Determination of abortifacient activity

Three groups of mature virgin female rats (n= 5) weighing 195-225g were employed in this experiment. The rats were allowed mating with males of proven fertility at night.The vaginal smears were examined every morning for detection of spermatozoa.The day on which spermatozoa were detected in vaginal smears was considered day 1 of pregnancy⁷. On the 15th day of pregnancy groups I and II were given the methanolic leaves extract by gavage in a single dose of 3 g/kg and 5.5g/kg body weight, respectively and group III (control) was given an equal volume of vehicle ( 2% Tween - 80) by the same route. All animals were observed daily and autopsied 48 hours after dosing. Then the number of dead and viable fetuses was evaluated as described by Gebrie et al ⁸.

Determination of estrogenicity

Uterotrophic bioassay of bilaterally ovariectomized (OVX) female rats weighting 150-170g was used to determine estrogenicity of the extract⁹. Two groups of OVX rat models (n=5) were considered. After 10 days of ovariectomy the first group received 1 g/kg body weight of methanolic leaves extract by gavage for 7 days. The other group (control) received by the same route an equal volume of vehicle (2% Tween - 80) by the same route for the same number of days. On the 8th day, body weights were recorded, and all rats were sacrificed by cervical dislocation. The uterus was carefully dissected and removed with its luminal fluid and weighed quickly on a balance with 0.0001 precision.The ratio of the uterine weight to body weight was calculated for each animal by using the method of Yamasaki et al ¹⁰.

Effect of the extract on pituitary weight

The experiment was done on two groups of female rats (n=6) with body weight ranging between 150 to 175g. One of the groups was given methanolic leaves extract at a dose of 1g/kg body weight by gavage for 15 days, while another group was given an equal volume of vehicle (2 % Tween- 80) by the same route for the same duration. At day 16, all rats were deeply anesthetized with diethyl ether and, thoracic cavity was opened and brains were fixed with perfusate solution composed of 4% formalin in 0.1 M phosphate buffered saline by applying the gravity method of Miki et al.¹¹. After perfusing the brain, the skull was opened, and the pituitary was carefully detached from the brain tissue and weighed wet on a balance with 0.0001 precision.Then the ratio of weight of pituitary to body weight was calculated according to the method of Choundhary et al¹².

Effect of the extract on hormones and lipid profile

Two groups of female rats (n=5) weighing 205- 230 were used.The first group was given 1g/ kg body weight of methanolic leaves extract by gavages for 14 days as described by Benie et al ¹³. The control group was given an equal volume of vehicle (2% Tween - 80) by gavage for the same duration. On the 15^th days, all rats were anesthetized with ether, and blood was directly collected by puncture of the right atrium. The blood was allowed to coagulate and centrifuged at 3000 rpm for 10 minutes.The serum was collected and stored at – 20 °C until analysis. The sera were analyzed for progesterone and estradiol by using electrochemiluminescence immunoassay (ECLIA). At the same time sera were also analyzed for total cholestrol, triglyceride, LDL and HDL concentrations by using enzymatic colorimetric methods (SEAC ch 16)

Statistical analysis

Data were analyzed by using SPSS and Graphpad prism softwares. all the data were expressed to the mean value ±S.E.M and the level of significance were determined by student’s t-test. A probability level less than 5% (p<0.05) was considered statistically significant difference between test and control groups for measured values.

Results

Table 1 shows that the methanolic leaves extract of Achyranthes aspera significantly (P<0.05) reduced survival of fetuses at the higher dose (5.5g/kg). It, however, did not show significant abortifaccient activity at the lower dose (3g/kg). The extract significantly (p<0.05) increased the uterine wet weight compared to the controls ( Table 2). As shown in Table 3, the mean wet weight of pituitary was significantly (p<0.05) higher for the test group. The mean serum concentration of estradiol and progesterone for the extract treated group were not significantly higher than that for the control ( Table 4). The extract was observed to have significant (p<0.05) hypolipidemic effect only on HDL ( Table 5).

Discussion

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