Opium was dedicated by anti-drug section of Kerman Police (Iran). Based on their information the origin of opium was Helmand in Afghanistan. Streptozocin (STZ) were purchased from Pfizer Company (AG, Zurich, Switzerland). Terminal deoxynucleotidyl transferase (TdT)-mediated dUTP-X nick end labeling (TUNEL) kit was purchased from Roche Diagnostic, Manheim, Germany. Proteinase K was from Roche, Germany [20µg/ml in phosphate-buffered saline (PBS)]. DNA extraction kit was from Cinnagen, Iran. Glucose oxidase kit was also prepared from Pars azemoon company (Tehran, Iran). All of other materials were of analytical grade and obtained from standard sources.

In this experimental study, 70 male and 70 female Wistar rats (weighting 250~300 gr) were entered into the study. Animals were kept on a 12 hours light-dark cycle and had freely accessed to food and water. All animals' procedures were in accordance to "guide for the care and use of laboratory animals (NIH US publication no. 85-23 revised 1985)". 20 of each group were used as control and 50 male and 50 female rats were used for inducing diabetes by injection of streptozocin (dissolved in sodium citrate buffer, pH 4.4) with a single dose of 60 mg/kg of the body weight intravenously into the tail vein [21]. After 3 days, 0.5 ml blood was collected from orbit cavity by a thin heparinized tube. Plasma glucose was measured using glucose oxidase method and the animals with glucose level more than 250 mg/dl were regarded as diabetic [22]. The success rate of inducing diabetes was approximately 90%. 25 of the above animals along with 10 of the control (non-diabetic) animals were treated with a daily double dose (8 AM and 8 PM, ip) of opium for 8 consecutive days (Opium was dissolved in fresh saline). The protocol of opium treatment was as follow: Days one to five, 30, 60, 90, 120 and 150 mg/kg respectively and continued on 150 mg/kg for the consecutive three days (150 mg/kg was the maximum tolerable dose for animals). At day 9 after weight measurement, a single dose of 150 mg/kg opium was injected and after 3 hours animals were humanly killed by decapitation under ether anesthesia. The control groups received normal saline. All control animals survived during 14 days of experiment period. Overall 40% of STZ-diabetic rats survived during this period and there were no significant difference between males and females in this regard. Finally the liver and brain of 7 animals of each group were used for apoptosis assessment. The withdrawal signs in opium-dependent rats were observed from the 5^th day of opium injection. These signs which were sometime observed for a short time before next injection were wet-dog shakes as the first sign, and then hyperactivity, irritability, head shakes, ptosis, and writhing.

The rat brains and liver were rapidly removed and fixed at room temperature in phosphate-buffered saline (PBS; 0.1 M Sodium phosphate, 0.14 M NaCl, pH 7.4) containing 3.7% paraformaldehyde for 30 minutes. The tissues transferred to fresh 3.7% paraformaldehyde and incubated for 7.5 hours. Brains transferred to 75% ethanol and wash for 1 hour and repeated the wash using fresh 75% ethanol. This step was repeated by using of 95% ethanol and washing process was followed by 100% ethanol. The tissues transferred to xylenes and washed twice for 1 hour. The tissues embedded in molten paraffin wax (58℃) for 1 hour using new paraffin wax.

The apoptotic nuclei DNA fragmentation (the final result of the apoptotic process), was evaluated by Terminal deoxynucleotidyl transferase (TdT)-mediated dUTP-X nick end labeling (TUNEL) technique using the in situ cell death detection kit as described by manufacturer. Briefly, paraffin-embedded tissue sections (5µm), were treated with proteinase K (2µg/ml in PBS) at room temperature for 10 min and then soaked in PBS for 5 min. Sections were then incubated with 50µl terminal deoxynucleotidyl transferase and nucleotide mixture (TUNEL Label Mix) in a humidified chamber at 37℃ for 1 hour in the dark. The sections were immersed in PBS. Slides were washed in PBS, and visualized with a fluorescent microscope (Micros Austria) using an excitation wavelength of 450~500 nm. Quantitative evaluation of apoptosis index was performed by manual counting of positively stained nuclei in 30 microscopic fields at ×100 magnifications.

Gel electrophoresis is a simple method for detection of apoptosis. DNA extraction was performed according to the manufacturer's protocol. Briefly, a volume of 100µl protease was added to 50 mg brain or liver tissue and was vigorously vortexed, and followed by addition of 5µl of protease and then was incubated at 55℃ for 2 hours. At the end of incubation time 400µl of lyses solution was added, vortexed and homogenized for 15~20 minutes and followed by addition of 300µl of precipitation solution and vortexing for 3~5 seconds and then centrifuged for 10 minutes at 1,200 g. The supernatant was discarded and 1 ml of washing buffer was added to the resultant pellet, 3~5 seconds vigorously vortexed and centrifuged for 5 minutes at 1,200 g. The washing step was repeated twice and at the end of second step washing buffer was discarded and the pellet was dried at 65℃ for 5 minutes. Finally 50µl of solvent buffer was added, gently vortexed and incubated at 65℃ for 5 minutes, centrifuged for 30 seconds at 1,200 g. The resultant product is a biphasic solution which the upper layer is DNA product and the lower is the other materials. DNA was run on a 1.8% agarose gel electrophoresis at 5 V/cm in 0.5×TE buffer (Tris 10 mM; EDTA 1mM, pH 8.0) containing 10µg/ml ethidum bromide.

All analysis was performed by SPSS (version 18; SPSS Inc.). For comparison of mean values between two groups, the student's t-test was used. To compare values between multiple groups, analysis of variance (ANOVA) was applied. All values are means±SEM. p<0.05 was considered statistically significant.