Abstracts

INTRODUCTION

Ischemia is defined as partial or complete oxygen (O₂) deprivation in tissues due to reduced or completely interrupted blood flow. In ischemia, the synthesis of high-energy phosphates, such as ATP, is decreased in cells due to interruption of the O₂ flow into the tissue (JENNINGS & REIMER, 1991; REITER, 1995REITER, R. J. Oxidative processes and antioxidative defense mechanisms in the aging brain. The FASEB Journal, Rockville Pike, v.9, p.526-533, 1995. Available from: <http://www.fasebj.org/content/9/7/526.abstract>.
http://www.fasebj.org/content/9/7/526.ab... ). The decrease in ATP leads to inhibition of the Na⁺, K⁺ ATPase pump in the cell membrane and an increase in intracellular Na⁺ and Ca²⁺ concentrations (GREEN et al., 1989GREEN, C.J. et al. The importance of iron, calcium and free radicals in reperfusion injury: an overview of studies in ischaemic rabbit kidneys. Free radical research communications, Tokyo, v.7, p.255-264, 1989. Available from: <http://www.ncbi.nlm.nih.gov/pubmed/2684800>.
http://www.ncbi.nlm.nih.gov/pubmed/26848... ). Increased intracellular Ca²⁺ concentrations are reported to be cytotoxic (ORRENIUS et al., 1992ORRENIUS, S. et al. Calcium ions and oxidative cell injury. Annals of Neurology, Wiley-Blackwell, v.32, p.33-42, 1992. Available from: <http://onlinelibrary.wiley.com/doi/10.1002/ana.410320708/pdf>.
http://onlinelibrary.wiley.com/doi/10.10... ). ATP, adenosine mono-phosphate (AMP), adenosine, inosine and hypoxanthine are produced from ATP, and ATP utilisation continues during the ischemia period. Furthermore, xanthine dehydrogenase (XD) is converted to xanthine oxidase (XO) in this period. In healthy tissues, hypoxanthine is metabolised by XD, whereas it is metabolised by XO in ischemic tissue (PARKS et al., 1988PARKS, D.A. et al. Conversion of xanthine dehydrogenase to oxidase in ischemic rat intestine: a reevaluation. American Journal of Physiology, Rockville Pike, v.254, p.768-774, 1988. Available from: <http://ajpgi.physiology.org/content/254/5/G768>.
http://ajpgi.physiology.org/content/254/... ). Toxic O₂ radicals are not formed in healthy tissues because nicotinamide dinucleotide is used in the metabolism of hypoxanthine by XD. Toxic O₂ radicals are produced as intermediates in ischemic tissues because O₂ is used in the metabolism of hypoxanthine by XO (GRACE, 1994GRACE, P. A. Ischaemia-reperfusion injury. British Journal of Surgery, Glasgow, v.81, p.637-647, 1994. Available from: <http://onlinelibrary.wiley.com/doi/10.1002/bjs.1800810504/full DOI: 10.1002/bjs.1800810504>.
http://onlinelibrary.wiley.com/doi/10.10... ; PARKS et al., 1988PARKS, D.A. et al. Conversion of xanthine dehydrogenase to oxidase in ischemic rat intestine: a reevaluation. American Journal of Physiology, Rockville Pike, v.254, p.768-774, 1988. Available from: <http://ajpgi.physiology.org/content/254/5/G768>.
http://ajpgi.physiology.org/content/254/... ). Hypoxanthine cannot be metabolised by XO unless reperfusion occurs in ischemic tissue. As is known, the emptying of cellular energy stores may lead to cell death in long-lasting ischemia (PARKS et al., 1988PARKS, D.A. et al. Conversion of xanthine dehydrogenase to oxidase in ischemic rat intestine: a reevaluation. American Journal of Physiology, Rockville Pike, v.254, p.768-774, 1988. Available from: <http://ajpgi.physiology.org/content/254/5/G768>.
http://ajpgi.physiology.org/content/254/... ; ZIMMERMAN & GRANGER, 1992ZIMMERMAN, B.J.; GRANGER, D.N. Reperfusion injury. Surgical Clinics of North America, Canada, v.72, p.65-83, 1992. Available from: <http://www.ncbi.nlm.nih.gov/pubmed/1731390>.
http://www.ncbi.nlm.nih.gov/pubmed/17313... ). Therefore, the intervention in ischemic conditions has always been adequate perfusion of the tissue. During reperfusion, XO produced during ischemia converts hypoxanthine to xanthine using locally available O₂, leading to excessive free O₂ radical production and a decrease in antioxidant defence mechanisms (LINDSAY et al., 1990LINDSAY, T.F. et al. The effect of ischemia/reperfusion on adenine nucleotide metabolism and xanthine oxidase production in skeletal muscle. Journal of Vascular Surgery, Chicago, v.12, p.8-15, 1990. Available from: <http://www.sciencedirect.com/science/article/pii/074152149090360M>.
http://www.sciencedirect.com/science/art... ; LI & JACKSON, 2002LI, C.; JACKSON, R.M. Reactive species mechanisms of cellular hypoxia-reoxygenation injury. American Journal of Physiology - Cell Physiology, Rockville Pike, v.282, p.227-241, 2002. Available from: <http://ajpcell.physiology.org/content/282/2/C227.full-text.pdf+html>.
http://ajpcell.physiology.org/content/28... ). Previous studies showed that XO, the production of which increases during ischemia due to ATP deficiency, is an essential component in the mechanism of reperfusion injury. This indicates that ATP administration may be beneficial for the prevention of ischemia/reperfusion (I/R) injury.

Thus far, no studies have investigated the potentially protective effect of exogenous administration of ATP on I/R-induced ovarian injury in rats. Therefore, the aim of the present study was to investigate the effect of exogenous administration of ATP prior to experimentally induced ischemia and I/R of the rat ovary on biochemical variables and histopathological parameters.

MATERIAL AND METHODS

Animals

A total of 42 female adult Albino Wistar rats weighing between 220-235g were used for the experiment. The rats were obtained from Ataturk University Medical Experiments Research and Training Center (Erzurum, Turkey). The protocols and the procedures were approved by the local Animal Experimentation Ethics Committee (Date: 24. 04. 2012, meeting no: B.30.2.ATA.0.01.02/1845).

Chemical substances

Thiopental sodium was provided by IE Ulagay-Turkey and ATP was supplied by Zdorove Narodu Ukraine.

General procedure

The animals were allocated to 7 groups as Ovarian Ischemia (OI), Ovarian Ischemia/Reperfusion (OIR), 2mg kg^-1 ATP + Ovarian Ischemia (AOI-2), 4mg kg^-1 ATP + Ovarian Ischemia (AOI-4), 2mg kg^-1 ATP+ Ovarian Ischemia/Reperfusion (AOIR-2), 4mg kg^-1 ATP+ Ovarian Ischemia/Reperfusion (AOIR-4), and Control Group (Sham Operated- Healthy Control Group (CG). Surgical procedures were performed under sterile conditions in a suitable laboratory environment by administering 25mg kg^-1 intraperitoneal (IP) thiopental sodium anesthesia.

Surgical and pharmacological procedures

ATP was injected into AOI-2, AOI-4, AOIR-2 and AOIR-4 groups via the intraperitoneal route 1h before anaesthesia. A 3h ischemia period was then simulated through vascular clamping to the lower part of the right ovaries of rats assigned to OI, OIR, AOI-2, AOI-4, AOIR-2 and AOIR-4 groups. At the end of this period, the ovaries of the rats in the OI, AOI-2, AOI-4 groups were removed. Reperfusion was provided for 2h by removing the vascular clamp in the OIR, AOIR-2 and AOIR-4 groups. The ovaries of the rats in the OIR, AOIR-2 and AOIR-4 groups were removed. Histopathological and biochemical analyses were performed subsequently in all the samples (KURT et al., 2013KURT, A. et al. An investigation about the inhibition of acut ischemia / reperfusion damage by dexmedetomidine in rat ovarian tissue. Gynecological Endocrinology, London, v.29, p.222-225, 2013. Available from: <http://informahealthcare.com/doi/abs/10.3109/09513590.2012.665104>.
http://informahealthcare.com/doi/abs/10.... ). A 2-2.5cm long vertical incision was made in the lower abdomen of each rat to reach the ovaries. Ischemia was not performed in the ovaries of the rats in CG. The ovarian tissue samples were collected from all the experimental groups, and the assay was conducted simultaneously.

Biochemical procedures

Biochemical analysis of ovarian tissue

The homogenates were prepared to measure the enzymatic activity in the ovarian tissues. The XO, malondialdehyde (MDA), myeloperoxidase (MPO) and total glutathione (tGSH) enzyme activities in the supernatants obtained from these homogenates were determined using established methods reported in the literature.

Determination of xanthine oxidase (XO) activity

The XO activity was measured spectrophotometrically by the formation of uric acid from xanthine through the increase in absorbance at 293nm. In this method, phosphate buffer with EDTA (pH 7.5) is used as the solvent that reaction takes place. A total of 50µl of the sample and 50µl of xanthine (4mM) were added to the phosphate buffer, and then the mixture was incubated for 30min at 37°. A total of 100% (w/v) of TCA was added to stop the reaction mixture. The mixture was centrifuged at 4500g for 20min. The increase in the absorbance of the supernatant was then measured at 293nm (ROWE et al., 1966).

Determination of malondialdehyde (MDA) activity

The concentrations of ovarian lipid peroxidation were determined by estimating MDA activity using the thiobarbituric acid test (OHKAWA et al., 1979OHKAWA, H. et al. Assay for lipid peroxides in animal tissues by thiobarbituric acid reaction. Analytical Biochemistry, Oxford, v.95, p.351-358, 1979. Available from: <http://www.sciencedirect.com/science/article/pii/0003269779907383>.
http://www.sciencedirect.com/science/art... ). The rat ovaries were promptly excised and rinsed with cold saline. The ovarian tissue, weighed and homogenised in 10ml of 100g l^-1 KCl. The homogenate (0.5ml) was added to a solution containing 0.2ml of 80g l^-1 sodium lauryl sulfate, 1.5ml of 200g l^-1 acetic acid, 1.5ml of 8g l^-1 2-thiobarbiturate and 0.3ml of distilled water. The mixture was incubated at 98°C for 1h. Upon cooling, 5ml of n-butanol:pyridine (15:l) were added. The mixture was vortexed for 1min and centrifuged for 30min at 4000rpm. The absorbance of the supernatant was measured at 532nm. The standard curve was obtained by using 1,1,3,3-tetramethoxypropane.

Determination of myeloperoxidase (MPO) activity

The activity of MPO in the total homogenate was measured according to the method of Wei and Frenkel, with some modifications (WEI & FRENKEL, 1991WEI, H.; FRENKEL, K. In vivo formation of oxidized DNA bases in tumor promoter-treated mouse skin. Cancer Research, Philadelphia, v.5, p.4443-4449, 1991. Available from:<http://cancerres.aacrjournals.org/content/51/16/4443.long>.
http://cancerres.aacrjournals.org/conten... ). The sample was weighed and homogenised in a 2ml of 50mM phosphate buffer containing 0.5% hexadexyltrimethyl ammonium bromide (HDTMAB) and centrifuged at 3500rpm for 60min at 4°C. The MPO activity in the supernatant was determined using 1,3ml 4-aminoantipyrine-2% phenol (25mM) solution. A total of 25mM 4-aminoantipyrine-2% phenol solution and 0.0005% 1.5ml H₂O₂ were added and equilibrated for 3-4min. After establishing the basal rate, 0.2ml of sample suspension was added and quickly mixed. Increases in the absorbance at 510nm were recorded at 0.1min intervals for 4min. The absorbance was measured at 412nm using a spectrophotometer.

Determination of total glutathione (tGSH)

The amount of tGSH in the total homogenate was measured according to the method of Sedlak and Lindsay with some modifications (SEDLAK & LINDSAY, 1968SEDLAK, J.; LINDSAY, R.H. Estimation of total, protein-bound, and nonprotein sulfhydryl groups in tissue with Ellman's reagent. Analytical Biochemistry, Oxford, v.25, p.192-205, 1968. Available from: <http://www.sciencedirect.com/science/article/pii/0003269768900924>.
http://www.sciencedirect.com/science/art... ). The sample was weighed and homogenised in 2ml of 50mM Tris-HCl buffer containing 20mM of EDTA and 0.2mM of sucrose at pH 7.5. The homogenate was immediately precipitated with 0.1ml of 25% trichloroacetic acid, and the precipitate was removed after centrifugation at 4200rpm for 40min at 4°C. The GSH level of the supernatant was then determined. A total of 1500µl of measurement buffer (200mMTris-HCl buffer containing 0.2mM of EDTA at pH 7.5), 500µl of supernatant, 100µl of 5,5-dithiobis (2-nitrobenzoic acid) (DTNB) (10mM) and 7900µl of methanol were added to a tube, vortexed and incubated for 30min at 37°C. DTNB was used as a chromogen, and it formed a yellow-coloured complex with SH groups. The absorbance was measured at 412nm using a spectrophotometer. The standard curve was obtained using reduced glutathione.

Histopathological procedures

The ovaries that were removed from the rats were fixed in 10% formalin solution, sections 4µm in thickness were obtained from the paraffin blocks obtained after the routine tissue follow-up process, and the sections were stained with hematoxylin&eosin (H&E) stain after deparaffinization and rehydration. All the sections were encoded and examined under light microscopy (Olympus CX 51, Tokyo, Japan).

Statistical analysis

All data were subjected to a one-way analysis of variance (ANOVA) using Statistical Package for the Social Sciences (SPSS) 18.0 software. Multiple comparisons were analysed using the Duncan's multiple range test. A P-value 0.05 was considered statistically significant. The results are presented as the mean  standard error of mean (SEM).

RESULTS

Biochemical results

As seen in table 1, XO activity in the ovarian tissue of the ischemia-induced OI group was significantly higher than in the OIR group (<0.0001). In addition, the levels of MDA and MPO in the OIR group in which XO activity was lower increased in comparison to the OI group, and the amount of tGSH significantly decreased (P<0.0001). ATP administered in 2 and 4mg kg^-1 doses significantly prevented increases in XO, MDA and MPO levels during ischemia and postischemia-induced reperfusion in ovarian tissue and decreases in tGSH. No significant change was observed in the MPO activity of the ischemic ovarian tissue.

Histopathological result

A normal histopathological appearance is observed in figure 1.1.A-B. A moderate dilation, congestion (arrow) and mild hemorrhage (star) were observed in the vessels of the ipsilateral ovarian stroma in the OI group (Figure 1.2A.) compared to a normal histopathological ovary in control group. High magnification assessment provide a better insight in figure 1.2B. In figure 1.3A, vasodilation and congestion (arrow), edema, permanent and severe hemorrhage (star) were observed in the low power field; in Figure. 1.3B, migration and adhesion of a large number of PMNLs (double arrow) to the endothelium were observed in the high power field in the OIR group.

A mild congestion (arrow) and mild stromal hemorrhage were observed in figure 1.4A for the AOI-2 group. High magnification assessment provide a better insight in figure 1.4B. In figure 1.5A., a near-normal histomorphological appearance was observed in the AOI-4 group. High magnification assessment provide a better insight in figure 1.5B.In the AOIR-2 group, moderate congestion, dilation (arrow), moderate stromal hemorrhage and edema (star) were observed in the low power field in figure. 1.6A, while migration and adhesion of PMNLs to the endothelium (arrow) were observed in figure. 1.6B. As seen in figure 2.7. mild hemorrhage (arrow) in the ovarian stroma, mild vascular congestion (star) and minimal edema were observed in the AOIR-4 group (Table 2). High magnification assessment provide a better insight in figure 1.7B.

DISCUSSION AND CONCLUSION

This study investigated the effect of ATP on biochemical and histopathological damage caused by I/R. The results of the biochemical tests demonstrated that XO activity in the ischemia-induced OI group was 1.6 times higher than in the OIR group. In the literature, it has been reported that the presence of higher XO activity in ischemic tissue is due to the conversion of the xanthine dehydrogenase enzyme into XO by a calcium-mediated protease catalyst in the ischemia mediator (GRACE, 1994GRACE, P. A. Ischaemia-reperfusion injury. British Journal of Surgery, Glasgow, v.81, p.637-647, 1994. Available from: <http://onlinelibrary.wiley.com/doi/10.1002/bjs.1800810504/full DOI: 10.1002/bjs.1800810504>.
http://onlinelibrary.wiley.com/doi/10.10... ). In addition, the reduced occurrence of XO activity in the OIR group in comparison to the OI group could possibly be attributed to the XO activity being consumed in the production of XO oxidant. ATP used in doses of 2 and 4mg kg^-1 in this study significantly decreased XO activity during the formation of ischemia and postischemia-induced reperfusion in the ovarian tissue. The oxidation of sulfhydryl groups within XD molecules of cells leads to the formation of XO (HARRISON, 2002HARRISON, R. Structure and function of xanthine oxidoreductase: where are we now? Free radical biology and medicine, local, v.33, p.774-797, 2002. Available from: <http://dx.doi.org/10.1016/S0891-5849(02)00956-5>.
http://dx.doi.org/10.1016/S0891-5849(02)... ). Thus, the decrease in the formation of XO in the ovarian tissue of the rat groups that received ATP exogenously may be due to antioxidant activity associated with the generation of ATP. Similarly, the levels of oxidants, such as MDA and MPO, in the ovarian tissue of the OIR group significantly increased in comparison to those in the OI group, and their tGSH levels decreased. Paller M.S. demonstrated that free radicals develop at a low rate during ischemia but that they are produced in greater numbers when re-oxygenation of the tissue by reperfusion takes place (PALLER, 1994). Another study also reported that while XO accumulates during the ischemia period, a large number of toxic radicals are produced by transforming hypoxanthine into xanthine using the O₂ introduced by reperfusion, (CARDEN & GRANGER, 2000CARDEN, D.L.; GRANGER, D.N. Phatophsiology of ischemia-reperfusion injury. Journal of Pathology, London, v.190, p.255-266, 2000. Available from: <http://onlinelibrary.wiley.com/doi/10.1002/(SICI)1096-9896(200002)190:3%3C255::AID-PATH526%3E3.0.CO;2-6/full>.
http://onlinelibrary.wiley.com/doi/10.10... ). In common with these studies, Ingec et al. reported that the amount of oxidant increased only in ischemia-induced ovarian tissue and that it was greatly intensified by reperfusion (INGEC et al. 2011). As is well-known, AMP produced by aerobic tissues in the aerobic tissues provides the energy required to maintain cell viability by being broken down into adenosine, inosine and hypoxanthine. In ischemia, the consumption of ATP increases, and its production decreases (JENNINGS & REIMER, 1991). This event leads to the depletion of energy stores and the inhibition of the Na+, K+-ATPase pump found in the cell membrane. ATPase pump inhibition causes an excessive increase in intracellular Na+ and Ca²+ ion concentrations and leads to cell damage (GREEN et al., 1989GREEN, C.J. et al. The importance of iron, calcium and free radicals in reperfusion injury: an overview of studies in ischaemic rabbit kidneys. Free radical research communications, Tokyo, v.7, p.255-264, 1989. Available from: <http://www.ncbi.nlm.nih.gov/pubmed/2684800>.
http://www.ncbi.nlm.nih.gov/pubmed/26848... ). The prevention of ischemia and reperfusion damage by the administration of ATP in the experiment coincides with the information reported in the literature.

The use of ATP in doses of 2 and 4mg kg^-1 significantly prevented the rise of MDA and the reduction of tGSH in ischemic ovarian tissue. At the same doses, ATP significantly suppressed the levels of MDA and MPO, both of which had increased as a result of reperfusion. Free O₂ radicals, which are known to mediate reperfusion, result in the release of toxic products, such as aldehydes and MDA, from lipids and stimulate oxidation in the cell membrane (GOULART et al., 2005GOULART, M. et al. Lipoperoxidation products and thiol antioxidants in chromium exposed workers. Mutagenesis, Oxford, v.20, p.311-315, 2005. Available from: <http://mutage.oxfordjournals.org/content/20/5/311.full.pdf+html>.
http://mutage.oxfordjournals.org/content... ). MDA, as the final product of lipid peroxidation, causes severe damage to the cell membrane and its intracellular structures (GOULART et al., 2005GOULART, M. et al. Lipoperoxidation products and thiol antioxidants in chromium exposed workers. Mutagenesis, Oxford, v.20, p.311-315, 2005. Available from: <http://mutage.oxfordjournals.org/content/20/5/311.full.pdf+html>.
http://mutage.oxfordjournals.org/content... ). The high level of MPO in reperfusion could possibly originate from the release of MPO by large numbers of polymorphonuclear nuclear leukocytes (PMNLs) in the blood entering the ischemic tissue during reperfusion (ZIMMERMAN & GRANGER, 1992ZIMMERMAN, B.J.; GRANGER, D.N. Reperfusion injury. Surgical Clinics of North America, Canada, v.72, p.65-83, 1992. Available from: <http://www.ncbi.nlm.nih.gov/pubmed/1731390>.
http://www.ncbi.nlm.nih.gov/pubmed/17313... ). PNLs convert molecular O₂ into superoxide and hydrogen peroxide. The hydrogen peroxide in the chloride ions is reduced to hypochlorous acid, a toxic and strong oxidant, via the MPO enzyme found in the azurophilic granules of neutrophils (ZIMMERMAN & GRANGER, 1992ZIMMERMAN, B.J.; GRANGER, D.N. Reperfusion injury. Surgical Clinics of North America, Canada, v.72, p.65-83, 1992. Available from: <http://www.ncbi.nlm.nih.gov/pubmed/1731390>.
http://www.ncbi.nlm.nih.gov/pubmed/17313... ). Studies have experimentally demonstrated that postischemia reperfusion leads to severe damage of other tissues, as well as the ovaries (BOREKCI et al., 2009BOREKCI, B. et al. The protective effect of dehydroepiandrosterone on ovarian tissues after torsion-detorsion ınjury: a stereological and histopathological study. Eurasian Journal of Medicine, Erzurum, v.41, p.22-27, 2009. Available from: <http://www.eajm.org/sayilar/180/buyuk/pdf_EAJM_154.pdf.>.
http://www.eajm.org/sayilar/180/buyuk/pd... ; COSKUN et al., 2011; TOK et al., 2012TOK, A. et al. Effect of mirtazapine on oxidative stress created in rat kidneys by ischemia-reperfusion. Renal Failure, London, v.34, p.103-110, 2012. Available from: <http://informahealthcare.com/doi/abs/10.3109/0886022X.2011.623499>.
http://informahealthcare.com/doi/abs/10.... ). Moreover, previous studies reported that levels of ATP and Na+-K+-ATPase are decreased in ischemic tissue (GABRYEL et al., 2012GABRYEL, B. et al. Neuronal autophagy in cerebral ischemia--a potential target for neuroprotective strategies? Pharmacological Reports, Poland, v.64, p.1-15, 2012. Available from: <http://www.if-pan.krakow.pl/pjp/pdf/2012/1_1.pdf>.
http://www.if-pan.krakow.pl/pjp/pdf/2012... ; SINGH et al., 2012). The biochemical results obtained in the present study coincide with the histopathological findings. In addition, the severity of the pathological findings, such as dilatation, congestion, haemorrhage, oedema and PNLs, increased in parallel with the rise in XO metabolism products. In conclusion, exogenously administered ATP prevented the increase of XO, MDA and MPO, all of which are known to be oxidant parameters in ovarian tissue in ischemia and postischemia-induced reperfusion. These results suggest that the use of ATP at the clinic would be helpful as a preventive agent of both ovarian ischemia and post ischemia reperfusion damage.

ACKNOWLEDGEMENTS

Authors do not have financial support.

REFERENCES

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