RETRACTED ARTICLE: Neuropathological and neuroprotective features of vitamin B₁₂ on the dorsal spinal ganglion of rats after the experimental crush of sciatic nerve: an experimental study

All experimental protocols were approved by the local animal care committee in accordance with Faculty of Urmia Veterinary Medicine office regulations. In current study, 36 Wister-albino rats of both sexes, weighing 200–250 g, with averagely 6 weeks old were selected. The animals were kept two by two in individual propylene cages under standard laboratory conditions by the dimensions of 30×50×25 cm³. Rats were maintained on a 12 hour light/dark cycle at 22±1°C and 50±10% humidity. The animals were kept in standard room conditions and fed with standard rat diet and water ad libitum.

The rats were divided into six groups and randomly allotted into one of six experimental groups each group contained six animals. Control animals in group A received normal saline (for 42 days) (n=6), and test animals in group B received vit B₁₂following surgery (0.5 mg/kg/day for 21 days) (n=6); however, test animals of group C received vit B₁₂following surgery (1 mg/kg/day for 21 days) (n=6). Test animals in group D received vit B₁₂following surgery (0.5 mg/kg/day for 42 days) (n=6), whereas test animals in group E received vit B₁₂following surgery (1 mg/kg/day for 42 days) (n=6), and in F: Sham group had no surgery and vit B₁₂injection, and were euthanized after 42 days (n=6) in order to necropsy examination. In addition, the vit B₁₂in experimental group was injected intraperitoneally.

DRG of the spinal cord segment L5 which mainly sciatic nerve is originated from is located in L1 vertebral column of the rat. Therefore, to remove it, according to the method of the mentioned article, spinal segment, dorsal root and related ganglion were removed from L1 of the vertebral column [28]. All of the operations were performed under microscope by same surgeon. The left lateral thigh was operated after shaving and preparing the skin with 10% povidone iodine. The sciatic nerve was exposed by opening the fascial plane between the gluteal and femoral musculature via a longitudinal incision (2–3 cm). All surgical procedures were carried out under ketamine hydrochloride (75 mg /kg) and Xylazine hydrochloride (5 mg/kg) anesthetic solutions, the sciatic nerve of such 30 rats was exposed at mid-thigh level and either crushed for 5 minutes with a pair of hemostatic forceps (9–10 mm size). Subsequently, the muscles and skin were separately sutured by 4/0 catgut thread and allowed to breathe room air. The surgery was followed by the animals’ special care until recovery.

In both group animals (the control and experimental), the left sciatic nerve had been crushed before the treatment was started and then sutured. The animals were anaesthetized with IP injection of sodium thiopenthal after 21 and 42 days. The left and right dorsal root ganglia-L5 and sections from distal parts of the right (non-operated) and left (operated) sciatic nerves were collected, fixed, and prepared for light microscopic examination. A 10 mm-long sample of the right sciatic nerve segment was removed without any injury, fixed, and prepared for histopathological examination. Tissue fragments were fixed in 10% neutral buffered formalin solution (for 72 hours), upon stability embedded in paraffin, sectioned at 5 μm thickness and stained with hematoxylin and eosin (H&E).

To determine the total number of neurons in the spinal dorsal root node, the researchers used series of cross-sectional counting method. In this method, through examination of each neuronal population the sensory neurons, one of every 5 or 10 sections, were counted and the total cells were multiplied by 5 or 10, respectively to give an estimate of total cell numbers and neurons, containing clear nuclear or nucleus were counted. Finally, the total number of neurons in the dorsal root node was compared to that of different groups. The neuronal counting method was explained by Clarke [29]. Briefly, the left and right L5 DRG were removed and post-fixed in 4% paraformaldehyde then 30% sucrose, both at 4°C for 24 h. the ganglia were blocked in tissue freezing medium and stored at −80°C. Each entire ganglion was cut into serial 15-μm cryosections and 1 from 4 sections mounted onto gelatin-coated glass slides and dried overnight. Neuron counts were performed using light microscopy. By a camera (DP11 camera) mounted on top of the microscope, images from the sections were prepared at magnifications of ×100, ×400, and ×1000, normal and clear neuronal nuclei or nucleus were counted. Neuron loss was calculated by subtracting the number of neurons in ipsilateral ganglion from that in their contralateral controls. Loss was then expressed as a percentage of the neuron count in the control ganglia.

The data were expressed as mean ± standard deviation (SD), and analyzed by repeated measures of variance. In order to comparing number of counted neurons between different groups a one-way ANOVA test and to evaluate time interventions and drug dosage, Duncan test were used. Experimental results were considered to be significantly different from control values with p-value set at.05 (SPSS).