Crocus Sativus L. (Saffron) Extract and its Active Constituents (Crocin and Safranal) on Ischemia-Reperfusion in Rat Skeletal Muscle

Hossein Hosseinzadeh¹, Mohammad Hadi Modaghegh² and Zahra Saffari³

¹Pharmaceutical Research Center, ²Mashhad Vascular Surgery Research Center, Imam Reza Hospital and ³Pharmacology and Toxicology Department, School of Pharmacy, Mashhad University of Medical Sciences, Mashhad, I. R. Iran

Abstract

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Abstract
Introduction
Method
Biochemical Assays
Results
Discussion
Acknowledgements
References

Saffron and its constituents have been shown to decrease ischemia-reperfusion(I/R) injury in kidney or brain tissues. In this study, theeffects of saffron ethanolic extract and its constituents, crocinand safranal, were evaluated in skeletal muscle during I/R injury.Hind limb ischemia was induced using clamping the common femoralartery and vein. After 2 h ischemia, the clamp of the femoralvessels of animals was taken off and the animal underwent 1hreperfusion. Muscle injuries were evaluated by recording ofthe electromyographic (EMG) potentials and performing some biochemicalanalysis including thiobarbituric acid reactive substances (TBARS),total sulfhydryl (SH) groups and antioxidant capacity of muscle(using FRAP assay). The ethanolic extract of saffron (5, 20and 80 mg kg^–1), crocin (50, 200 and 400 mg kg^–1),safranal (0.1, 0.25 and 0.5 ml kg^–1) and normal saline(10 ml kg^–1) were administered intraperitoneally 1 h priorreperfusion. The average peak-to-peak amplitude during I/R wassignificantly increased in extract, crocin and safranal groupsin comparison with control-ischemic group. Following saffron,crocin and safranal administration, the total SH contents andantioxidant capacity were elevated in muscle flap. The MDA levelwas declined significantly in test groups. It is concluded thatsaffron extract and its constituents show a protective effectagainst lower limb I/R in rat.

Keywords: Saffron (Crocus sativus L.) – Crocin – Safranal – Oxidative stress – Lower limb ischemia – Reperfusion

Introduction

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Abstract
Introduction
Method
Biochemical Assays
Results
Discussion
Acknowledgements
References

Skeletal muscle ischemia and reperfusion injury remain an issueof concern because of the morbidity and mortality that followsrevascularization of an acutely ischemic limb (1). Many studieshave suggested the beneficial effects of nutrients or otheragents such as vitamin E (2), C (3), green tea extract (2),melatonin (4,5), carbenoxolone (6) and green propolis (7,8)in reducing or preventing cerebral or muscle injury during ischemia.-reperfusion(I/R).

Crocus sativus L. commonly known as saffron, is a perennialstemless herb of the Iridaceae family and widely cultivatedin Iran and other countries such as India and Greece (9). Commercialsaffron comprises the dried red stigma with a small portionof the yellowish style attached. Compounds considered pharmacologicallyactive and important are volatile agents (e.g. safranal), bitterprinciples (e.g. picrocrocin) and dye materials (e.g. crocetinand its glycoside, crocin) (9). In modern pharmacological studies,saffron, or its active constituents, has demonstrated anticonvulsant(10), antidepressant (11), anti-inflammatory (12) and antitumouractivities (13,14). Radical scavenger effects as well as learningand memory improving properties (15,16) and promote the diffusivityof oxygen in different tissues were also reported (9). Saffronextract is also chemopreventive and showed protective effectson genotoxins-induced oxidative stress in Swiss albino mice(17–19 ).

Recently, Assimopoulou et al. (20) showed that the saffron extract,crocin and safranal exhibited significant radical scavengingactivity and thus antioxidant activity. There was also a constantdecrease in lipoprotein oxidation susceptibility in healthyindividuals after administration of 50 mg of saffron twice aday (21). Saffron and its constituents have been shown to decreaseI/R injury in kidney (22) or brain tissues (23). Thus, in thisstudy the effect of saffron extract and its constituents wasevaluated during I/R on an animal model of I/R injury in anothertissue, the rat hind limb. Ischemia damages were evaluated usingrecording of EMG potentials (to show the viability of nerve)and measuring oxidative markers. Malondialdehyde and SH-groupswere measured as parameters for lipid peroxidation and oxidative-stressmarkers (24). Antioxidant capacity of muscle was evaluated usingFRAP assay (24).

Method

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Abstract
Introduction
Method
Biochemical Assays
Results
Discussion
Acknowledgements
References

Animals

Male Wistar rats, 200–250 g were housed in colony roomswith 12/12 h light/dark cycle at 21 ± 2°C and hadfree access to food and water. All animal experiments were carriedout in accordance with Mashhad University of Medical Sciences,Ethical Committee Acts.

Materials

Safranal and crocin were obtained from Fluka. DTNB (2, 2'-dinitro-5,5'-dithiodibenzoic acid), TPTZ (2, 4, 6-tri (2-pyridyl)-1, 3,5-triazine), TBA (2-thiobarbituric acid), n-butanol, Tris, Na₂EDTA,sodium acetate, glacial acetic acid, phosphoric acid, potassiumchloride, tetramethoxypropane (TMP), ferric chloride (FeCl₃.6H₂O),ferrous sulfate and hydrochloric acid was obtained from Merck.Xylazine and ketamine were obtained from Loughrea, Co. (Galway,Ireland) and Rotexmedica (GmbH, Germany), respectively. Fordilution, saffron and crocin were dissolved in distilled water.

Induction of Ischemia

The rats were anesthetized with intraperitoneal injection ofketamine/xylazine (60 mg kg^–1 and 6 mg kg^–1, respectively).Additional doses of these agents were used if anesthesia lightenedduring experiment.

An incision in the inner side of the hind leg from the inguinalligament to the tendon calcaneus insertion was made.

Then it was divided up and the triceps surae was dissected asa muscle flap, after that insertions to femur was cut. Previouslydissected femoral vessels, the artery and vein were clampedwith a single clamp of microsurgery. The absence of bleedingwas verified in the muscle flap. Then the incision was closedto prevent desiccation. For reperfusion periods, the clamp ofthe femoral vessels of animals was taken off and then the bleedingof the muscle flap was verified (6). The muscle tissues washomogenized in cold KCl solution (1.5%) to give a 10% homogenysuspension and used for biochemical assays. The results wereexpressed by n or micromolar tissue (1 ml of homogenate = 0.1g of tissue). In some references these data are expressed asn or µM/g protein.

Experimental Protocol

Eleven groups of animals were used, each of which contained8 rats: Group 1 including sham operated animals, group 2 servedas ischemic control to which saline (10 ml/kg^–1) was injectedintraperitoneally (i.p.). Group 3–5 was received the ethanolicextract of saffron (5, 20 and 80 mg kg^–1). Crocin wasinjected to group 6–8 (50, 200 and 400 mg kg^–1)and safranal (0.1, 0.25 and 0.5 ml kg^–1) was administeredto group 9–11. All drugs were administrated intraperitoneally1 h before reperfusion.

The hind legs of groups 2–11 were exposed to 2 h ischemiaand 1 h reperfusion.

Electromyography Data Collection

To determine the muscles and nerve activities during I/R, intramuscularelectromyograph (EMG) signals were recorded with PowerLab dataacquisition systems. Two pairs of pin electrodes in terminatingalligator clips were inserted into the triceps surae (muscleflap) in hind leg, and adductor muscles. The distance betweenthe two electrodes of a pair in each muscle was 5 mm. A groundingelectrode was gently attached to the rat tail (25). The EMGsignals were collected with sampling frequency of 12 PPM (MacLab/4SP).Duration for each stimulation was 20 ms. The raw EMG signalswere low-pass filtered at 50 Hz and EMG signal was expressedas average peak-to-peak amplitude for a 10 min recording periods.

Preparation of Saffron Extract

Crocus sativus L. stigmas were collected from Ghaen (Khorasanprovince, Northeast of Iran). In the maceration method, 10 gof stigmas were macerated in 500 ml ethanol (80 v/v) for threedays. The mixture was subsequently filtered and concentratedunder reduced pressure at 40°C. The extract yield was 52%w/w.

Saffron sample was analyzed according to the ISO 3632-2: Bitterness,expressed as direct reading of the absorbance of picrocrocineat about 257 nm, on dry basis was 96.9; safranal, expressedas direct reading of the absorbance at about 330 nm, on drycategories was 41.5 and coloring strength, expressed as directreading of the absorbance of crocin at about 440 nm, on drybasis was 259.

Biochemical Assays

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Abstract
Introduction
Method
Biochemical Assays
Results
Discussion
Acknowledgements
References

Thiobarbituric Acid Reactive Species (TBARS) Measurement

Malondialdehyde (MDA) levels, as an index of lipid peroxidation,were measured. MDA reacts with thiobarbituric acid (TBA) asa thiobarbituric acid reactive substance (TBARS) to producea red colored complex which has peak absorbance at 532 nm (26).

3 ml phosphoric acid (1%) and 1 ml TBA (0.6%) was added to 0.5ml of muscle homogenate in a centrifuge tube and the mixturewas heated for 45 min in a boiling water bath. After cooling,4 ml of n-butanol was added the mixture and vortex-mixed for1 min followed by centrifugation at 20000 rpm for 20 min. Theorganic layer was transferred to a fresh tube and its absorbancewas measured at 532 nm. The standard curve of MDA was constructedover the concentration range of 0–40 µM (27).

Ferric Reducing/Antioxidant Power (FRAP) Assay

The FRAP assay measures the change in absorbance at 593 nm owingto the formation of a blue colored Fe^II-tripyridyltriazine compoundfrom the colorless oxidized Fe^III form by the action of electrondonating antioxidants (28).

The FRAP reagent consist of 300 mM acetate buffer (3.1 g sodiumacetate + 16 ml glacial acetic acid, made up to 1 l with distilledwater; pH = 3.6), 10 mM TPTZ in 40 mM HCl and 20 mM FeCl₃.6H₂Oin the ratio of 10:1:1.

Briefly, 50 µl of muscle homogenate was added to 1.5 mlfreshly prepared and prewarmed (37°C) FRAP reagent in atest tube and incubated at 37°C for 10 min. The absorbanceof the blue colored complex was read against reagent blank (1.5ml FRAP reagent + 50 µl distilled water) at 593 nm. Standardsolutions of Fe^II in the range of 100 to 1000 mM were preparedfrom ferrous sulphate (FeSO₄.7H₂O) in distilled water. The datawas expressed as mM ferric ions reduced to ferrous form perliter (FRAP value) (29).

Total Sulfhydryl (SH) Groups Assay

Total SH groups were measured using DTNB (2, 2'-dinitro-5, 5'-dithiodibenzoicacid) as the reagent. This reagent reacts with the SH groupsto produce a yellow colored complex which has a peak absorbanceat 412 nm (30).

Briefly, 1 ml Tris-EDTA buffer (pH = 8.6) was added to 50 µlmuscle homogenate in 2 ml cuvettes and sample absorbance wasread at 412 nm against Tris-EDTA buffer alone (A₁). Then 20µl DTNB reagent (10 mM in methanol) was added to the mixtureand after 15 min (stored in laboratory temperature) the sampleabsorbance was read again (A₂). The absorbance of DTNB reagentwas also read as a blank (B). Total thiol concentration (mM)was calculated from the following equation:

Statistical Analysis

Data are expressed as mean ± SEM. Statistical analysiswas performed using one-way ANOVA followed by Tukey–Kramerpost-hoc test for multiple comparisons. The P-values less than0.05 were considered to be statistically significant.

Results

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Abstract
Introduction
Method
Biochemical Assays
Results
Discussion
Acknowledgements
References

Electromyography Data

The average peak-to-peak amplitudes in the control-ischemicgroup and sham were 1.71 ± 0.03, 1.57 ± 0.068V and 2.03 ± 0.03, 2.06 ± 0.63 V) respectivelyduring ischemia and reperfusion. The ethanolic extract of saffron,crocin and safranal increased the amplitude compare with ischemiaand reperfusion groups (Table 1).

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Table 1. Effects of ethanolic saffron extract, crocin and safranal on average peak-to-peak amplitudes of EMG signals, prior, during and after ischemia-reperfusion in rat skeletal muscle

Thiobarbituric Acid Reactive Species (TBARS) Measurement

There was an increase in the MDA levels following I/R as comparedwith sham-operated animals (Fig. 1). The saffron extract, crocinand safranal pretreatment resulted in a significant reductionin the free radical-mediated lipid peroxidation as indicatedby a decrease in the MDA levels, at various dose levels (Figs 1,2 and 3). In safranal-pretreated groups, a reduction in TBARSlevels was very prominent in the higher doses.

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Figure 1. Effect of ethanolic saffron extract on lipid peroxidation following muscle ischemia reperfusion injury. MDA levels were measured in 10% homogenates of muscle samples from rats subjected to 120 min of ischemia and 60 min of reperfusion. All drugs were administrated intraperitoneally 60 min prior to reperfusion. Values are mean ± SEM (n = 8). *P <0.05, ***P <0.001 as compared with vehicle (normal saline) treated animals (One-way ANOVA followed by Tukey–Kramer test).

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Figure 2. Effect of crocin on lipid peroxidation following muscle ischemia reperfusion injury. MDA levels were measured in 10% homogenates of muscle samples from rats subjected to 120 min of ischemia and 60 min of reperfusion. All drugs were administrated intraperitoneally 60 min prior to reperfusion. Values are mean ± SEM (n = 8). *P <0.05, ***P < 0.001 as compared with vehicle (normal saline) treated animals (One-way ANOVA followed by Tukey–Kramer test).

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Figure 3. Effect of safranal on lipid peroxidation following muscle ischemia reperfusion injury. MDA levels were measured in 10% homogenates of muscle samples from rats subjected to 120 min of ischemia and 60 min of reperfusion. All drugs were administrated intraperitoneally 60 min prior to reperfusion. Values are mean ± SEM (n = 8). *P <0.05, ***P <0.001 as compared with vehicle (normal saline) treated animals (One-way ANOVA followed by Tukey–Kramer test).

Modulation of FRAP Value

I/R caused a significant reduction in FRAP value of muscle homogenatesamples as compared with sham-operated animals (3.31 ±0.16 versus 2.45 ± 0.17 µmol/g tissue, P < 0.05)(Fig. 4). The ethanolic saffron extract, crocin and safranalpretreatment increased antioxidant power (FRAP value) of musclehomogenate samples (Figs 4, 5 and 6).

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Figure 4. Effect of ethanolic saffron extract on antioxidant power of muscle homogenate samples following muscle ischemia reperfusion injury. FRAP values were measured in 10% homogenate samples from rats subjected to 120 min of ischemia and 60 min of reperfusion. All drugs were administrated intraperitoneally 60 min prior to reperfusion. Values are mean ± SEM (n = 8). *P <0.05, **P <0.01 as compared with vehicle (normal saline) treated animals (One-way ANOVA followed by Tukey–Kramer test).

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Figure 5. Effect of crocin on antioxidant power of muscle homogenate samples following muscle ischemia reperfusion injury. FRAP values were measured in 10% homogenate samples from rats subjected to 120 min of ischemia and 60 min of reperfusion. All drugs were administrated intraperitoneally 60 min prior to reperfusion. Values are mean ± SEM (n = 8). **P <0.01 as compared with vehicle (normal saline) treated animals (One-way ANOVA followed by Tukey–Kramer test).

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Figure 6. Effect of safranal on antioxidant power of muscle homogenate samples following muscle ischemia reperfusion injury. FRAP values were measured in 10% homogenate samples from rats subjected to 120 min of ischemia and 60 min of reperfusion. All drugs were administrated intraperitoneally 60 min prior to reperfusion. Values are mean ± SEM (n = 8). *P <0.05, ***P <0.001 as compared with vehicle (normal saline) treated animals (One-way ANOVA followed by Tukey–Kramer test).

Total Thiol Concentration

Following I/R injury, a significant reduction in total SH groups(0.57 ± 0.03 versus 0.31 ± 0.02 mM, P < 0.01)in muscle homogenate samples was observed (Fig. 7). The ethanolicsaffron extract, crocin and safranal pretreatment caused a significantelevation in total thiol concentration, as compared with control-ischemicgroup (Figs 7, 8 and 9).

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Figure 7. Effect of ethanolic saffron extract on total thiol concentrations following muscle ischemia reperfusion injury. Total sulfhydryl (SH) groups were measured in 10% muscle homogenate samples from rats subjected to 120 min of ischemia and 60 min of reperfusion. All drugs were administrated intraperitoneally 60 min prior to reperfusion. Values are mean ± SEM (n = 8). *P <0.05, **P <0.01 as compared with vehicle (normal saline) treated animals (One-way ANOVA followed by Tukey–Kramer test).

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Figure 8. Effect of crocin on total thiol concentrations following muscle ischemia reperfusion injury. Total sulfhydryl (SH) groups were measured in 10% muscle homogenate samples from rats subjected to 120 min of ischemia and 60 min of reperfusion. All drugs were administrated intraperitoneally 60 min prior to reperfusion. Values are mean ± SEM (n = 8). ***P <0.01 as compared with vehicle (normal saline) treated animals (One-way ANOVA followed by Tukey–Kramer test).

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Figure 9. Effect of safranal on total thiol concentrations following muscle ischemia reperfusion injury. Total sulfhydryl (SH) groups were measured in 10% muscle homogenate samples from rats subjected to 120 min of ischemia and 60 min of reperfusion. All drugs were administrated intraperitoneally 60 min prior to reperfusion. Values are mean ± SEM (n = 8). ***P <0.001 as compared with vehicle (normal saline) treated animals (One-way ANOVA followed by Tukey–Kramer test).

	Discussion

Top Abstract Introduction Method Biochemical Assays Results Discussion Acknowledgements References

The results obtained in the present investigation suggest thatthe saffron extract and its active constituents, crocin andsafranal, have an overall protective effect against muscle I/Rinjury in a rat model.

A number of processes have been implicated in the pathogenesisof oxygen deprivation-induced cell injury. These include thedisturbances of cell calcium homeostasis, depletion of adeninenucleotides, activation of enzymes like phospholipases withproduction of toxic lipid metabolites, proteases and endonucleasesand generation of free radicals (ROS) that can cause oxidativedamage to cellular macromolecules (31,32). Antioxidant therapyhas been well documented to help in the improvement of organfunctions (33).

We assessed the effect of the saffron extract, crocin and safranalby studying their effects on lipid peroxidation. MDA levelsincreased significantly following muscle I/R. The saffron extractand its bioactive constituents reversed the increase of MDAlevels to a considerable extent, thereby confirming its antioxidantrole in I/R.

Under acute and chronic pathologic conditions such as ischemia,the balance between oxidant and antioxidant systems has beeninterrupted (34,35). Therefore we evaluate the antioxidant orreducing potential of muscle homogenate samples following muscleI/R, using FRAP assay. As expected following this, a significantreduction in antioxidant power, as indicated by FRAP value,was observed. The extract, crocin and safranal increased theantioxidant power of muscle homogenate samples.

Sulfhydryl (SH) groups are highly-reactive constituents of proteinmolecules, and they participate in important biochemical andmetabolic process such as cell division, blood coagulation,maintenance of protein systems and enzymatic activation includingantioxidant enzymes (catalase, superoxide dismutase, etc.) (36).There are also important scavengers of oxygen-derived free radicals(37). SH groups known to be sensitive to oxidative damage anddepleted following ischemic insult (38), therefore we studiedthe effect of these agents on total thiol concentration duringmuscle I/R. Similarly, in our studies, total sulfhydryl groupswere decreased following I/R injury. These agents exhibitedhigher SH contents in muscle tissues than their respective controls,indicating that helped in replenishing the total thiol pool.

As we said crocin and crocetin are main constituents that haveantioxidant activity, these means that these components werestudied for these effects. There are a lot other ingredientsin saffron extract which should evaluate for this effect. Inour study the saffron extract was more potent than crocin. Thismay be attributed to a synergistic action of many constituentssuch as crocins, crocetin, dimethyl crocetin, safranal and flovonoidswhich quench free radicals and have antioxidant effects andmay have role in protective effect of saffron on muscle I/R.In addition saffron contains proteins, sugars, vitamins (especiallyriboflavin), amino acids, minerals and gums. Also it seems crocinfrom Fluka is not completely pure.

Among the constituents of saffron stigmas, crocins and crocetinare the most abundant agents with established antioxidant andantitumor effects (9, 13 and 18). These carotenoids scavengefree radicals, especially superoxide anions and thereby mayprotect cells from oxidative stress (39). The aqueous saffronextract and its active constituent, crocin also prevent renalI/R-induced oxidative injury in rats (22). In our study thesaffron extract was more potent than crocin. This may be attributedto a synergistic action of many constituents such as crocins,crocetin, dimethyl crocetin, safranal and flovonoids which quenchfree radicals and have antioxidant effects and may have rolein protective effect of saffron on muscle I/R. In addition saffroncontains proteins, sugars, vitamins (especially riboflavin),amino acids, minerals and gums (9). It is also possible thatcrocin may be impure.

Safranal also showed anti-ischemia activity in this study. Thismonoterpene aldehyde, which is the major constituent of theessential oil of saffron (20) showed good antioxidant activity.Our recent studies showed that safranal also attenuated cerebralischemia induced oxidative damage in rat hippocampus (23). Assafranal showed suitable activity in almost all doses, it maybe concluded that safranal is major antioxidant constituentor played a major role in protecting I/R-induced oxidative injury.But it should be mentioned that safranal is usually presentin less than 1% of saffron extract (40).

It seems that I/R injury reduced the conductivity and viabilityof muscles and nerves. In this study, the saffron extract andits constituents maintained the nerve conductivity. Nerve conductionis decreased during I/R (41,42). Mild muscle necrotic changesoccur after 2–3 h ischemia (43,44). Oxidative stress andthe production of oxygen free radicals during I/R is one mechanismof ischemic fiber degeneration, causing a breakdown of the blood-nervebarrier, endoneurial edema and lipid peroxidation (45). Saffronand its constituents prevented lipid peroxidation and showedantioxidant activity in this study. These effects and otheractivities such as anti-inflammatory effect (12) may preserveviability of nerve conductivity. A reduction in the EMG potentialwas more severe in reperfusion phase than the ischemia stageas shown in another study (46).

In conclusion, the present study showed that saffron extractand its constituents, crocin and safranal, have protective effecton I/R injury-induced oxidative stress in rats muscle that atleast partly is due to antioxidant properties of saffron andits constituents.

Footnotes

For reprints and all correspondence: Hossein Hosseinzadeh, Pharmaceutical Research Center, Faculty of Pharmacy, 1365-91775, Mashhad University of Medical Sciences, Mashhad, I. R. Iran. Tel: 98 511 8823252; Fax: 98511 8823251; E-mail: hosseinzadehh{at}mums.ac.ir

Acknowledgements

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Abstract
Introduction
Method
Biochemical Assays
Results
Discussion
Acknowledgements
References

The authors are thankful to the Vice Chancellor of Research,Mashhad University of Medical Sciences for financial support.

References

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Discussion
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References

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Received July 5, 2006; accepted June 9, 2007

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Evidence-based Complementary and Alternative Medicine

Crocus Sativus L. (Saffron) Extract and its Active Constituents (Crocin and Safranal) on Ischemia-Reperfusion in Rat Skeletal Muscle