 mg/ml showed significant (p<0.01) anthelminthic activity. The results indicated that the ethanolic extract of A. reticulata is a more potent anthelminthic agent against Pheretima posthuma when compared with chloroform extract but less potent when compared with the standard drug. Conclusions: The results of this investigation justifies the use of the seed extracts of A. reticulata in traditional medical practice for the treatment of helminth infections.
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This study was performed to evaluate the antimicrobial activity of aerial parts of chloroform extract of Cassia auriculata L. The chloroform extract of C. auriculata were shown to possess an antimicrobial activity against two gram positive and two gram negative human pathogenic bacteria and fungi, viz. Bacillus subtilis, Staphylococcus aureus, Pseudomonas aeruginosa, Escherichia coli and fungus cultures Candida albicans and Aspergillus niger by using disc diffusion method. The extract showed antibacterial activity at all concentrations selected, but only the extract with the concentration of 300μg/ml showed maximum antibacterial activity against all the organisms except Pseudomonas aeruginosa which are comparable with the standard control, amikacin. The anti fungal activity of chloroform extract of C. auriculata revealed significant effect against Candida albicans and Aspergillus niger with the net inhibition zone of 14 and 14 mm, respectively at 300μg/ml concentration, which is almost comparable with standard control, ketokonazole used as an antifungal agent. The phytochemical analysis showed the presence of alkaloids, carbohydrates, fixed oils, fats, tannins, gum & mucilage, flavonoids, saponins, terpenoids, lignin and sterols. It is concluded that the antimicrobial activity showed by the plant was due to the presence of these phytochemicals. Further studies are highly needed for future drug development.
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This study was performed to evaluate the antimicrobial activity of aerial parts of chloroform extract of Cassia auriculata L. The chloroform extract of C. auriculata were shown to possess an antimicrobial activity against two gram positive and two gram negative human pathogenic bacteria and fungi, viz. Bacillus subtilis, Staphylococcus aureus, Pseudomonas aeruginosa, Escherichia coli and fungus cultures Candida albicans and Aspergillus niger by using disc diffusion method. The extract showed antibacterial activity at all concentrations selected, but only the extract with the concentration of 300μg/ml showed maximum antibacterial activity against all the organisms except Pseudomonas aeruginosa which are comparable with the standard control, amikacin. The anti fungal activity of chloroform extract of C. auriculata revealed significant effect against Candida albicans and Aspergillus niger with the net inhibition zone of 14 and 14 mm, respectively at 300μg/ml concentration, which is almost comparable with standard control, ketokonazole used as an antifungal agent. The phytochemical analysis showed the presence of alkaloids, carbohydrates, fixed oils, fats, tannins, gum & mucilage, flavonoids, saponins, terpenoids, lignin and sterols. It is concluded that the antimicrobial activity showed by the plant was due to the presence of these phytochemicals. Further studies are highly needed for future drug development.
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The present study investigates the anti-inflammatory activity of methanolic and chloroform extracts of Tragia cannabina. The whole plant of Tragia cannabina was extracted with methanol and chloroform by using soxhlet appara-tus. The effect of both extracts of Tragia cannabina was studied on carrageenan induced paw edema. The methanolic extract decreased the edema induced in hind paw. The percentage inhibition of paw edema was maximum with methanolic and chloroform extracts of Tragia cannabina at 300mg/kg body weight and has showed significant anti-inflammatory activity. It has been concluded that both the methanolic and chloroform extracts of Tragia cannabina showed significant anti-inflammatory activity comparable to that of reference standard Ibuprofen.
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Background & objectives: Drug resistant microbes are a serious challenge to human health. During the search for novel antibiotics/inhibitors from the agricultural soil, a bacterial colony was found to inhibit the growth of clinical isolates including Staphylococcus (resistant to amikacin, ciprofloxacin, clindamycin, clinafloxacin, erythromycin, gentamicin and methicillin) and Candida (resistant to fluconazole and itraconazole). The culture was identified as Burkholderia gladioli and produced at least five different antimicrobial compounds which were highly stable at high temperature (121°C) and in the broad pH range (3.0-11.0). We report here the antimicrobial activity of B. gladioli against drug resistant bacterial pathogens. Methods: The bacterial culture was identified using morphological, biochemical and 16S rRNA gene sequencing techniques. The antimicrobial activity of the identified organism against a range of microbial pathogens was checked by Kirby-Bauer's disc diffusion method. The antimicrobial compounds in the cell free supernatant were chloroform-extracted and separated by thin layer chromatography (TLC). Results: B. gladioli OR1 exhibited broad spectrum antimicrobial activity against drug resistant clinical isolates belonging to various genera of bacteria (Staphylococcus, Enterobacter, Enterococcus, Acinetobacter and Citrobacter) and a fungus (Candida). Based on TLC profile and bioautography studies, the chloroform extract of B. gladioli OR1 consisted of at least three anti-staphylococcal and two anti-Candida metabolites. The antimicrobial activity was heat stable (121°C/20 min) as well as pH stable (3.0-11.0). Interpretation & conclusions: The bacterial soil isolate, B. gladioli OR1 possessed the ability to kill various drug resistant bacteria and a fungus. This organism produced many antimicrobial metabolites which might have the potential to be used as antibiotics in future.
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Burkholderia gladioli/metabolismo , Candida , Clorofórmio , Resistência a Múltiplos Medicamentos , Antibacterianos , Testes de Sensibilidade Microbiana , Extratos Vegetais/farmacologia , StaphylococcusRESUMO
The present study investigates the anti-inflammatory activity of methanolic and chloroform extracts of Tragia cannabina. The whole plant of Tragia cannabina was extracted with methanol and chloroform by using soxhlet appara-tus. The effect of both extracts of Tragia cannabina was studied on carrageenan induced paw edema. The methanolic extract decreased the edema induced in hind paw. The percentage inhibition of paw edema was maximum with methanolic and chloroform extracts of Tragia cannabina at 300mg/kg body weight and has showed significant anti-inflammatory activity. It has been concluded that both the methanolic and chloroform extracts of Tragia cannabina showed significant anti-inflammatory activity comparable to that of reference standard Ibuprofen.
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Objective: To evaluate the larvicidal activity of plant extracts on Aedes aegypti. Methods:Petroleum ether, Chloroform and aqueous extracts obtained from Acalypha indica, Aerva lanata,Boerhaavia diffusa, Commelina benghalensis, Gompherna sps, Datura stramonium, Euphorpia hirta, Cynodon dactylon, Lantana camara and Tridax procumbens were used for larvicidal activity at concentration of 1000μg/ml and the mortality rate was calculated after 24 and 48hrs . The LC50 for the extracts were also estimated after 24 hrs. Results: The petroleum ether extract ofLantana camara, Tridax procumbens and Datura stramonium showed 100% mortality after 48hrs of incubation. Tridax procumbens petroleum ether extract had the least LC50 of 219 μg/ml followed by Lantana and Datura with 251and 288 μg/ml respectively. A combination of petroleum ether extracts of Aerva lanata and Cynodon dactylon, Boerhaavia diffusa and Commelina benghalensis exhibited 100% mortality of larvae. Formulation-1 inhibited the metamorphosis of the larvae by retaining 60% in its larval stage. Petroleum ether extracts of Lantana, Tridax, Datura and a combination of extracts were effective larvicide. The formulations proved to be effective in inhibiting the metamorphosis. Alkaloids and flavonoids were present in datura petroleum ether extract . Conclusions: Either the crude extracts of Datura stramonium, Lantana camara and Tridax procumbens or its phytochemicals can be used as effective vector control agents individually or in combination.
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The anti-inflammatory activity of ethanol, methanol and chloroform extracts of Exacum wightianum, was evaluated by carrageenan induced rat paw odema method. The dose effects of 200 mg/kg b.wt. of the ethanolic, methanolic and chloroform extracts of E. wightianum was more active than 100 mg/kg b.wt. and found to be statistically significant. In acute inflammation as produced by carrageenan 72.30% and 86.89% protection was observed in methanol extract of E. wightianum. These extracts did not show any sign of toxicity up to a dose of 1000 mg/kg.bw in rats.The results suggested that the methanolic extract of E. wightianum has exhibited an effective anti-inflammatory activity mediated via either by inhibition of cyclooxygenase cascade and by blocking the release of vasoactive substances like histamine, serotonin and kinins. The results also justified the use of this plant in traditional Indian medicine in the treatment of inflammation.
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OBJECTIVE: To compare TLC fingerprints between different batches of compound Herba taraxaci enemas (CHTE) ant to lay a foundation for establishing a more stable preparation technics and quality standards for CHTE. METHODS: The chloroform extract of 2 batches of CHTE were chromatographed by TLC and the samples were scanned by TLC scanner at a single wavelength of 280nm,the difference between different batches was compared. RESULTS: The TLC of chloroform extracts was well-separated,there were 6 common peaks and 2 non-common peaks in the TLC of 2 batches of samples, with some of the peaks identified in terms of the medicinal material categories, but there was a significant difference in contents among the common peaks. CONCLUSIONS: It was hard to guarantee the relative conformity in numbers of components and the contents between different batches of preparations,the preparation technics and quality standard of raw materials remain to be further optimized and the quality standard for Chinese herb medicinal preparations in hospital should be improved further.
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The experiment was conducted on the actions of 5 kinds of reagents on HL - 60 cellular wither, viz. Yisuiling chloroform extract, rabbit serum chloroform extract, rabbit liver paste chloroform extract, Etoposide, and normal rabbit serum. Results revealed that after fluid incubation for a short period, the HL-60 cultured cells showed no wither in the former 4 groups under microscope and flowing cytometer. Among them, action was strongest in rabbit liver paste of Yisuiling extract group, similar to the positive control of Etoposide. Followed by rabbit serum, and the action was weak in Yisuiling chloroform extract. There was no obvious action of induced wither by normal rabbit serum. The mechanism of induced wither is still under investigation.