January-April 2023 UNIVERSA MEDICINA    Vol.42- No.1 

 
pISSN: 1907-3062 /  eISSN: 2407-2230 

 
 

Resveratrol protects against copper and iron toxicity 

in Drosophila melanogaster 

Osaretin Godwin Igharo1* , Lucky Osemu Ebaluegbeifoh2 , Godwin Aigbedo 

Aikpitanyi- Iduitua3 , Henry Uzor Oshilonyah4 , and Idris Babatunde Momodu5  

 
 

ABSTRACT 
 

 

BACKGROUND 

Copper (Cu) and iron (Fe) are essential trace elements that when in excess 

are capable of causing cytotoxic effects leading to lipid peroxidation and 

promoting oxidative stress. Resveratrol (RES) is a natural polyphenol with 

antioxidant and anti-inflammatory properties. This study was carried out 

to evaluate the protective role of RES in Fe and Cu sulphate-induced 

oxidative stress in Drosophila melanogaster. 

 
METHODS 

Adult wild type flies were fed Cu2+ and Fe2+ (1 mM each) and/or RES (30 

and 60 mg/kg diet) for 7 days. Survival, negative geotaxis and emergence 

rate were evaluated by daily recording of fruit fly mortality and final analysis. 

Fruit flies were anaesthetized using CO
2 
gas, homogenized and centrifuged 

at 4,000 rpm for 10 minutes at 4°C. Aliquots of the supernatants were used 

for the estimation of biochemical markers using spectrophotometry. 

 
RESULTS 

Fruit flies co-treated with FeSO4 + CuSO4 (1 mM each) + RES (30 and 60 

mg/Kg) significantly elevated H2O2, NO, lipid peroxidation, 

acetylcholinesterase as well as GSH, GST, catalase and total thiols (p<0.05) 

compared with the Cu2+ + Fe2+ (1mM each) treated group. Flies co-treated 

with FeSO4 + CuSO4 (1mM each) + RES (30 and 60mg/Kg) also had 

significantly improved (p< 0.05) eclosion and climbing rates compared with 

the Cu2+ + Fe2+ (1mM each) treated group. 

 

1Biomedical Toxicology and Chemical 

Safety Research Group, Department 

of Medical Laboratory Sciences, 

School of Basic Medical Sciences, 

College of Medical Sciences, 

University of Benin, Benin City, 

Nigeria 
2Centre of Excellence in Reproductive 

Health Innovative, University of 

Benin, Benin City, Nigeria 
3Education Department, Medical 

Laboratory 

Science Council of Nigeria,           Abuja, 

Nigeria 
4Department of Microbiology, Faculty 

of Science, University of Delta, Agbor, 

Delta State, Nigeria 
5Department of Science Laboratory 

Technology, Federal Polytechnic, 

Kaltungo, Gombe State 

 
*Correspondence: 

Dr. Osaretin Godwin Igharo  

University of Benin, Benin City, 

Nigeria 

Tel.: +2348038664896 

 Email: osaretin.igharo@uniben.edu 

 ORCID ID: 0000-0002-7086-534

   CONCLUSION 

This study demonstrated that RES reduced Cu2+ and Fe2+-induced radical 

generation in D. melanogaster and improved the antioxidant buffering 

capability of the flies. Therefore, RES could be used in management of 

disorders involving oxidative stress. 

 
Keywords: Resveratrol, reactive oxygen species, antioxidant, Drosophila 

melanogaster 

Date of first submission, October 31, 

2022 

Date of final revised submission, 

March 1, 2023 

Date of acceptance, March 8, 2023 

 
This open access article is distributed 

under a Creative Commons Attribution- 

Non Commercial-Share Alike 4.0 

International License 

 

 

 
 

ORIGINAL ARTICLE 

Cite this article as: Igharo OG, Ebaluegbeifoh LO, Aikpitanyi-Iduitua GA, Oshilonyah HU, Momodu IB. Resveratrol protects against 

copper and iron toxicity in Drosophila melanogaster. Univ Med 2023;42:29-40. doi: 10.18051/ UnivMed.2023.v42:29-40 

29 

DOI:        http://dx.doi.org/10.18051/UnivMed.2023.v42:29-40 

Copyright@Author(s)      -       https://univmed.org/ejurnal/index.php/medicina/article/view/1385 

https://orcid.org/0000-0002-7086-5347
https://orcid.org/0000-0001-5382-428X
https://orcid.org/0000-0002-8914-1998
https://orcid.org/0000-0003-2202-2713
https://orcid.org/0000-0002-8877-1998


30

Igharo, Ebaluegbeifoh, Aikpitanyi-Iduitua. et al                                                            Drosophila melanogaster

INTRODUCTION

Iron (Fe2+)) and copper (Cu2+) are essential
trace elements (ETE) for biological processes and
vital functions such as cell respiration, maturation
of erythrocytes, antioxidant defence, and enzyme
cofactors.(1) Iron and copper are cofactors
required by enzymes for structural and catalytic
activities in oxidative phosphorylation, protein
synthesis, and neurotransmission modulation.(2)

The routes for copper and iron administration are
through inhalation, consumption of contaminated
food and water, and dermal contact with polluted
air, water, and soil. Once inside the body, copper
and iron are first deposited in the liver after which
liver detoxification activities occur. These metals
are present in trace amounts because a variety
of homeostatic mec hanisms in normal
circumstances maintains a physiologically
essential amount of these metals.(1) However,
when in excess, dyshomeostatic mechanisms of
iron and copper are capable of causing cytotoxic
effects and production of highly damaging free
radicals by Fenton or Haber-Weiss reactions, thus
causing brain lipid peroxidation and protein
oxidation which promotes oxidative stress.(3,4)

Reactive oxygen species (ROS) are formed by
the ability of copper to change states, from cupric
(Cu2+) to cuprous (Cu+) by cuproenzymes which
are involved in redox reactions. Cuprous ions can
catalyse hydrogen peroxide decomposition,
through the Fenton reaction, which forms hydroxyl
radicals (OH) capable of reacting with biological
molecules such as proteins, lipids and DNA,
thereby damaging them.(5) The ability of iron to
accept and donate electrons can lead to the
formation of reactive nitrogen and oxygen species
which trigger the oxidative attack of the brain,
thereby contributing to brain disease and perhaps
aging itself. The buildup of copper or iron in the
liver, kidneys, brain, and eyes results in possible
cell death, permanent nerve damage, oxidative
stress, and reduced cell proliferation.(6,7)

Re s ve r a tr o l  ( RE S)  i s  a  po l yp h e no l
commonly found in grapes, wine, peanuts, and

soy, and is known to possess anti-oxidative, anti-
carcinogenic, and anti-inflammatory properties.(8,
9) A study showed that RES can alleviate liver
injury in iron-overloaded mice. The mechanism
may be related to improving antioxidant capacity
and reducing excess iron in the liver.(10)

Interestingly, Drosophila melanogaster
models have been used in vivo to investigate
disease mechanisms. (8-10) Drosophila has a
genetic makeup of about 60% homology to that
of humans. Also, the fruit fly possesses 75% of
the genes responsible for human diseases as
homologues, thereby making it a very good model
organism.(11) As a result of ROS production
which links oxidative stress, resveratrol mitigates
ROS generation through (i) the prevention of
molecular oxygen and/or peroxide reactions and
the chelation of iron and copper ion; (ii) the
chelation of iron and copper to the redox state
being kept, making the iron and copper incapable
to reduce molecular oxygen; (iii) the trapping of
formed radicals.(12) Previous studies have shown
that RES has the potency to increase glutathione
peroxidase, superoxide dismutase as well as
glutathione levels. Futher more, RES also
dec reases  lipi d pero xidati on and prot ein
oxidation. Thus, a decrease in the amount of lipid
peroxides also confirms the decrease in oxidative
stress.(8, 9)

One study showed that RES can alleviate
liver injury in iron-overloaded mice. The
mechanism may be related to improvement of
antioxidant capacity and reduction of excess iron
i n t he  l ive r. ( 13 ) St u di e s  on  t h e us e of D.
melanogaster in iron and copper-induced
oxidative stress and the preventive effects of
r e s ve r a t r ol  a r e  s c a r c e  i n t h e  l i t e r a t u r e .
Therefore, as an alternative to conventional
rodent models, a study is needed to investigate
the Cu2+ and Fe2+-induced toxicity and the
r e l e va n c e o f  RES p r o t e c t i ve  r ol e  in  D.
me la n og as t e r.  In  t hi s  r e s e a r c h , D.
melanogaster was employed as a model to
examine Cu2+ and Fe2+-induced toxicity and the
ameliorative impact of RES.



31

Univ Med                                                                                                                                                             Vol. 42 No. 1

METHODS

Research design
The experimental study was carried out at

the Drosophila laboratory, Department of
Biochemistry, University of Ibadan, Nigeria,
between January and August, 2021.

Drosophila melanogaster stock and culture
Dros o ph i l a me l a no g as t e r  ( Ha r wi c h

strain) of both genders (1-3 days old) were
cultured and maintained in the Drosophila
me la n og as t e r  Re se a r c h  La bo r a t o r y,
De pa rtment  of  Bioc he mistry, Col le ge of
Medicine, University of Ibadan, Oyo State,
Nigeria. The flies were allowed to mate in vials
monitored at regulated temperature and humidity
(22–24°C; 60–70% relative humidity) until the
eggs hatched into young adult fruit flies under
12 hours’ light and 12 hours’ dark daily cycles
for the period of administration of the chemical
compound under investigation.

Chemical compounds
Re sve ra tr ol  wa s p ro cur e d fro m A K

Scientific, 30023 Ahern Ave, Union City, CA
94587, United States of America at a percentage
purity of 95%. Copper sulphate and ferrous
sulphate were procured from Sigma Aldrich. All
chemicals used were of analytical grade. 1-
chloro-2,4-d initr obenzene ( CDNB), 5, 5'-
d it h i ob i s-2-n i t r o -be nzo i c a ci d  ( DT N B) ,
acetylthiocholine iodide, and hydrogen peroxide
(30% solution [w/w]) were purchased from
Sigma USA. Other reagents were commercial
products of high analytical grade.

Treatment of D. melanogaster with CuSO
4

and FeSO
4
 for oxidative stress inducement

The flies were fed on diet mixed with
CuSO

4
 and FeSO

4
 at a final dose of FeSO

4
 0.5

mM, FeSO
4 
1 mM, FeSO

4
 0.5 mM + CuSO

4 
0.5

mM a n d Fe SO
4
 1 mM  +  CuSO

4 
1 mM ,

respectively. The flies were monitored for 7 days,
harvested and homogenized, after which free
radical generation was determined.

Treatment of D. melanogaster with CuSO
4
,

FeSO
4
 and resveratrol

The flies were fed on a diet mixed with
CuSO

4
, FeSO

4
, and/or RES, while the final group

(G5) received EDTA instead of RES, at a dose
of 50mg/kg diet. The flies were divided into six
groups, each containing five replicates/groups
with 40 flies/vial: positive control: 50 mg EDTA
/kg diet, G1: 30 mg RES/kg diet), G2: 60 mg
RES/kg diet), G3: 1mM CuSO

4
 + 1mM FeSO

4

+ 30 mg RES/kg diet), G4: 1mMCuSO
4
 + 1mM

FeSO
4
 + 60 mg RES/kg diet and G5: (1mM

CuSO
4
 + 1mM FeSO

4
 + 50mg EDTA/kg diet).

The flies were monitored for 7 days, harvested
and homogenized, followed by determination of
free radical generation.

Preparation of  samples for biochemical
assays

For the determination of biochemical
assays, 50 flies (of both genders) were exposed
to final concentrations of FeSO

4
 0.5 mM, FeSO4

1 mM, FeSO
4
 0.5 mM + CuSO

4
 0.5 mM and

FeSO
4
 1 mM + CuSO

4
 1mM and RES (30 and

60 mg/kg diet) for 7 days. At the end of the
treatment period, flies were anaesthetized using
CO

2
, weighed, homogenized in 0.1M phosphate

buffer, pH 7.0 (ratio of 1 mg:10 mL), and
centrifuged at 4000 g for 10 min at 4 æ%C in a
T he r mo  Sc i e n t i f i c So r va l Mi c r o 1 7  R
refrigerated centrifuge. Subsequently, the
supernatants were separated from the pellets
into labelled Eppendorf tubes, stored at -20 o C
a n d u s e d f or  t he  d e t e r min a t io n  of
acetylcholinesterase (AChE), GST and catalase
activities as well as cell viability and TSH and
H

2
O

2
 levels. All the assays were carried out in

duplicate for each of the five replicates of FeSO
4

+ CuSO
4
 and resveratrol concentrations.

IN VIVO ASSAYS

Survival and negative geotaxis (climbing)
rate of flies

The flies were exposed to a diet mixed with
CuSO

4
 and FeSO

4
, namely FeSO

4
 0.5 mM,



32

FeSO
4 
1 mM, FeSO

4
 0.5 mM + CuSO

4 
0.5 mM

and FeSO
4
 1 mM + CuSO

4 
1mM for 21 days.

The survival rates were evaluated by daily
recording of fly mortality after which the data
were analysed.(14) We determined negative
ge ot a x i s a n d e me r ge nc e  r a t e  o f  D.
melanogaster offspring after being fed for a
period of seven days on a diet mixed with CuSO

4
,

FeSO
4
, and/or RES and EDTA, respectively, in

the positive control group and groups G1–G5,
as stated in a previous section.

EX VIVO ASSAYS

Sample preparation for biochemical assays
Drosophila melanogaster treated with

CuSO
4
, FeSO

4
, and RES for 7 days were

anaesthetized using CO
2
 gas. The fruit flies were

weighed and homogenized in 0.1 M potassium
phosphate buffer (pH 7.4, 1 mg: 10 μL buffer).
The homogenates were centrifuged at 4,000g
for 10 minutes at 4 °C in a Thermo Scientific
Sorval Legend Micro 7R centrifuge. The aliquots
of the supernatants were separated from the
pellets into Eppendorf tubes, kept at “20°C in a
freezer and were used for the estimation of
biochemical markers, ie. lipid peroxidation,
hydrogen peroxide (H

2
O

2
), total thiols (TSH),

glutathione (GSH), protein, and nitric oxide (NO,
nitrate and nitrite) levels as well as the activity
of  enzymes such as acetylcholinesterase,
catalase and glutathione-S-transferase (GST).
In addition, behavioural parameters such as
negative geotaxis were also determined.

BIOCHEMICAL ASSAYS

Protein determination
The principle of the assay is based on the

reaction of Cu+, produced by the oxidation of
peptide bonds, with Folin-Ciocalteu reagent (a
mi xt u r e  of  ph o sp hot u ngs ti c  a c i d  a n d
phosphomolybdic acid. The reaction mechanism
involves reduction of the Folin-Ciocalteu reagent
and oxidation of aromatic residues (mainly
tryptophan, also tyrosine). Cysteine residues in

p r o te in  p ro ba b l y a l s o  c o nt r i but e  t o  t he
absorbance seen in the Lowry assay. The
concentration of the reduced Folin reagent was
measured by absorbance at 750nm.

De t e r m ina t i o n o f  c a t al as e  an d
acetylcholinesterase activity

Catalase activity was determined by the
method descri bed by A ebi .(15) The reaction
mi xt u r e  co ns i s t e d o f  5 0 mM  po t a s si u m
phosphate buffer (pH 7.0), 300 mM H

2
O

2
 and

sample (1:50 dilution). The loss in absorbance
of H

2
O

2
 was monitored for 2 min at 240 nm and

thence used for the calculation of catalase
activity expressed as μmol of H

2
O

2
 consumed

per minutes per milligram of protein.
The reaction was carried out in 0.1 M

potassium phosphate buffer of pH 7.4, 1 mM
DTNB and 0.8 mM acetylthiocholine as the
initiator. The reaction was monitored for 2 min
(at 30 s intervals) at 412 nm. The enzyme activity
was determined as μmol of acetylthiocholine
hydrolysed/minute/mg protein. The activity of
acetylcholinesterase was determined according
to the method described by Ellman et al.(16)

Determination of total thiols, hydrogen
peroxide, and nitric oxide (nitrate/nitrite)
le ve l

The reaction mixture contained 510 μL of
0.1 M phosphate buffer (pH 7.4), 20 μL of
sample, 35 μL of 1 mM DTNB and 35 μL of
distilled water. Then, incubation was carried out
at room temperature for 30 min. The absorbance
was measured at 412 nm. Hydrogen peroxide
level was determined using the method of
Wolff.(17) The reaction mixture consisted of FOX
1 (10 ml of 100 mM xylenol orange, 50 ml of
250 mM ammonium ferrous sulphate, 10 ml of
100 mM sorbitol, 5 ml of 25 mM H

2
SO

4
 and 30

ml of distilled water) and was reacted with the
sample. After 30 min incubation at room
temperature, the absorbance was measured at
560 nm and the values were extrapolated from
the standard curve and expressed in micromole
per milligram (μm/mg) protein.

Igharo, Ebaluegbeifoh, Aikpitanyi-Iduitua. et al                                                            Drosophila melanogaster



33

Univ Med                                                                                                                                                             Vol. 42 No. 1

Nitric oxide (nitrate and nitrite) level was
estimated according to the method of the Griess
reaction. 250 μL of sample was incubated with
250 μL of Griess reagent [0.1 % N-(1-naphthyl)
ethylenediamine di hydrochloride; 1%
sulfanilamide in 5% phosphoric acid; 1:1 ratio] at
room temperature for 20 min. The absorbance
was measured spectrophotometrically at 550 nm
(OD 550) and nitrite concentration was quantified
by comparison with the OD 550 of a standard
sodium nitrite solution of known concentration.

Determination of glutathione S-transferase
activity

The activity of GST was quantified based
on the method of Habig and Jakoby (18) where 1-
chloro-2, 4-dinitrobenzene (CDNB) was used as
substrate. The reaction mixture contained 270 μL
of a solution made up of 20 μL of 0.25 M
potassium phosphate buffer, pH 7.0, with 2.5 mM
EDTA, 10.5 μL of distilled water and 500 μL of
0.1 M GSH at 25 °C),10 μL of 25 mM CDNB
and 20 μL of sample (1:5 dilution). The mixture
was monitored for 5 min (at 10 s intervals) and
absorbance was read  at 340 nm using a
spectrophotometer.

Determination of lipid peroxidation
Lipid peroxidation was estimated by

measuring the formation of thiobarbituric acid
reactive substances (TBARS) following the
method of Varshney and Kale. (19) Under acidic
condition, malondialdehyde (MDA) produced
from peroxidation of membrane fatty acids and
food products react with the chromogenic reagent,
2-thiobarbituric acid (TBA). A pink coloured
complex is generated and absorbance is read at
532 nm.

Determination of reduced glutathione level
The reduced glutathione (GSH) level was

measured according to the method of Beutler et
al. (20) The reduced form of glutathione comprises
in most instances the bulk of cellular non-protein
sulphhydryl groups. This technique depends on
the development of a relatively stable (yellow)

colour when 5´, 5´-dithiobis-(2-nitrobenzoic acid)
(Ellman’s reagent) is added to sulphhydryl
compounds. The chromophoric product resulting
from the reaction of Ellman’s reagent with the
reduced glutathione is measured at 412nm.

Estimation of glutathione (GSH) content
Glutathione (GSH) content was determined

colorimetrically using Ellman’s reagent (DTNB)
according to the procedure described by Jollow
et al.(21) The supernatant was precipitated with
4% sulphosalicylic acid (4%) in the ratio of 1:1.
The samples were preserved at 4 æ%C for 1 h
and then subjected to centrifugation at 5000 rpm
for 10 min at 4 æ%C. The assay mixtures
consisted of 550 µl of 0.1 M phosphate buffer,
100 µl of supernatant and 100 µl of DTNB. The
OD was read at 412 nm and the results were
expressed as moles of GSH/gram tissue.

Statistical Analysis
Data were expressed as mean  standard

error of mean. Treated and control groups were
compared using One-way ANOVA followed by
Tukey’s post hoc test. In all the groups,
differences with a p-value < 0.05 were considered
statistically significant.

RESULTS

Survival rate and selected biochemical
markers af ter exposure to fe rrous and
copper sulphate induced oxidative stress in
Drosophila melanogaster

Figure 1 shows the effects of ferrous and
copper sulphate on the survival biochemical
markers in of D. melanogaster. All doses of
FeSO

4
 and CuSO

4
 induced a toxic effect thus,

reducing the survival of flies (Figure 1). At varied
concentration, FeSO

4
 and CuSO

4
 significantly

(p<0.05) depleted T-SH, GST, GSH levels and
catalase activities except 1mM FeSO

4
 where

there was no significant difference for both GST
and catalase after 7 days of treatment when
compared to the control group (Figure. 1B, 1C,
1E and 1G) (p>0.05). Furthermore, significant



34

(a) (b)

(c) (d) (e)

(f)

(f)
(g)

Figure.1. Effects of FeSO
4
 and CuSO

4
 on survival rate and biochemical parameters in D. melanogaster. Data

are presented as Mean ± SE of 40 flies/ vial with 5 replicates per treatment group. Significant differences
when compared with the control group are indicated by (p<0.05)

Igharo, Ebaluegbeifoh, Aikpitanyi-Iduitua. et al                                                            Drosophila melanogaster



35

Univ Med                                                                                                                                                             Vol. 42 No. 1

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36

increase was observed in NO (nitrate and nitrite,
Figure. 1D) and H

2
O

2 
(Figure 1F) levels at varied

concentration of FeSO
4
 and CuSO

4
 when

compared to the control goup (p<0.05).

Resveratrol reverses ferrous and copper
sulphate induced oxidative stre ss in
Drosophila melanogaster

We assessed hydrogen peroxide and nitric
oxide levels in D. melanogaster after 7 days of
ferrous and copper sulphate exposure and
observed that RES restored ferrous and copper
sulphate -induced elevations of H

2
O

2
 (p < 0.05),

and NO levels (p<0.05). We also evaluated
selected markers of antioxidants such as TBARS,
TSH, GSH, GST, and catalase (Table 1). The
levels of total thiols (TSH) in Cu + Fe and RES-
exposed flies were not significantly different when
compared with the controls (p>0.05) as shown in
Table 1. In addition, RES reversed Cu + Fe-
induced inhibition of catalase activity and
improved GST activity that was inhibited by Cu
+ Fe in D. melanogaster (p<0.05). For TBARS,
a significant increase (p<0.05) was observed in
the flies when comparisons between the control
group and the various treatment groups were
made. However, flies that were treated with 60mg
RES /kg diet were closer in values to that of the
control group. It could be inferred that resveratrol
restored ferrous and copper sulphate-induced
elevated H

2
O

2
, NO and TBARS levels in

Drosophila melanogaster.

Compar ison of  amel ior ative impact of
resveratrol on negative geotaxis (climbing
rate), eclosion and selected biochemical
markers after exposure of D. melanogaster

Table 2 shows th e c omparison of
ameliorative impact of RES on climbing rate,
eclosion and selected biochemical marker after
exposure of  D. melanogaster to var ied
concentration of ferrous and copper sulphate after
seven days of treatment. There was a significant
reduction in the climbing rate (p<0.05) in Cu +
Fe challenged flies when compared with other
groups; however, resveratrol significantly

increased the climbing rate (p<0.05). A significant
reduction in the eclosion rate (Table 2, p<0.05) in
Cu + Fe challenged flies when compared with
the control and other groups was also observed.
However, resveratrol significantly increased the
eclosion rate of flies as shown in Table 2.

For  acetylcholine sterase enzyme, a
significant increase (p<0.05) was observed when
comparison between control and Cu + Fe
challenged flies were made. Interestingly, a
significant decrease (p<0.05) was observed in the
acetylcholinesterase activities of flies treated with
resveratrol. Therefore, resveratrol significantly
reduced the activities of acetylcholinesterase
after co-treatment with toxicants to a level
comparable to the control group as well as
improved the climbing rate and the eclosion rate
in Drosophila melanogaster.

Effects of ferrous sulphate (FeSO
4
) and

copper sulphate (CuSO
4
) on survival rate of

Drosophila melanogaster
The effect of ferrous sulphate (FeSO

4
) and

copper sulphate (CuSO
4
) on sur viva l of

Drosophila melanogaster is shown in Figure 2
below. Selected concentrations of FeSO

4 
and

combination of
 
FeSO

4 
and CuSO

4 
doses were used

as shown in Figure 2., 7 days exposure duration
was carried out and daily mortality was recorded
in the survival study. It was observed that FeSO

4

and CuSO
4 
induced toxic effect at all doses used

when compared with the control. Hence, FeSO
4

and CuSO
4 
reduced the survival rate of the flies.

DISCUSSION

This study showed that ferrous and copper
sulphate reduced the  sur vival rate of D.
melanogaster, suggesting that these metal ions
are harmful at 1mM. Excessive ROS formation,
which is an unavoidable by-product of cellular
breakdown, leads to oxidative damage to
macromolecules, increasing the susceptibility to
degenerative disorders.(22) The significant
increase in the levels of H

2
O

2
, nitric oxide, lipid

peroxidation (TBARS) with reduced total thiols

Igharo, Ebaluegbeifoh, Aikpitanyi-Iduitua. et al                                                            Drosophila melanogaster



37

Univ Med                                                                                                                                                             Vol. 42 No. 1

and glutathione as well as catalase inhibition across
flies treated with ferrous and copper sulphates
(1mM each) in this study suggests that the
formation of oxidants in the metal-treated flies
outpaced the antioxidant buffering capability of
the flies, resulting in ineffective oxidant
detoxification. Elevated nitric oxide (NO) serves
as a pro-inflammatory mediator.(14,23) Therefore,
both the ineffective oxidant detoxification and
inflammation directly reduced the survival rate
of the flies in the face of oxidative stress.

Remarkably, treati ng flie s with j ust
resveratrol (30 or 60 mg/kg) increased their
antioxidant and anti-inflammatory capacity, as
seen by the lowering of hydrogen peroxide, nitric
oxide, and lipid peroxidation, while increasing
catalase activity and elevating glutathione,
glutathione-S-transferase and total thiols. Our
study agrees with a previous study done by
Konyalioglu et al.,(24) which suggested that
resveratrol partially protected embryonic neural
stem cells from hydrogen peroxide-induced
toxicity. These findings also agreed with a
previous study carried out by Rege et al.,(25) which
postulated that resveratrol inhibited membrane
lipid peroxidation and decreased the toxic effects
produced by ROS. In  living organisms,
glutathione-S-transferases (GSTs) as detoxifying
enzymes catalyse the conjugation of GSH to
exogenous and endogenous electrophilic sites.(26)

Glutathione-S-transferase is a component of the
first line of antioxidant defence. It aids in the
prevention of free radical chain reactions and the
detoxification of harmful ROS when used in
conjunction with GSH-dependent enzymes.(27

Indeed, resveratrol corrected the depletion of
GSH and total thiols caused by copper and ferrous
sulphate in the flies. Total thiols (including non-
protein and protein thiols) protect the body from
oxidative stress.(28) In addition, resveratrol shielded
GST activity from copper and iron-induced
reduction, and the flies’ response to oxidative
stress and heavy metal detoxification was
activated. This finding led us to believe that
resveratrol’s protective mechanism against
copper and iron-induced toxicity is improved

further by the enhancement of thiol-containing
proteins other than the GSH molecule alone.

These findings agree with a previous report
that RES restored cigarette smoke extract (CSE)-
de pleted GSH levels by up regulation of
antioxidant genes such as glutamate-cysteine
ligase (GCL) through activation of nuclear
erythroid-related factor 2 (Nrf2) and also
quenched CSE-induced release of reactive
oxygen species.(29) The antioxidative effects of
RSV determined in the current study were
consistent with the results of a study by Li et
al.,(30) which indicate the role of RSV in protecting
against oxidative stress by decreasing ROS levels
and increasing the expression of CAT, GSH-Px,
GSH and T-SOD in obese-asthmatic rat models.
Increased catalase by resveratrol catalyses the
dismutation of H

2
O

2
 to molecular oxygen and

water to reduce oxidative stress-induced
toxicity.(31) The fact that resveratrol significantly
decreases ferrous and copper sulphate-induced
nitric oxide increase to levels comparable to the
control group, shows that the flies’ basal level of
NO, which is essential for physiological functions,
was restored. This finding is in line with Man et
al.,(32) who suggested that resveratrol inhibits the
acetylation of endogenous eNOS on lysine
residues in vitro and postulated that SIRT 1 gene
activation may play a fundamental role in
regulating endothelial NO and endothelium-
dependent vascular tone by deacetylating nitric
oxide synthase (eNOS). Also, Oh and Yun (33)

state that activation of SIRT 1 through resveratrol
in RINm5F cells (a pancreatic islet cell line) or
isolated rat islets also prevented the pro-
inflammatory stress induced by IL-1β and IFN-γ
by inhibiting iNOS and nitric oxide production
likely through the inhibition of the NFκB signalling
pathway. This observation also agrees with a
previous report that resveratrol is effective in
reducing the inflammatory status in vitro and in
vivo settings of neuroinflammation.(34,35)

The levels of TBARs, the end result of lipid
peroxidation, were also measured to support the
idea that ferrous and copper sulphate cause
oxidative stress. The copper- and ferrous-sulphate



38

treated groups had significantly higher levels of
TBARS, indicating ox idative stress, but
resveratrol treatment was able to ameliorate this
impact. This observation is in agreement with a
previous study, in that resveratrol prevents iron-
driven mitochondrial dysfunction by inhibiting
glycogen synthase kinase-3 beta activity (a
mechanism useful also to prevent tau hyper
phosphorylation),(36) and by reducing peroxidation
of lipoproteins and lipids through its activity as
scavenger. Therefore, the protective effects of
resveratrol on ferrous and copper sulphate-
induced oxidative stress can be related to its ability
to scavenge free radicals and restore the cellular
redox balance as well as control physiological
activities of the flies. Due to certain constraints,
elucidation of the possible mechanism by which
these metals induce their oxidative effects on
Drosophila melanogaster could not be
ascertained. However, the ability of resveratrol
in ameliorating these effects may present it as a
suitable antioxidant agent in the prevention of
heavy metal-associated diseases.

CONCLUSION

We demonstrated that FeSO
4
 and CuSO

4

were able to induce oxidative stress. Interestingly,
resveratrol was able to ameliorate free radical
generation. As a result, resveratrol protects
against copper and iron oxidant toxicity in vivo
when studied in combination. Because of the
greatly complex chemical composition and
multiple pharmacological effects of RES, further
research on its protective mechanism is required.

CONFLICT OF INTEREST

The authors declare that there is no conflict
of interests.

ACKNOWLEDGEMENT

The authors sincerely appreciate all staff
members of the Drosophila unit, Department of
Biochemistry, University of Ibadan.

CONTRIBUTORS

All authors take public responsibility for the
contents of the manuscript submitted to Universa
Medicina. The concept of this research was
developed by OGI and LOE. OGI, LOE, and
GAAII performed the animal experiments. HUO
and IBM worked on the concept and draft, and
prepared the manuscript. All authors have read
and approved the final manuscript.

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Igharo, Ebaluegbeifoh, Aikpitanyi-Iduitua. et al                                                            Drosophila melanogaster