Int J Pharm Pharm Sci, Vol 8, Issue 6, 253-259Original Article

THE THERAPEUTIC AND NEUROPROTECTIVE EFFECTS OF GREEN TEA IN A RAT MODEL OF TERLIPRESSIN-INDUCED CHRONIC HYPONATREMIA

REHAB HEGAZY¹*, RASHA MOSTAFA¹, REHAM EL-MELIGY²

¹Pharmacology Department, Medical Division, National Research Centre, Giza, Egypt, ²Medicinal and Aromatic Plants Department, Desert Research Center, Cairo, Egypt
Email: rehab_hegazy@hotmail.com  

 Received: 06 Mar 2016 Revised and Accepted: 20 Apr 2016

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ABSTRACT

Objective: Hyponatremia (HN) is associated with mortality and morbidity risks due to the development of hyponatremic encephalopathy. Its rapid correction also carries a high risk of development of the serious cerebral disorder. This study investigated the possible therapeutic and neuroprotective effects of the green tea (GT) extract against HN and its complications in rats and compared those effects with the outcome of the rapid correction of chronic HN using hypertonic saline (HtNaCl).

Methods: Chronic HN was induced using terlipressin (TP; 0.2 mg/kg, s. c) and 2.5% d-glucose solution (equivalent to 5% initial bw/day, i. p) for 3 d. A stabilizing dose of TP (0.1 mg/kg) was used for the following 3 d, along with administration of either saline, GT (600 mg/kg/day, p. o), or HtNaCl (15 ml/kg/day, i. p). Serum sodium level, locomotor activity, pain reflex, and brain contents of iNOS and NO were assessed, together with a histopathological examination of brain tissues.

Results: TP-induced profound chronic HN that was corrected with administration of GT and HtNaCl. In a GT-treated group, correction of HN was coupled with improvement of TP-induced alteration of locomotor activity and brain histopathological picture. Elevation of brain iNOS and NO contents, along with detection of focal cellular necrosis and gliovascular proliferation changes in the HtNaCl-treated group indicated neuro pathological complications are accompanying the correction of HN with HtNaCl; a result that was not found in the GT-treated group.

Conclusion: Our findings revealed that GT corrected HN induced by TP in rats, and protected against the neuropathological features that characterized hyponatremic encephalopathy and accompanied with its rapid correction.

Keywords: Green tea, Terlipressin, Hyponatremia, Hyponatremic encephalopathy, iNOS, Rat

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© 2016 The Authors. Published by Innovare Academic Sciences Pvt Ltd. This is an open access article under the CC BY license (http://creativecommons.org/licenses/by/4.0/)

INTRODUCTION

Hyponatremia (HN) is defined as a decrease in serum sodium concentration to a level below 136 mmol/l [1]. It is the most common electrolyte disorder occurring in 15–30% of hospitalized patients [2]. Etiologies of HN include renal and extra-renal loss of sodium with water retention as in cases of mineralocorticoid deficiency, autoimmune diseases, adrenal hemorrhage, muscle trauma, burns, sweat losses, and gastrointestinal losses due to vomiting and diarrhea [3]. Moreover, various pharmacological agents are known to be associated with induction of HN, including, narcotics, sedatives, analgesics, hypoglycaemic agents, anti-neoplastic drugs, and antidepressants [4, 5]. HN can also arise in a variety of diseases such as congestive heart failure, liver cirrhosis, and renal failure whether acute or chronic [6]. The most common cases of HN include exercise-associated HN, particularly in athletes who participate in endurance events [7], ecstasy-associated HN [8], and postoperative HN [9].

HN is physiologically significant when it indicates a state of extracellular hypo-osmolality and a tendency for free water to shift from the vascular space to the intracellular space. However, although cellular edema is well tolerated by most tissues, it is not tolerated in the brain as its maximum swelling is limited to 8% secondary to the presence of the rigid calvarium [3]. In severe HN, this cytotoxic cerebral edema results in the development of hyponatremic encephalopathy, which is a medical emergency that can be lethal [10]. The rate of development of HN plays a critical role in its pathophysiology and subsequent treatment [11]. In acute HN that is developed rapidly over a period of hours (<48 h), a more severe degree of cerebral edema for a given serum sodium level results. Thus, it occurs with alarming hyponatremicencephalopathy findings, and the primary cause of morbidity and death is brainstem herniation and mechanical compression of vital midbrain structures [12]. In chronic HN, when serum sodium concentration falls slowly over a period of several days or weeks (≥ 48 h), a slower process of adaptation then occurs in which the brain cells extrude sodium and potassium as well as organic solutes including phosphocreatine, myoinositol, and amino acids, such as glutamine and taurine, from their cytoplasm to the extracellular space [13]. Compensatory extrusion of solutes allows intracellular osmolality to be equal to plasma osmolality and, in turn, reduces the flow of free water into the intracellular space [14]. Therefore, brain swelling is minimized with more modest symptoms and cases, almost, never die from brain herniation [14]. However, the principal causes of morbidity and death in chronic HN are status epilepticus, when chronic HN reaches levels of 110 mmol/l or less, and osmotic demyelination syndrome (ODS), which occurs in association with rapid correction of chronic HN [11]. ODS is characterized by focal destruction of myelin sheaths that cover axons in the brainstem, in the pontine and extrapontine areas, associated with serious neurologic sequelae [15]. Several lines of evidence have linked the pathogenesis of myelinolysis to the slow reuptake of organic osmolytes by the brain. [16, 17].

Treatment of HN consists of free water restriction and correction of the underlying condition. The daily fluid intake must be restricted to less than the urine output volume and the insensible losses of water during 24 h in order to cause a negative water balance and increase serum sodium concentration [3]. Some cases of chronic HN do not tolerate or comply with this degree of daily fluid restriction. In these cases, the use of diuretics that increase electrolyte-free water excretion may be added to the treatment protocol [18-20].

Green tea (GT) is a popular worldwide beverage that has been shown to possess several pharmacological activities [21-24]. It has been reported for its diuretic [25-28], anti-inflammatory [29], antiarthritic [30], antibacterial [31], antiviral [32], antiproliferative [33], antioxidant [34,35], neuroprotective [36, 37], and cholesterol-lowering effects [23, 38, 39]. Moreover, consuming green tea has been found to protect against obesity [40, 41], cancer [42, 43], and cardiovascular diseases [44-46]. The chemical composition of green tea is complex; it contains xanthic bases (caffeine and theophylline), polyphenols commonly known as catechins, pigments, volatile compounds, proteins, amino acids, carbohydrates, vitamins (B, C, E), minerals, trace elements, and trace amounts of lipids and sterols [23, 24, 45]. Caffeine and theophylline account for the diuretic effect of GT [25-28]. It has been demonstrated that caffeine could increase urine production in patients with congestive heart failure and edema; however, theophylline has been found to induce even higher diuretic effect than caffeine [47, 48]. On the other hand, GT polyphenols are responsible for the neuroprotective and the antioxidant properties of GT. The present study aimed at testing the possible protective effects of GT extract against chronic HN and hyponatremic encephalopathy induced in rats using terlipressin (triglycyl–lysine vasopressin; TP), which is a long-acting analog of the antidiuretic hormone, vasopressin (VP) [49]. Moreover, the study compared the effects of GT with those resulted from the rapid correction of chronic HN using hypertonic saline (HtNaCl).

MATERIALS AND METHODS

Animals

Adult male albino Wister rats, weighing 180–200 g, was utilized in the present study. Standard food pellets and tap water were supplied ad libitum unless otherwise stated. Animals and food pellets were obtained from the animal house colony of the National Research Center (NRC, Egypt). Ethical considerations in handling laboratory animals that stated by NRC were followed throughout the study period.

Drugs

TP vials (Glypressin^®; Ferring Pharmaceuticals, Germany) were used in the current study. GT water extract, in the form of powder, was obtained from Technomate for Chemicals and Pharmaceuticals (Egypt), and was used orally in a dose of 600 mg/kg/day [35]. All other chemicals were of the highest available commercial grade.

Experimental design

Chronic HN was induced in rats according to the method established in our previous study with colleagues [49]. The animals were randomly allocated into four groups; each group consisted of 10 rats. During the induction phase of this experiment (days 1–3), rats of the first group received s. c injections of saline and served as the normal group. In the remaining three groups, chronic HN was induced by injections of TP (0.2 mg/kg/day, s. c) and 2.5% d-glucose solution (equivalent to 5% initial bw/day, i. p) for 3 successive days. Rats of TP-induced HN group had free access to distilled water only during this phase of experiment with no access to food.

In the 2^nd phase of the experiment (days 4–6), animals of all groups had free access to food and tap water. In this phase, the normal group received saline; the other three groups received TP (0.1 mg/kg/day, s. c.) as a stabilizing dose. Group 2 served as the HN-control group; groups 3 and 4 were treated with GT (600 mg/kg/day, p. o.) and 1 M sodium chloride solution (hypertonic saline, HtNaCl; 15 ml/kg/day, i. p.), respectively.

Estimation of serum sodium level

Blood samples were withdrawn from the retro-orbital plexus of each animal, under light diethyl ether anesthesia, following induction phase (on day 4), and one hour following the last drug administration in the treatment phase (on day 6). The blood was allowed to coagulate and then centrifuged, using a cooling centrifuge (Sigma and laborzentrifugen, 2k15, Germany), at 3000 rpm for 20 min for serum separation. Serum sodium level was estimated using specific reagent kit (Stanbio Laboratory, USA).

Measurement of locomotor activity

On days 0, 4 and 6 of the experiment, locomotor activity was assessed by detecting rat movements using grid floor activity cage (Model no. 7430, Ugo-Basile, Italy). Interruptions of infrared beams were automatically detected during a 10 min test session. Beam interruption information was processed in the activity cage software to provide an index of horizontal movements [50, 51]. Change of the basal locomotor activity was calculated for each rat.

Evaluation of pain reflex

The delay in pain reactivity, as a neuronal reflex, was evaluated on days 0, 4 and 6 of the experiment using the hot-plate test (7280 Ugo Basile, Italy) according to the method described by Laviola and Alleva [52]. Change of the basal response to the nociceptive stimulus was calculated for each rat.

Tissue sampling and estimation of brain inducible nitric oxide synthase (iNOS) and nitric oxide (NO) contents

Directly after collecting the last blood sample in the experiment, rats were decapitated under light diethyl ether-anesthesia, and their brain was carefully isolated and dissected through the midline into two hemispheres. One brain hemisphere from each rat was immediately weighed and homogenized in ice-cold potassium chloride (1.15%; pH 7.4) to yield a 20% (w/v) tissue homogenate (using MPW–120 homogenizers, Med instruments, Poland). The homogenates were centrifuged using a cooling centrifuge (Sigma and laborzentrifugen, 2k15, Germany) at 4000 r. p. m for 10 min; the supernatant was used for biochemical estimation of brain content of iNOS, using iNOS ELISA kit (MyBioSource, USA), and NOx (nitrite and nitrate, stable metabolites of NO) utilizing an NOx concentration assay kit (Cayman chemical company, Germany).

Histopathological examination of brain tissues

The other brain hemisphere of each rat was removed and immediately placed in 10% formalin. Afterward, brains were sectioned coronally at six levels. Sections were stained with hematoxylin and eosin (H&E), and processed for light microscopy evaluation of neuronal density, edema, and inflammation.

Statistical analysis

All the values are presented as means±standard error of the means (SE). Comparisons between different groups were carried out using one-way analysis of variance (ANOVA) followed by Tukey’s multiple comparison post hoc tests. For behavioral parameters, square root transformed percent was calculated according to Jones et al. [53] then comparisons between different groups were carried out using the nonparametric one-way ANOVA followed by Dunn's multiple comparisons post hoc test. The difference was considered significant when p˂0.05. GraphPad prismsoftware (version 6) was used to carry out these statistical tests.

RESULTS

Serum sodium level

Subcutaneous injection of TP produced stable HN demonstrated by decreased serum sodium level to 109.85±4.8 and 112.08±5.3 mmol/l on days 4and 6, respectively. Treatment of rats with GT or HtNaCl corrected TP-induced HN (fig. 1).

Saline, rats, treated with saline and represented the normal group; TP, rats treated with terlipressin and served as a hyponatremia (HN)-model group; TP-GT, rats with TP-induced HN treated with green tea; TP-HtNaCl, rats with TP-induced HN treated with hypertonic saline.

^a Significantly different from the normal group at the corresponding day at p<0.05.

^bSignificantly different from TP group at the corresponding day at p<0.05.

Locomotor activity and Pain reflex

Induction of HN in rats using TP was coupled with a decrease in the basal locomotor activity that was observed on days 4 and 6 (table 1). A delay of the basal pain reflex was also observed following the induction phase (on day 4); however, no significant difference was observed in a TP-treated group on day 6 (table 2). Treatment of rats with GT improved that TP-induced decrease in locomotor activity; however, HtNaCl failed to do so (table 1). On the other hand, rats treated with GT showed a significant delay of the response to pain stimulus as compared to both normal and HN group (table 2).

Fig. 1: Effects of TP-induced HN, and the co-administration of GT and HtNaCl on serum sodium level in rats

Saline, rats treated with saline and represented the normal group; TP, rats treated with terlipressin and served as hyponatremia (HN)-model group; TP-GT, rats with TP-induced HN treated with green tea; TP-HtNaCl, rats with TP-induced HN treated with hypertonic saline.

^aSignificantly different from normal group at the corresponding day at p < 0.05., ^bSignificantly different from TP group at the corresponding day at p < 0.05.

Table 1: Effects of TP-induced HN, and the co-administration of GT and HtNaCl on the locomotor activity of rats

Groups	Locomotor activity
	Count/10 min.			Square-root-transformed % of basal activity
	Day 0	Day 4	Day 6	Day 4	Day 6
Saline	162.40±13.43	179.80±11.91	178.60±7.81	1.06b±0.04	1.06b±0.03
TP	118.60±25.24	55.20±16.70	80.40±15.36	0.69a±0.12	0.83a±0.02
TP-GT	161.20±26.84	96.00±21.19	155.60±25.08	0.78a±0.09	0.98b±0.01
TP-HtNaCl	123.40±10.09	73.80±14.35	70.20±8.50	0.76a±0.11	0.76a±0.08

Saline, rats treated with saline and represented the normal group; TP, rats treated with terlipressin and served as a hyponatremia (HN)-model group; TP-GT, rats with TP-induced HN treated with green tea; TP-HtNaCl, rats with TP-induced HN treated with hypertonic saline.

Data are presented as mean±SE., ^a Significantly different from the normal group at the corresponding day at p<0.05., ^bSignificantly different from TP group at the corresponding day at p<0.05.

Table 2: Effects of TP-induced HN, and the co-administration of GT and HtNaCl on the response of rats to the nociceptive stimulus

Groups	Delay of pain reflex
	Nociceptive response (sec)			Square-root-transformed % of basal response
	Day 0	Day 4	Day 6	Day 4	Day 6
Saline	38.25±3.71	27.72±3.05	29.02±2.62	0.84b±0.07	0.86±0.06
TP	24.30±4.25	31.06±3.58	26.56±3.38	1.20a±0.08	0.98±0.13
TP-GT	26.58±2.60	35.38±4.51	38.38±5.61	1.13a±0.05	1.21ab±0.10
TP-HtNaCl	33.25±2.36	39.30±4.18	34.18±3.33	1.06a±0.04	0.99±0.03

Saline, rats treated with saline and represented the normal group; TP, rats treated with terlipressin and served as a hyponatremia (HN)-model group; TP-GT, rats with TP-induced HN treated with green tea; TP-HtNaCl, rats with TP-induced HN treated with hypertonic saline.

Data are presented as mean±SE., ^a Significantly different from the normal group at the corresponding day at p<0.05., ^bSignificantly different from TP group at the corresponding day at p<0.05.

Fig. 2: Effects of TP-induced HN, and the co-administration of GT and HtNaCl on brain contents of iNOS and NOx in rats

Saline, rats treated with saline and represented the normal group; TP, rats treated with terlipressin and served as hyponatremia (HN)-model group; TP-GT, rats with TP-induced HN treated with green tea; TP-HtNaCl, rats with TP-induced HN treated with hypertonic saline., ^a Significantly different from normal group at p<0.05., ^bSignificantly different from TP group at p<0.05.

Brain iNOS and NO contents

Treatment of rats with TP to induce HN had no effect on the brain contents of iNOS and NOx. Similarly, administration of GT to TP-treated rats showed normal iNOS and NOxcontent; whereas, administration of HtNaCl increased brain iNOS and NOx content in rats with TP-induced HN (fig. 2).

Histopathological examination of brain tissues

The brain sections prepared from normal rats showed normal brain tissue with normal astrocytes and fibrillary background (fig. 3a), while those prepared from rats with TP-induced chronic HN indicated a marked glial brain edema (fig. 3b). Treatment of rats with GT markedly ameliorated the brain edema observed in rats with TP-induced chronic HN and restored the normal histological structures of brain tissues (fig. 3c). The brain sections prepared from rats with TP-induced chronic HN treated by HtNaCl revealed marked amelioration of brain edema; however, neuronal cell necrosis associated with congestion of cerebral blood vessel was detected (fig. 3d).

Fig. 3: Photomicrographs of brain sections prepared from (a) a normal rat, (b) a rat with TP-induced chronic HN, (c) a rat with TP-induced chronic HN treated by GT, and (d) a rat with TP-induced chronic HN treated by HtNaCl (H&E X 400)

(a) Showing normal brain tissue with normal astrocytes and fibrillary background. (b) Showing marked glial brain edema (arrow). (c) Showing marked amelioration of the glial astrocytes and fibrillary background brain edema observed in rats with TP-induced chronic HN. (d) Showing neuronal cell necrosis (short arrow) associated with congestion of cerebral blood vessel (long arrow).

DISCUSSION

In the present study, injection of TP (0.2 mg/kg/day, s. c.) along with 2.5% d-glucose solution (equivalent to 5% initial bw/day, i. p), for 3 successive days, induced profound (<115 mmol/l) chronic (>48 h) HN that was evidenced by decreased serum sodium level on days 4 and 6. A hypotonic dextrose solution was used as a source of electrolyte-free water to produce expansion of the extracellular fluid volume; while, TP was used as an antidiuretic agent to prevent the excretion of that electrolyte-free water for the entire period of the experiment. Both elements must be satisfied to induce HN [54]; since the administration of antidiuretic agent without water does not result in HN [55], and administration of electrolyte-free water in the absence of antidiuretic agent leads, only, to a large water diuresis [56]. TP is a long-acting analog of VP, the antidiuretic hormone [57]. Like VP, TP stimulates vascular vasopressin type 1 (V₁) receptor and renal tubular V₂ receptor, resulting in vasoconstriction and renal free water reabsorption, respectively. However, TP has a relatively higher affinity for the V₁ receptor and lower affinity to the V₂ receptor compared to VP [58]. Nevertheless, in agreement with the finding of the present study, Krag et al. [59] reported that TP induces V₂ receptor-mediated antidiuresis and induces a decrease in plasma sodium level. In the common experimental animal models of HN, VP has been used, either as multiple doses per day or as a continuous infusion via subcutaneously implanted osmotic minipump [60, 61]. Interestingly, a single daily dose of 0.2 mg/kg TP for three successive days induced chronic HN in the current model. The different pharmacokinetic properties of VP and TP explain this outcome. TP has a long duration of action and its effective half-life time is 6 h, whereas that of VP is only 6 min [58, 62]. For that, this TP-induced HN model that was established in our previous study with colleagues (unpublished data [49]), is less complicated than the common VP model. In addition, TP is available in the markets (glypressine; Ferring Company, Germany), while VP is not commercially available in all countries [62]. A stabilizing dose of TP (0.1 mg/kg/day, s. c.) was used for another three days following the induction phase. This regimen was carried out to prevent the spontaneous correction of chronic HN [48], and to simulate its clinical conditions [63]. The current TP-induced HN resulted in neurological complications in rats evidenced by the deterioration of the locomotor activity and pain reflex and confirmed by the histopathological findings revealed a marked brain edema. The chronic locomotor deficit that persisted for 6 d, and the delay of pain reflex detected on the 4^th day, in rats with TP-induced HN are parallel to some of the typical signs of hyponatremic encephalopathy found in patients with HN [14]. However, the improvement of the pain reflex on day 6 may be due to the gradual adaptation of the brain to HN by extruding organic solutes from their cytoplasm, which decreases the degree of cerebral edema by allowing intracellular osmolality to be equal to plasma osmolality without a large increase in cell water [64]. This explanation may be supported by the study established that the impaired response to pain stimuli in patients with HN occurs in the more advanced state of cerebral edema rather than that associated with a reduction of locomotor activity [11].

Following the induction phase, administration of GT (600 mg/kg/day, p. o), for 3 successive days, corrected the serum sodium level in rats. This protective effect of GT against HN may be attributed to its diuretic effect [25, 26, 28], as previous studies showed that diuretics are useful in controlling edematous hyponatremic states [65, 66]. Improvement of locomotor activity was also observed in GT-treated rats; a finding that indicates a neuroprotective effect of GT against TP-induced hyponatremic encephalopathy. This conclusion was confirmed by the outcome of the histopathological investigation that revealed a marked improvement of TP-induced brain edema in the GT-treated group. In addition, Michna et al. [67] reported a direct stimulatory effect of oral administration of green tea and caffeine on locomotor activity in mice.

On the other hand, delayed response to the nociceptive stimulus was noticed in GT-treated rats; though it was normal in untreated rats with TP-HN. This finding may be explained by the stated analgesic effect of GT [68, 69].

Administration of HtNaCl in the present study corrected HN itself but not its effect on locomotor activity. Actually, administration of high concentrations of NaCl results in a rapid correction of serum sodium level, which causes a serious cerebral demyelinating disorder known as osmotic demyelination syndrome (ODS) [70]. The clinical manifestations of ODS usually develop after a couple of days (average 4–6 d) following changes in sodium levels. Hence, the non-corrected locomotor activity observed with HtNaCl administration in the current study may be due to the beginning of the pathological changes in the brain that finally led to ODS. Fortunately, these findings were supported by the present histopathological observations of focal cellular necrosis with neovascular proliferation changes in the cerebral tissue of rats treated with HtNaCl, though the marked amelioration of brain edema. These observations are in agreement with those of previous studies showing that rapid correction of experimental animal models of HN with HtNaCl resulting in demyelinative lesions associated with focal cellular necrosis, gliovascular proliferation changes, and accumulation of active microglia [71-73]. These microglia have been found to produce proinflammatory cytokines, which are potent inducers of iNOS [74]. The induction of iNOS by proinflammatory cytokines results in NO production, which aggravates oligodendroglial injury and demyelination [73]. In the present study, significantly high levels of iNOS and NOx were observed in the brain tissues of hyponatremic rats treated with HtNaCl; this indicated the presence of inflammatory cerebral damage coupled with excessive iNOS activation and NO production. The presence of this inflammatory cerebral damage in HtNaCl-treated rats was also supported by the findings of the locomotor assessment and histopathological analysis. On the other hand, iNOS and NOx levels were normal in the brain tissues of rats with TP-induced HN, indicating that, iNOS activation and NO production are not involved in the neuropathological features of hyponatremic encephalopathy. In accordance, studies that assessed iNOS activity in experimental animals with HN showed that iNOS activity increases only with rapid correction of chronic HN [71-73]. GT successfully managed brain iNOS and NOx levels after the correction of HN in the present study. This result, together with the findings of the histopathological investigation, demonstrated the neuro-protective effect of GT against the pathological consequences of rapid correction of HN. The study of Nakagawa and Yokozawa [75] showed a direct scavenging of nitric oxide and superoxide by GT. On the other hand, Srivastava et al. [76] demonstrated that GT polyphenols act as potent inhibitors of nitric oxide generation independent of their antioxidant properties. Correspondingly, many studies reported the inhibition of iNOS expression by GT and GT polyphenols [77-80]; and considered it as an important mechanism underlying the neuroprotective effect of GT [81]. Choosing the 8 d duration for the experiment, before sacrificing the animals and isolation of brain for estimation of iNOS and NOx contents and histopathological examination, was guided by a previous study [60], to allow the development of the inflammatory cerebral damage that eventually leads to ODS, if any. In addition, another study [73] found that prominent accumulation of activated microglia was seen by 3 d after correction and that accumulation occurred parallel to the demyelinating changes.

CONCLUSION

In conclusion, the current study revealed that TP-induced HN rat model produced the main neuropathological features of human HN as manifested by the observed decrease of locomotor activity, delay of pain reflex, and development of the characteristic histopathological changes of the brain tissues. Administration of GT markedly improved TP-induced chronic HN in rats and protected against the neuropathological features that characterized hyponatremic encephalopathy and accompanied with its rapid correction. The study suggests GT as a therapeutic agent for protection against the neuropathological complications associated with chronic HN and its rapid correction.

CONFLICT OF INTERESTS

Declared none

REFERENCES

1. Adrogue HJ, Madias NE. Hyponatremia. N Engl J Med 2000;342:1581-9.
2. Upadhyay A, Jaber BL, Madias NE. Incidence and prevalence of hyponatremia. Am J Med 2006;119:S30-5.
3. Verbalis JG, Goldsmith SR, Greenberg A, Schrier RW, Sterns RH. Hyponatremia treatment guidelines: expert panel recommendations. Am J Med 2007;120:S1-21.
4. Liamis G, Milionis H, Elisaf M. A review of drug-induced hyponatremia. Am J Kidney Dis 2008;52:144-53.
5. Gandelman MS. Review of carbamazepine-induced hyponatremia. Prog Neuropsychopharmacol Biol Psychiatry 1994;18:211-33.
6. Schrier RW, Bansal S. Diagnosis and management of hyponatremia in acute illness. Curr Opin Crit Care 2008;14:627-34.
7. Rosner MH, Kirven J. Exercise-associated hyponatremia. Clin J Am Soc Nephrol 2007;2:151-61.
8. Ghatol A, Kazory A. Ecstasy-associated acute severe hyponatremia and cerebral edema: a role for osmotic diuresis? J Emerg Med 2009;42:e137-40.
9. Sterns RH. Postoperative hyponatremia in menstruant women. Ann Intern Med 1993;118:984-5.
10. Moritz ML, Ayus JC. The pathophysiology and treatment of hyponatraemic encephalopathy: an update. Nephrol Dial Transplant 2003;18:2486-91.
11. Adrogue HJ, Madias NE. Hyponatremia. N Engl J Med 2000;342:1581-9.
12. Sjoblom E, Hojer J, Ludwigs U, Pirskanen R. Fatal hyponatraemic brain oedema due to common gastroenteritis with accidental water intoxication. Intensive Care Med 1997;23:348-50.
13. Sterns RH. Severe symptomatic hyponatremia: treatment and outcome. A study of 64 cases. Ann Intern Med 1987;107:656-64.
14. Kozniewska E, Podlecka A, Rafalowska J. Hyponatremic encephalopathy: some experimental and clinical findings. Folia Neuropathol 2003;41:41-5.
15. Sterns RH, Cappuccio JD, Silver SM, Cohen EP. Neurologic sequelae after treatment of severe hyponatremia: a multicenter perspective. J Am Soc Nephrol 1994;4:1522-30.
16. Lien YH. Role of organic osmolytes in myelinolysis. A topographic study in rats after rapid correction of hyponatremia. J Clin Invest 1995;95:1579-86.
17. Sterns RH, Silver SM. Brain volume regulation in response to hypo-osmolality and its correction. Am J Med 2006;119:S12-6.
18. Decaux G, Mols P, Cauchi P, Delwiche F. Use of urea for the treatment of water retention in hyponatraemic cirrhosis with ascites resistant to diuretics. Br Med J 1985;290:1782-3.
19. Verbalis JG. AVP receptor antagonists as aquaretics: review and assessment of clinical data. Cleve Clin J Med 2006;73 Suppl 3:S24-33.
20. Schrier RW. The sea within us: disorders of body water homeostasis. Curr Opin Invest Drugs 2007;8:304-11.
21. McKay DL, Blumberg JB. The role of tea in human health: an update. J Am Coll Nutr 2002;21:1-13.
22. Cabrera C, Artacho R, Gimenez R. Beneficial effects of green tea--a review. J Am Coll Nutr 2006;25:79-99.
23. Chacko SM, Thambi PT, Kuttan R, Nishigaki I. Beneficial effects of green tea: a literature review. Chin Med 2010;5:13.
24. Afzal M, Safer AM, Menon M. Green tea polyphenols and their potential role in health and disease. Inflammopharmacology 2015;23:151-61.
25. Fenton RA, Poulsen SB, de la Mora Chavez S, Soleimani M, Busslinger M, Dominguez Rieg JA, et al. Caffeine-induced diuresis and natriuresis is independent of renal tubular NHE3. Am J Physiol Renal Physiol 2015;308:F1409-20.
26. Ming Z, Lautt WW. Caffeine-induced natriuresis and diuresis via blockade of hepatic adenosine-mediated sensory nerves and a hepatorenal reflex. Can J Physiol Pharmacol 2010;88:1115-21.
27. Wu CD, Wei GX. Tea as a functional food for oral health. Nutrition 2002;18:443-4.
28. Zhang Y, Coca A, Casa DJ, Antonio J, Green JM, Bishop PA. Caffeine and diuresis during rest and exercise: a meta-analysis. J Sci Med Sport 2015;18:569-74.
29. Dona M, Dell'Aica I, Calabrese F, Benelli R, Morini M, Albini A, et al. Neutrophil restraint by green tea: inhibition of inflammation, associated angiogenesis, and pulmonary fibrosis. J Immunol 2003;170:4335-41.
30. Haqqi TM, Anthony DD, Gupta S, Ahmad N, Lee MS, Kumar GK, et al. Prevention of collagen-induced arthritis in mice by a polyphenolic fraction from green tea. Proc Natl Acad Sci USA 1999;96:4524-9.
31. Sudano Roccaro A, Blanco AR, Giuliano F, Rusciano D, Enea V. Epigallocatechin-gallate enhances the activity of tetracycline in staphylococci by inhibiting its efflux from bacterial cells. Antimicrob Agents Chemother 2004;48:1968-73.
32. Weber JM, Ruzindana-Umunyana A, Imbeault L, Sircar S. Inhibition of adenovirus infection and adenain by green tea catechins. Antiviral Res 2003;58:167-73.
33. Sartippour MR, Shao ZM, Heber D, Beatty P, Zhang L, Liu C, et al. Green tea inhibits vascular endothelial growth factor (VEGF) induction in human breast cancer cells. J Nutr 2002;132:2307-11.
34. Osada K, Takahashi M, Hoshina S, Nakamura M, Nakamura S, Sugano M. Tea catechins inhibit cholesterol oxidation accompanying oxidation of low-density lipoprotein in vitro. Comp Biochem Physiol Part C: Toxicol Pharmacol 2001; 128:153-64.
35. Salama A, Elsayeh B, Ismaiel I, El-Shenawy S. Comparative evaluation of protective effects of green tea and lycopene in potassium dichromate-induced acute renal failure in rats. J Chem Pharm Res 2014;6:168-77.
36. Weinreb O, Mandel S, Amit T, Youdim MB. Neurological mechanisms of green tea polyphenols in Alzheimer's and Parkinson's diseases. J Nutr Biochem 2004;15:506-16.
37. Assuncao M, Andrade JP. Protective action of green tea catechins in neuronal mitochondria during aging. Front Biosci 2015;20:247-62.
38. Raederstorff DG, Schlachter MF, Elste V, Weber P. Effect of EGCG on lipid absorption and plasma lipid levels in rats. J Nutr Biochem 2003;14:326-32.
39. Kapoor S. Green tea: beneficial effects on cholesterol and lipid metabolism besides endothelial function. Eur J Cardiovascular Prevention Rehabilitation 2008;15:497.
40. Ahmad RS, Butt MS, Sultan MT, Mushtaq Z, Ahmad S, Dewanjee S, et al. Preventive role of green tea catechins from obesity and related disorders especially hypercholesterolemia and hyperglycemia. J Transl Med 2015;13:79.
41. Bajerska J, Mildner-Szkudlarz S, Walkowiak J. Effects of rye bread enriched with green tea extract on weight maintenance and the characteristics of metabolic syndrome following weight loss: a pilot study. J Med Food 2015;18:698-705.
42. Kavanagh KT, Hafer LJ, Kim DW, Mann KK, Sherr DH, Rogers AE, et al. Green tea extracts decrease carcinogen-induced mammary tumor burden in rats and rate of breast cancer cell proliferation in culture. J Cell Biochem 2001;82:387-98.
43. Cerezo-Guisado MI, Zur R, Lorenzo MJ, Risco A, Martin-Serrano MA, Alvarez-Barrientos A, et al. Implication of Akt, ERK1/2 and alternative p38MAPK signaling pathways in human colon cancer cell apoptosis induced by green tea EGCG. Food Chem Toxicol 2015;84:125-32.
44. Sueoka N, Suganuma M, Sueoka E, Okabe S, Matsuyama S, Imai K, et al. A new function of green tea: prevention of lifestyle-related diseases. Ann N Y Acad Sci 2001;928:274-80.
45. Vinson JA. Black and green tea and heart disease: a review. Biofactors 2000;13:127-32.
46. Keske MA, Ng HL, Premilovac D, Rattigan S, Kim JA, Munir K, et al. Vascular and metabolic actions of the green tea polyphenol epigallocatechin gallate. Curr Med Chem 2015;22:59-69.
47. Osswald H, Schnermann J. Methylxanthines and the kidney. Handb Exp Pharmacol 2011:391-412.
48. Schnermann J, Osswald H, Hermle M. Inhibitory effect of methylxanthines on feedback control of glomerular filtration rate in the rat kidney. Pflügers Archiv 1977;369:39-48.
49. Hegazy R, Zaki H, Ismail I, Sharaf O, Kenawy S. Effects of strawberry leaves and celery seeds extracts in terlipressin-induced chronic hyponatremia in rats. Toxicol Lett 2011;205:95.
50. Kauppila T, Tanila H, Carlson S, Taira T. Effects of atipamezole, a novel alpha 2-adrenoceptor antagonist, in open-field, plus-maze, two compartment exploratory and forced swimming tests in the rat. Eur J Pharmacol 1991;205:177-82.
51. Kelly MA, Rubinstein M, Phillips TJ, Lessov CN, Burkhart-Kasch S, Zhang G, et al. Locomotor activity in D₂ dopamine receptor-deficient mice is determined by gene dosage, genetic background, and developmental adaptations. J Neurosci 1998;18:3470-9.
52. Laviola G, Alleva E. Ontogeny of muscimol effects on locomotor activity, habituation, and pain reactivity in mice. Psychopharmacology 1990;102:41-8.
53. Jones M, Onslow M, Packman A, Gebski V. Guidelines for statistical analysis of the percentage of syllables stuttered data. J Speech Hear Res 2006;49:867-78.
54. Gowrishankar M, Chen CB, Cheema-Dhadli S, Steele A, Halperin ML. Hyponatremia in the rat in the absence of positive water balance. J Am Soc Nephrol 1997;8:524-9.
55. Leaf A, Bartter FC, Santos RF, Wrong O. Evidence in man that electrolyte urinary loss induced by pitressin is a function of water retention. J Clin Invest 1953;32:868-78.
56. Kleeman CR, Rubini ME, Lamdin E, Epstein FH. Studies on alcohol diuresis. II. The evaluation of ethyl alcohol as an inhibitor of the neurohypophysis. J Clin Invest 1955;34:448-55.
57. Forsling ML, Aziz LA, Miller M, Davies R, Donovan B. Conversion of tri glycyl vasopressin to lysine-vasopressin in man. J Endocrinol 1980;85:237-44.
58. Bernadich C, Bandi JC, Melin P, Bosch J. Effects of F-180, a new selective vasoconstrictor peptide, compared with terlipressin and vasopressin on systemic and splanchnic hemodynamics in a rat model of portal hypertension. Hepatology 1998;27:351-6.
59. Krag A, Bendtsen F, Pedersen EB, Holstein-Rathlou NH, Moller S. Effects of terlipressin on the aquaretic system: evidence of antidiuretic effects. Am J Physiol Renal Physiol 2008;295: F1295-300.
60. Soupart A, Penninckx R, Stenuit A, Perier O, Decaux G. Treatment of chronic hyponatremia in rats by intravenous saline: comparison of rate versus the magnitude of correction. Kidney Int 1992;41:1662-7.
61. Wada K, Matsukawa U, Fujimori A, Arai Y, Sudoh K, Sasamata M, et al. A novel vasopressin dual V_1A/V₂ receptor antagonist, conivaptan hydrochloride, improves hyponatremia in rats with the syndrome of inappropriate secretion of antidiuretic hormone (SIADH). Biol Pharm Bull 2007;30:91-5.
62. Delmas A, Leone M, Rousseau S, Albanese J, Martin C. Clinical review: vasopressin and terlipressin in septic shock patients. Crit Care 2005;9:212-22.
63. Coenraad MJ, Bolk JH, Frolich M, Meinders AE. Plasma arginine vasopressin and atrial natriuretic peptide concentration in patients with hyponatremia at diagnosis and the following treatment. Eur J Intern Med 2007;18:221-9.
64. Moritz ML, Ayus JC. New aspects in the pathogenesis, prevention, and treatment of hyponatremic encephalopathy in children. Pediatr Nephrol 2010;25:1225-38.
65. Szatalowicz VL, Miller PD, Lacher JW, Gordon JA, Schrier RW. Comparative effect of diuretics on renal water excretion in hyponatraemic oedematous disorders. Clin Sci 1982;62:235-8.
66. Goh KP. Management of hyponatremia. Am Fam Physician 2004;69:2387-94.
67. Michna L, Lu YP, Lou YR, Wagner GC, Conney AH. The stimulatory effect of oral administration of green tea and caffeine on locomotor activity in SKH-1 mice. Life Sci 2003;73:1383-92.
68. Eshghpour M, Mortazavi H, Mohammadzadeh Rezaei N, Nejat A. Effectiveness of green tea mouthwash in postoperative pain control following surgical removal of impacted third molars: double-blind, randomized clinical trial. Daru 2013;21:59.
69. Renno WM, Saleh F, Klepacek I, Al-Khaledi G, Ismael H, Asfar S. Green tea pain modulating effect in sciatic nerve chronic constriction injury rat model. Nutr Neurosci 2006;9:41-7.
70. Norenberg MD, Leslie KO, Robertson AS. Association between the rise in serum sodium and central pontine myelinolysis. Ann Neurol 1982;11:128-35.
71. KeQH, Chen JH, Zheng SS, Yu J, Liang TB. Prevention of central pontine myelinolytic in rats by early treatment with dexamethasone. Zhejiang Daxue Xuebao Yixueban 2006;35:424-9.
72. KeQH, Liang TB, Yu J, Zheng SS. A study of the pathogenesis and prevention of central pontine myelinolysis in a rat model. J Int Med Res 2006;34:264-71.
73. Takefuji S, Murase T, Sugimura Y, Takagishi Y, Hayasaka S, Oiso Y, et al. Role of microglia in the pathogenesis of osmotic-induced demyelination. Exp Neurol 2007;204:88-94.
74. Xie QW, Kashiwabara Y, Nathan C. Role of transcription factor NF-kappa B/Rel in the induction of nitric oxide synthase. J Biol Chem 1994;269:4705-8.
75. Nakagawa T, Yokozawa T. Direct scavenging of nitric oxide and superoxide by green tea. Food Chem Toxicol 2002;40:1745-50.
76. Srivastava RC, Husain MM, Hasan SK, Athar M. Green tea polyphenols and tannic acid act as potent inhibitors of phorbol ester-induced nitric oxide generation in rat hepatocytes independent of their antioxidant properties. Cancer Lett 2000;153:1-5.
77. Peristiowati Y, Indasah I, Ratnawati R. The effects of catechin isolated from green tea GMB-4 on NADPH and nitric oxide levels in endothelial cells exposed to high glucose. J Intercult Ethnopharmacol 2015;4:114-7.
78. Faria AM, Papadimitriou A, Silva KC, Lopes de Faria JM, Lopes de Faria JB. Uncoupling endothelial nitric oxide synthase is ameliorated by green tea in experimental diabetes by re-establishing tetrahydrobiopterin levels. Diabetes 2012;61: 1838-47.
79. Agnetti G, Bordoni A, Angeloni C, Leoncini E, Guarnieri C, Caldarera CM, et al. Green tea modulation of inducible nitric oxide synthase in hypoxic/reoxygenated cardiomyocytes. Biochimie 2005;87:457-60.
80. Chan MM, Fong D, Ho CT, Huang HI. Inhibition of inducible nitric oxide synthase gene expression and enzyme activity by epigallocatechin gallate, a natural product from green tea. Biochem Pharmacol 1997;54:1281-6.
81. Kim JS, Kim JM, O JJ, Jeon BS. Inhibition of inducible nitric oxide synthase expression and cell death by (-)-epigallocatechin-3-gallate, a green tea catechin, in the 1-methyl-4-phenyl-1,2,3,6-tetrahydropyridine mouse model of Parkinson's disease. J Clin Neurosci 2010;17:1165-8.