Stereological analysis of sciatic nerve in chickens following neonatal pinealectomy: an experimental study

Mehmet Turgut; Süleyman Kaplan; Burçin Zeynep Ünal; Mehmet Bozkurt; Sinan Yürüker; Çigdem Yenisey; Bünyamin Sahin; Yigit Uyanıkgil; Meral Baka

doi:10.1186/1749-7221-5-10

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J Brachial Plex Peripher Nerve Inj 2010; 05(01): e50-e56
DOI: 10.1186/1749-7221-5-10

Research article

Turgut et al; licensee BioMed Central Ltd.

Stereological analysis of sciatic nerve in chickens following neonatal pinealectomy: an experimental study^[*]

Mehmet Turgut

¹Department of Neurosurgery, Adnan Menderes University School of Medicine, Aydın, Turkey

,

Süleyman Kaplan

³Department of Histology & Embryology, Ondokuz Mayıs University School of Medicine, Samsun, Turkey

,

Burçin Zeynep Ünal

⁵Ondokuz Mayıs University School of Dentistry, Samsun, Turkey

,

Mehmet Bozkurt

⁶Institute of Agricultural Research of Erbeyli, Aydın, Turkey

,

Sinan Yürüker

⁷Department of Histology and Embryology, Hacettepe University School of Medicine, Ankara, Turkey

,

Çigdem Yenisey

² Department of Biochemistry, Adnan Menderes University School of Medicine, Aydın, Turkey

,

Bünyamin Sahin

⁴Department of Anatomy, Ondokuz Mayıs University School of Medicine, Samsun, Turkey

,

Yigit Uyanıkgil

⁸Department of Histology and Embryology, Ege University School of Medicine, İzmir, Turkey

,

Meral Baka

⁸Department of Histology and Embryology, Ege University School of Medicine, İzmir, Turkey

› Author Affiliations
Subject Editor:

Further Information

Corresponding author

Mehmet Turgut

Email: drmturgut@yahoo.com

Publication History

18 November 2009

21 April 2010

Publication Date:
19 September 2014 (online)

Also available at

Abstract
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Background
Materials and methods

Reagents

Animals

Neonatal pinealectomy

Histology

Stereological analysis

Biochemical measurement

Data analysis

Results
Discussion
Conclusion
Abbreviations
Competing interests
Authors’ contributions
References

Abstract

Background Although the injury to the peripheral nervous system is a common clinical problem, understanding of the role of melatonin in nerve degeneration and regeneration is incomplete.

Methods The current study investigated the effects of neonatal pinealectomy on the sciatic nerve microarchitecture in the chicken. The chickens were divided into two equal groups: unpinealectomized controls and pinealectomized chickens. At the end of the study, biochemical examination of 10 sciatic nerve samples from both groups was performed and a quantitative stereological evaluation of 10 animals in each group was performed. The results were compared using Mann-Whitney test.

Results In this study, the results of axon number and thickness of the myelin sheath of a nerve fiber in newly hatched pinealectomy group were higher than those in control group. Similarly, surgical pinealectomy group had significantly larger axonal cross-sectional area than the control group (p < 0.05). In addition, the average hydroxyproline content of the nerve tissue in neonatal pinealectomy group was higher than those found in control group. Our results suggest that melatonin may play a role on the morphologic features of the peripheral nerve tissue and that melatonin deficiency might be a pathophysiological mechanism in some degenerative diseases of peripheral nerves. The changes demonstrated by quantitative morphometric methods and biochemical analysis has been interpreted as a reflection of the effects of melatonin upon nerve tissue.

Conclusion In the light of these results from present animal study, changes in sciatic nerve morphometry may be indicative of neuroprotective feature of melatonin, but this suggestion need to be validated in the human setting.

Background

Although the injury to the peripheral nervous system is a common clinical problem, a clear understanding of both morphological and pathophysiological alterations associated with this entity is incomplete [[1],[2],[3],[4]]. A basic understanding of specific peripheral nerve biology is critical for the process of nerve degeneration and regeneration. In the clinical setting, the ability to manipulate nerve biology at the cellular level provides a significant improvement in nerve recovery [[2],[5]]. In the last decade, some substances such as tacrolimus, an immunosuppressive agent, and alpha-lipoic acid have been shown to protect peripheral nerve from ischemic degeneration [[6],[7]]. However, controversy still exists regarding peripheral nerve injuries with potentially devastating results at the moment.

On the other hand, the pineal gland, a neuroendocrine transducer organ with neuronal input and endocrine output, produces the hormone of darkness, melatonin (N-acetyl-5-methoxytryptamine), shown in the peripheral nerve tissue [[8]]. It is well known that melatonin inhibits the process of peripheral nerve degeneration and has a neuroprotective action in a variety of pathological processes including ischemic injury, edema formation, and infarction in experimental studies [[3],[9],[10],[11],[12],[13],[14]]. Recently, it was reported that this protective effect has been linked with its inhibitory role on mitochondria via signaling [[15]]. Indeed, the growing knowledge about this substance is reflected in the steadily increasing number of publications. To our knowledge, however, there is no stereological study in the literature, which specifically addresses the effects of neonatal pinealectomy on peripheral nerve architecture.

This study was undertaken to investigate the effects of neonatal pinealectomy upon the ultrastructural features of peripheral nerve in the chickens, and thus to provide a better understanding of the role of melatonin in nerve degeneration and regeneration.

Materials and methods

Reagents

Chloramine-T, p-dimetylaminobenzaldehyde, and L-hydroxyproline as standard were purchased from Sigma Chemical Co. (St. Louis, USA). Sodium acetate, citric acid, perchloric acid, n-propanol, sodium hydroxide, and acetic acid were purchased from Merck Chemical Co. (Darmstadt, Germany).

Animals

The ethical committee of Ege University School of Medicine approved all experimental procedures employed in the study. Experiments were performed using 30 newly hatched Hybro Broiler chickens weighing 40-70 g each. Three day-old chicks were obtained from a local hatchery (Institute of Agricultural Research of Erbeyli). They were kept in individual cages under constant laboratory conditions (20 to 22°C room temperature and a 12-hour light/dark cycle). They were given free access to commercial diet and water ad libitum. The chickens were divided randomly into two groups: unpinealectomized control group (n = 15) and surgical pinealectomy group (n = 15) on the day of experiment.

Neonatal pinealectomy

Neonatal pinealectomy was done under the general anesthesia of intraperitoneal sodium pentobarbital (Nembutal sodium^®, Abbott Laboratories Comp., İstanbul-Türkiye, 40 mg/kg), as described previously [[16]]. In brief, after shaving the part of under surgical intervention was disinfected using polyvidon iyod. In aseptic conditions, a 2-cm midline incision was made through the skin above the superior sagittal sinus and was extended posteriorly to just below the confluence of sinuses and a skull flap was raised with a scalpel. Then the pineal gland, which lies just beneath the dura mater and between two cerebral hemispheres and cerebellum, was taken out by using a microsurgical forceps after cutting from its pedicle. The skin was sutured with vicryl 6/0.

Histology

At the end of the experiment (8 weeks later), 10 animals from each experimental group were randomly selected and sacrificed for histopathological evaluation. In each animal, right sciatic nerve was exposed and a nerve segment of 10 mm in length was carefully removed. Then, the excised segments were cut into blocks of equal length followed by fixation with 2% glutaraldehyde buffered in cacodylate 0.1 M and 2% paraformaldehyde solution (pH 7.4) for 24 hours after fixation. After fixation tissues were rinsed in cacodylate buffer (pH 7.4) twice. Following this step, specimens were postfixed in 1% osmium tetroxide for 2 hours, dehydrated in an ascending alcohol series and took into propylene oxide two times. After this, the tissues were embedded in epoxy resin. Following hardening, serial semi-thin sections of 1-μm thickness were cut by using a LKB 11800 ultramicrotome (Bromma, Sweden). The resin was removed from epoxy embedded tissue sections [[17],[18]]. Then, the sections were stained with 1% toluidine blue [[19]] and examined under light microscopy.

Stereological analysis

Stereological analyses of sciatic nerves by an observer blinded to the groups were done according to principles described by Larsen [[20]] and Geuna et al. [[21]]. The sampled sections, 1-μm-thickness, were examined with a modified light microscope, which has a counting frame in the eyepiece, and dial indicators attached to the stage of microscopes [[22]]. To obtain an estimation of total axon number in an unbiased manner from nerve cross-section, the unbiased counting frame with 900 μm² in area was utilized [[23]]. The section of each nerve was examined in a systematic uniform random manner ([Fig. 1]) and nerve fibers were counted if they were in a countable position (Figs. [2] and [3A]). Area sampling of nerve section was done with a 100 × 100-μm successive, systemic-random steps. This ensures that all locations within a nerve cross section are equally represented and that all axon profiles are sampled with an equal probability regardless of shape, size, orientation and location [[24],[25]]. Counting of axons was done with an objective (100× oil objective; NA = 1.25) and total magnification was 1000 that allowed accurate recognition of myelinated nerve fibers. Total axon number in each nerve was estimated by multiplying counted axon numbers with reverse of the area fraction [[24]].

Figure 1 The point counting method for estimation of the cross section area of sciatic nerve. The profile area of nerve can be estimated by placing a tested point grid on the profile of nerve. The number of points, P, that hits the profile area multiplied by the area associated with each grid point, a(p), is an unbiased estimate of cross section area of nerve. A = a (p)·ΣP. The same approach can be also used for estimation of cross section area of axon.

Figure 2 The counting principle of the axon number in nerve cross-section. The section of nerve is sampled in a systematic random manner to gain an unbiased estimation of total axon number in a nerve. Each square represents a sampling area. An unbiased counting frame is seen in the center of this area. The axons are counted if nerve fiber being in the unbiased counting frame (f) in each sampling area. Estimates of the total number of myelinated axons are calculated as the product of the number of axons counted in a known fraction and multiplied by the inverse sampling fraction. In this study, upper and right lines of unbiased counting frames represent the inclusion lines (dot lines) and the lower and left lines including the extensions are the exclusion lines. Any profile of myelinated nerve fiber section hitting the exclusion lines is excluded and profile of nerve fiber hitting the inclusion lines and located inside the frame are counted.

Figure 3 (A) A micrograph of nerve cross-section with an unbiased counting frame superimposed on it. Axons within the unbiased counting frame that are in countable position were marked with stars. Toluidine blue staining, scale bar = 10 μm. (B) The same micrograph with the point counting grid superimposed on it. If an axon is crossed with the right corner of the unbiased counting frame during systematic random sampling, cross section areas of this axon was estimated by means of counting the test points of grid coincide into the axon.

After the counting of the axons in a systematic random manner, myelin thickness and axon cross-sectional area (CSA) were measured at a stereology workstation, consisting of a modified light microscope (Leica, Germany), a motorized specimen stage for automatic sampling (Prior, Rockland, MA, USA), an electronic microcator (Heidenhain, Traunreut, Germany), a CCD colour video camera (JVC, Tokyo, Japan), a PC with frame grabber board (type FlashPoint 3D, Integral Technologies, Indianapolis, IN, USA) and stereology software (CAST; Olympus, Glostrup, Denmark) and a 17” PC monitor (Hyundai, South Korea) ([Fig. 3B]). Myelin thickness of an axon was measured with length measurement of the software if it crossed with the right corner of the unbiased counting frame. After measuring myelin thickness, measurement values of CSA for both axon and nerve were obtained by superimposing of a test point grid [a(p) = 11,6 μm²] on that sampled axons (100× Leica, Plan Apo oil objective; NA = 1.40; 5107×). Coefficient of error (CE) and coefficient of variation (CV) for stereological analysis were estimated [[26],[27],[28]].

Biochemical measurement

In each animal, the left sciatic nerve was isolated and removed for biochemical analysis. Samples of the sciatic nerve were stored at -85°C until the analysis for the collagen content. The amino acid hydroxyproline was determined by a method of Reddy and Enwemeka [[29]]. One hundred μl 2N NaOH were added each of tissue samples (approximately 20 mg), and then samples were hydrolyzed by autoclaving at 120°C for 30 minutes. Then, hydrolyzed samples were mixed with a buffered chloramine-T reagent, and the oxidation was allowed to proceed for 25 minutes at room temperature. The chromophore was then developed with the addition of Erlich’s reagent, and the absorbance of reddish purple complex was measured at 550 nm using a spectrophotometer. Absorbance values were plotted against the concentration of standard hydroxyproline, and the presence of hydroxyproline is unknown tissue extracts was determined from standard curve. Based on an assumption that 12.5% of collagen is hydroxyproline [[30],[31]], sciatic nerve total collagen content were measured and expressed as μg hydroxyproline/mg of wet tissue weight.

Data analysis

All data are presented as the mean ± standard error of measurements (SEM). All statistical procedures were performed using SPSS statistical software package program (9.0, SPSS Inc, Chicago, IL, USA). The statistical analysis of the data was carried out by using Mann-Whitney U-test. A p-value of less than 0.05 was considered significant.

Results

All chickens showed no evidence of gross neurophysiologic deficit and no wound infections were noted in the postoperative period. At the end of the experiment, histological examination of the brains of the animals in neonatal pinealectomy group revealed that the pineal gland had been removed at surgery and no extraneous tissue had been left behind or had regenerated.

Histological examination of the specimens revealed an appearance of normal sciatic nerve in control group, while the presence of partly myelin sheath degeneration, increasing of vacuolization in the myelin and elevation of axon diameter in neonatal pinealectomy group ([Fig. 4]). Quantitative stereological evaluations for axon numbers, thickness of the myelin sheath of a nerve fiber, and CSA of both axon and nerve were performed in the sciatic nerve segment in both experimental groups. The results of axon numbers in both groups were summarized in [Table 1]. The axon number in surgical pinealectomy group was higher than the unpinealectomized control group, although a significant difference was not observed between groups (p < 0.05). The results of the mean myelin sheath thickness of a nerve fiber in all groups were summarized in [Table 2]. The mean myelin sheath thickness was increased in neonatal pinealectomy group as compared with unpinealectomized control group (1.821 ± 0.136 μm versus 1.715 ± 0.110 μm). However, no significant differences were found between groups (p > 0.05). In the comparison of axonal CSA, a significant difference was found between surgical pinealectomy and control group (p < 0.05) ([Table 3]). Thus, neonatal pinealectomy procedure resulted in an increased axon number, thickness of the myelin sheath, and CSA of the axon. However, there was no significant difference in the means of CSA of the nerve for both groups (p > 0.05) ([Table 4]).

Table 1
Comparison of the mean axon numbers for both groups of chickens at 8 weeks after neonatal pinealectomy.
Groups	Number of axons*
Surgical pinealectomy group (n = 10)	6811.444 ± 249.367
Unpinealectomized control group (n = 10)	6168.000 ± 219.034
p value	0.07