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Annona senegalsnsis

Afr. J. Trad. CAM (2006) 3 (1): 137 - 141
Complementary and
Alternative Medicines
Short communication

ISSN 0189-60162005
IN VIVO ANTIMALARIAL AND CYTOTOXIC PROPERTIES OF ANNONA
SENEGALENSIS
EXTRACT

Edith Ajaiyeoba1*, Mofolusho Falade2, Omonike Ogbole3, Larry Okpako4 and Dora
Akinboye2.
1Department of Pharmacognosy, Faculty of Pharmacy, University of Ibadan, Nigeria. 2Department of Zoology, Faculty of Science, University of Ibadan, Nigeria, 3Department of Pharmacognosy, Faculty of Pharmacy, Olabisi Onabanjo University Sagamu, Nigeria. 4National Institute for Pharmaceutical Research & Development, P.M.B. 21, Garki, Abuja,
Abstract

The in vivo animal antimalarial and in vitro cytotoxic activities of the methanol extract of Annona senegalensis Pers. (Annonaceae) was investigated in this study. The in
vivo
antimalarial activity of the methanol extract against Plasmodium berghei was assessed
using the 4-day suppressive test procedure. The extract of A. senegalensis had intrinsic
antimalarial property that were dose – dependent. At doses of 100mg/kg weight of mice, it
produced significant chemosuppression of parasitemia (> 57%) when administered orally.
It had the highest activity at 800mg/kg weight of mice (91.1%) compared to Chloroquine
disphosphate, the standard reference drug which had a chemosuppression of 96.2%. The in
vitro
cytotoxicity evaluations were perfomed using A2780 ovarian cancer cells in the drug
sensitivity assay. Extract of A. senegalensis exhibited low cytotoxicity with an IC50 of
28.8µg/ml. Preliminary phytochemical screening of the plant extract indicated the presence
of alkaloids, saponins, tannins and cardiac glycosides. This finding supports the traditional
use of the plant for the treatment of malaria.
Key words: Annona senegalensis, Mice Antimalarial, Cytotoxicity, Plasmodium berghei

Introduction

Malaria is one of the most important parasitic diseases in the world. It remains a major public health problem in Africa responsible for the annual death of over one million children below the age of five years (Butler, 1997; Geoffrey, 1998). Plasmodium falciparum, the most widespread etiological agent for human malaria, is becoming increasingly resistant to standard antimalarial drugs which necessitate a continuous effort to search for new drugs, particularly with novel modes of action (Muregi et al., 2003). Afr. J. Trad. CAM (2006) 3 (1): 137 - 141

Plants have invariably been a rich source for new drugs and some antimalarial drugs in use
today (quinine and artemisinin) were either obtained from plants or developed using their
chemical structures as templates (Gessler et al., 1994). It is already estimated that 122
drugs from 94 plant species have been discovered through ethnobotanical leads (Fabricant
and Farnsworth, 2001). Plants commonly used in traditional medicine are assumed to be
safe due to their long usage in the treatment of diseases according to knowledge
accumulated over centuries. However, recent scientific findings has shown that many
plants used as food or in traditional medicine are potentially toxic, mutagenic and
carcinogenic ( Schimmer et al., 1994; De Sã Ferrira and Ferrão Vargas, 1999). A number
of studies have been undertaken to evaluate the inhibitory effects of various plant extracts
on P. falciparum (Le Tran et al., 2003; Muregi et al., 2003). Similarly, the in vivo
antimalarial properties of several plant extracts have been studied in mice (Agbaje and
Onabanjo, 1991; Perez et al., 1994; Andrade-Neto et al., 2003). Following this trend, this
study presents the results obtained from the evaluation of the in vivo antiplasmodial
activity of A. senegalensis, a plant commonly used in Nigerian folk medicine against
malaria and its in vitro cytotoxicity evaluation using Human A2780 ovarian cancer cells.
Materials and Methods
Plant Preparation

The fresh leaves of A. senegalensis (Pers)(Annonaceae) were collected in Oyo, Oyo State of Nigeria. The identification and authentication was done by Mr. T. K. Odewo of
Forestry Research Institute of Nigeria (FRIN), Ibadan, where a voucher specimen was
deposited with FHI number 106411.
The leaves of the plant were carefully sun-dried for three days and samples were
pulverized to a coarse powder. 650g of the leaves were extracted exhaustively using
methanol by maceration for 72 hours. The extracts were filtered and the filtrate
concentrated over a water bath to dryness. Appropriate concentrations of the extract were
made in water and used in the experiments.
Phytochemical screening

Standard screening tests of the extract were carried out for various plant constituents. The methanol extract was screened for the presence of alkaloids, flavonoids,
saponins glycosides and tannins using standard procedures (Sofowora, 1993).
Malaria Parasites

The chloroquine-sensitive strain of Plasmodium berghei (NK-65) was used to test for antimalarial activity of the methanol extracts of A. senegalensis leaves. Parasite was obtained from the Malaria Research Laboratories, Institute for Advanced Medical Research and Training (IAMRAT), College of Medicine, University of Ibadan. Parasites are maintained through weekly blood passage in mice. Afr. J. Trad. CAM (2006) 3 (1): 137 – 141
In vivo antimalarial test

The Peters’ 4-day suppressive test against P. berghei infection in mice was employed (Peters, 1965). Briefly, adult Swiss male albino mice weighing 18-20g were
inoculated by intra-peritoneal (i.p.) injection with 1x107 infected erythrocytes. The mice
were randomly divided into groups of five per cage and treated during 4 consecutive days
with daily doses of the extracts by oral route (800, 600, 400, 200 and 100mg/kg). Two
control groups were used in each experiment, one treated with chloroquine at total dose of
25 mg/kg while the other group was kept untreated given normal saline as placebo. All
experiments were done in triplicate. On day 5 of the test, thin blood smears were prepared
and blood films were fixed with methanol. The blood films were stained with Giemsa, and
then microscopically examined (1000 x magnification). The percentage suppression of
parasitaemia was calculated for each dose level by comparing the parasitaemia in infected
controls with those of treated mice. Chloroquine disphosphate was used as positive control
while normal saline was used as a negative control.
In vitro cytotoxicity assay

Cytotoxicity against A2780 human ovarian cancer cells was performed at Virginia Polytechnic Institute and State University (USA) as previously reported (McBrien et al.,
1995). Briefly, growth inhibition was determined using a micro plate assay in which the
A2780 cells were seeded in RPMI 1640 media plus L-glutamine (Gibco) and 100% fetal
bovine serum (Gibco) at a density of 2.7x105 cells/ml. Samples were dissolved in 50%
DMSO and transferred to 96-well microtiter plates in a 1:50 dilution, for a final testing
concentration of 20 µg/ml. Microtiter plates were incubated at 37 0C in 5% CO2 for 48
hours. The medium was then replaced with RPMI 1640 plus 1% Alamar Blue (Bioresource
International). After a further 4 hours of incubation, fluorescent Alamar Blue was
measured using a microplate fluorometer (Cytofluor, Millipore) at an emission of 530 nm,
an excitation of 590 nm and a gain of 40. Percentage fluorescence is directly proportional
to percentage inhibition and growth inhibition was elucidated using a linear regression
analysis of the dose response curve. Activity is reported as IC50, which is the concentration
(µg/mL) necessary to produce 50% inhibition. Actinomycin (IC50, 2 ng/ mL) was used as a
positive control.
Results

The suppressive activity of the methanol extract of A. senegalensis against P. berghei in mice is shown in Table 1. The extract at 100mg/kg weight of mice gave 57.1% suppression of parasitaemia. At doses of 800mg/kg weight of mice, it induced the highest chemosuppression of parasitaemia (91.1%) compared to Chloroquine control group, which had a chemosuppression of 96.2%. Percentage chemosuppression was observed to increase as extract concentration increased. After 4 days treatment with extracts, the results showed mean parasitaemia in mice from the ranges of 0.33% ± 0.12% to 2.04% ± 0.34%. Afr. J. Trad. CAM (2006) 3 (1): 137 - 141
The mean parasitaemia in chloroquine control group was 0.17% ± 0.08%, while mean parasitaemia in the untreated control was 4.50 ± 0.17%. A. senegalensis was tested for cytotoxicity against human A2780 ovarian cancer cells. It was found to have an IC50 of 28.8µg/ml.

Table I. Antimalarial activity of Annona senegalensis
methanolic extracts and chloroquine in
mice infected with Plasmodium berghei.

Extract/Drug dosea Activity against P. berghei in mice (%)b
(mg/kg/day)
Mean % Chemosuppression Parasitaemia (%) aCQ, Chloroquine diphosphate (25 mg/kg/day); N.S (Untreated control), normal saline.
b Values are Parasite density ± Standard deviation (PD ± SD).
Discussion

Annona senegalensis, a plant commonly used in Nigerian folk medicine against malaria was observed to show some intrinsic antimalarial activity judging by its percentage chemosuppression in comparison with that of chloroquine in the 4 - day suppressive test (Peters, 1965). Treatment of mice infected with P. berghei with methanolic extracts of A. senegalensis showed a dose-dependent chemosuppression in comparison with chloroquine treated controls with the 800mg/kg treated group of mice showing the highest percent chemosuppression. The activity might be attributed to the presence of alkaloids that have been shown to be the major constituents identified in Annona species (Gbeassor et al, 1990; Rupprecht et al., 1990). However, the active compound(s) known to give this observed activity need to be identified. In this regard, efforts are presently directed towards biologically guided fractionation of this plant in order to isolate and identify the active compound(s) and also test for cytotoxic activity. The extract of A. senegalensis exhibited low cytotoxicity with an IC50 of 28.8µg/ml. Although plants used medicinally are widely assumed to be safe, many are potentially toxic. This study has however, established the rationale for the traditional use of this plant in Nigeria and like many others, showed that medicinal plants, which have folklore reputations for antimalarial properties, can be investigated, in order to establish their efficacy and to determine their potentials as sources of new antimalarial drugs. Afr. J. Trad. CAM (2006) 3 (1): 137 - 141

Acknowledgements

This study received partial funding from UNDP/WHO/TDR/MIM African grant ID 980046. We are grateful to Jennifer Schilling, Prof. DGI Kingston Research Group, VT,
Blacksburg, USA for cytotoxicity assay.

References
1. Andrade-Neto, V. F., Brandao, M.G. L., Stehmann, J. R., Oliveira, L. A. and Krettli, A. U.
(2003). Antimalarial activity of Cinchona- like plants used to treat fever and malaria in Brazil.
J. Ethnopharmacol. 87: 253-256.
2. Agbaje, E.O. and Onabanjo, A.O. (1991). The Effects of extracts of Enantia chlorantha in malaria. Ann. Trop. Med. Parasitol. 85:585-590.
3. Butler, D. (1997). Time to put malaria control on the global agenda. Nature 386: 535 -536.
4. De Sã Ferrira, I. C. F. and Ferrão Vargas, V. M. (1999). Mutagenicity of medicinal plant
extracts in salmonella/microsome assay. Phytother. Res. 13: 397 – 400.
5. Fabricant, D. S. and Farnsworth, N. R. (2001). The value of plants used in traditional medicine for drug discovery. Environmental Health Perspectives 109: 69 -75.
6. Gbeassor, M., Kedjagni, A.Y., Koumaglo, de Souza, C., Agbo, K., Aklikokou, K. and Amegbo, D. A. (1990). In vitro antimalarial activity of six medicinal plants. Phytother. Res. 4
(3):
115-117.
7. Geoffrey, P. (1998). The treatment of Falciparum malaria in African children. African Health 20: 19-20.
8. Gessler, M. C., Nkunya, M. H. H., Mwasunmbi, L. B., Heinrich, M. and Tanner, M. (1994). Screening Tanzanian medicinal plants for antimalarial activity. Acta Trop. 56:65-77.
9. Le Tran, Q., Tezuka, Y., Ueda, J., Nguyen, N. T., Maruyama, Y., Begum, K., Kim, H.S., Wataya, Y., Tran, Q.K. and Kadota, S. (2003). In vitro antiplasmodial activity of antimalarial
medicinal plants used in Vietnamese traditional medicine. J. Ethnopharmacol. 86: 249-252.
10. McBrien, K. D., Bery, R. L., Lewes, S.E., Nedderman, K. M., Bursuker, I., Huang. S., Wehr, S. E. and Leet, J. E. (1995). Rakicidins, a new cytotoxic lipopeptide from Micromonospora sp.
fermentation, isolation and characterization. J. Antibiot. 48: 1446-1452.
11. Muregi, F. W., Chhabra, S. C., Njagi, E. N. M., Lang’at-Thoruwa, C. C., Njue, W. M., Orago, A. S. S., Omar, S. A. and Ndiege, I. O. (2003). In vitro antiplasmodial activity of some plants
used in Kisii, Kenya against malaria and their chloroquine potentiation effects. J.
Ethnopharmacol. 84: 235-239.
12. Perez, H. A., De la Rosa, M. and Apitz, R. (1994). In vivo activity of ajoene against rodent malaria. Antimicrob. Agents Chemother. 38: 337-339.
13. Peters, W., 1965 Drug resistance in Plasmodium berghei I. Chloroquine resistance. Exptl. Parasitol. 17: 80-89.
14. Rupprecht, J. K, Hui, Y. H. and McLaughlin, J. L. (1990). Annonaceous acetogenins: a review. Journal of Natural Products 53(2): 237-278.
15. Schimmer, O., Kruger, A., Paulini, H. and Haefele, F. (1994). An evaluation of 55 commercial plant extracts in the Ames mutagenicity test. Pharmazie 49: 448 – 451.
16. Sofowora, E. A (1993). Medicinal plants and traditional medicine in Africa, 2nd edition, P.

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