Available online at www.sciencedirect.com
Assessment of the genotoxicity of imidacloprid and metalaxyl
in cultured human lymphocytes and rat bone-marrow
Marina Goumenou , Demetrios P. Matthopoulos
a Department of Environmental and Natural Resources Management, University of Ioannina, Agrinio Campus, Greece
b General Chemical State Laboratory, D Division of Athens, B Department, Athens, Greece
Received 2 January 2007; received in revised form 10 April 2007; accepted 20 May 2007
Abstract
Imidacloprid and metalaxyl are two pesticides that are widely used in agriculture, either separately, or in combination. These
agents were studied for their possible genotoxic effects with respect to the following cytogenetic end-points: (1) in vitro micronucleus(MN) formation and sister-chromatid exchange (SCE) induction in human lymphocytes and (2) in vivo micronucleus induction inpolychromatic erythrocytes (PCEs) of the rat bone-marrow. The results of the MN analysis indicate that MN frequencies aftertreatment with both pesticides, separately or as a mixture, do not significantly differ from those in the controls except after treatmentwith metalaxyl alone at 50 g/ml (p < 0.05). The results of the SCE analysis show that SCE frequencies after treatment withimidacloprid do not differ significantly from those in the controls. A statistically significant increase (p < 0.05) in SCE frequencyresulted from treatments with metalaxyl at 5, 10 and 100 g/ml and with the combination of imidacloprid and metalaxyl at 100and 200 g/ml. Finally, the in vivo micronucleus assay with rat bone-marrow polychromatic erythrocytes showed a statisticallysignificant effect upon separate treatments with imidacloprid and metalaxyl at doses of 300 mg/kg body weight (b.w.) (p < 0.01) orupon combined treatment with 200 mg/Kg b.w. (p < 0.001) and 400 mg/kg b.w. (p < 0.05). 2007 Elsevier B.V. All rights reserved. Keywords: Sister-chromatid exchange (SCE); Micronucleus (MN) test; Human lymphocytes; Rat bone-marrow; Genotoxicity; Pesticides
1. Introduction
Occupationally or incidentally, humans are exposed
not only to single pesticides, but also to pesticide mix-
The introduction of new chemicals in nature may be
tures. Limited in vitro studies have been conducted on
responsible for numerous negative effects in humans,
possible genotoxic side effects of pesticide mixtures
such as biochemical malfunctions or genetic instability
Pesticides are widely used noxious chemicals in
Imidacloprid and metalaxyl are two commonly used
agriculture, either separately or in mixtures, and they
pesticides applied either separately or as a mixture. In
invade the environment in large quantities. vivo results indicated that further studies are required toelucidate their genotoxic effects
Imidacloprid, a systemic chloro-nicotinyl insecticide
with soil, seed and foliar uses, blocks the nicotinergic
Corresponding author. Tel.: +30 26410 74148;
neuronal pathway, which is more abundant in insects
E-mail address: (D. Vlastos).
than in warm-blooded animals. It is a General Use
1383-5718/$ – see front matter 2007 Elsevier B.V. All rights reserved. G. Demsia et al. / Mutation Research 634 (2007) 32–39
Pesticide (GUP) classified by the US-EPA as a toxic-
2. Materials and methods
ity class II and class III agent Imidacloprid wasfound to induce DNA damage in a dose-related man-
ner in earthworms as well as to increase the frequency ofadducts in pesticide-treated calf thymus DNA, indicating
Blood samples were obtained from two healthy non-
smokers without previous known contact with pesticides. The
donors were between 20- and 25-year-old.
Metalaxyl, a systemic benzenoid fungicide used in
Imidacloprid (RDH 37894; purity, 99.9% by HPLC) and
mixtures as foliar spray for tropical and subtropical
metalaxyl (RDH 36153; purity, 99.9% by HPLC) obtained
crops, is a General Use Pesticide (GUP) classified by
from Pestanal Sigma–Aldrich, were dissolved in sterile dis-
the US-EPA as a toxicity class III agent is
tilled water at defined concentrations either as pure substances
not considered genotoxic However, a significant
or in 1:1 mixtures. The test concentrations are below the lim-
dose-dependent induction of chromosomal aberrations
its of solubility for imidacloprid metalaxyl
in cultured human peripheral blood lymphocytes was
derived from our preliminary studies, while they correspond to
observed after high-dose treatments, while in vivo
administration of 75–300 mg/kg b.w. to mice did notresult in any significant change in the frequency of
2.2. Micronucleus (MN) test in human lymphocytes in
micronuclei (MN) in the polychromatic erythrocytes
The genotoxic and mutagenic activities of cer-
Whole blood (0.5 ml) was added to 6.5 ml Ham’s F-10
tain pesticides have been studied both in in vitro
medium (Invitrogen), 1.5 ml foetal calf serum (Invitrogen)and 0.3 ml phytohaemagglutinin (Invitrogen) to stimulate cell
and in vivo cytogenetic test systems such as the
division. Cultures were incubated at 37 ◦C for 72 h. The appro-
cytokinesis-block micronucleus (CBMN) test and the
priate chemicals were added 41 h after the start of the culture
sister-chromatid exchange (SCE) assay in human lym-
at final concentrations of 0.1, 1, 5, 10, 50 and 100 g/ml in
phocytes in vitro and the micronucleus test on rat
separate treatments and of 10, 25, 50, 100 and 200 g/ml in
bone-marrow cells after in vivo exposure of the animals
mixed treatments. Mitomycin-C (Sigma) at a final concen-
tration of 0.5 g/ml served as positive control. Three hours
The CBMN assay in human lymphocytes devel-
after the addition of the pesticides, i.e. at 44 h post-culture
oped by Fenech and Morley cytochalasin-B,
initiation, 6 g/ml cytochalasin-B (Sigma) was added. Cells
an inhibitor of actin polymerisation, which pre-
were collected by centrifugation at 72 h, fixed with freshly
vents cytokinesis while permitting nuclear division
made methanol/acetic acid (Riedel-de Haen/Merck) mixture
As a result, binucleated (BN) cells are pro-
(3:1 v/v) after mild hypotonic treatment, and stained withGiemsa (Fluka) At least 1000 binucleate (BN) cells
duced, which are scored for the presence of MN
with preserved cytoplasm were scored, for each donor and for
each case, in order to calculate the frequency of MN. Standard
The SCE analysis has often been applied as a
cytogenetic assay for biomonitoring and genotoxic-
The cytokinesis block proliferation index (CBPI) is given
ity testing of potentially mutagenic and carcinogenic
by equation: CBPI = M1 + 2M2 + 3 (M3 + M4)/N, where M1, M2,
M3 and M4 correspond to the numbers of cells with one, two,
nation as well as alternative RAD-51 independent
three and four nuclei and N is the total number of cells
The CPBI was calculated by counting at least 2000 cells, to
determine possible cytotoxic effects.
The rodent bone-marrow MN test is the most widely
used short-term in vivo assay for the identification of
2.3. Sister-chromatid exchange (SCE) assay in human
genotoxic effects such as chromosome damage and ane-
uploidy associated with mutagenesis and carcinogenesis
Lymphocyte cultures from one healthy donor were set up
as described for the MN assay. At the start of the culture,
The present work focuses on the in vitro and in
5-bromodeoxyridine (5-BrdU) (Sigma) was added at a final
vivo analysis of genotoxic effects of imidacloprid and
concentration of 7.5 g/ml. The appropriate chemicals were
metalaxyl, as single agents and in combination, using
added 48 h after the initiation of the cultures at final con-
cytogenetic tests such as the cytokinesis-block micronu-
centrations of 0.1, 1, 5, 10, 50 and 100 g/ml in separate
cleus assay and sister-chromatid exchange analysis in
treatments and of 10, 25, 50, 100 and 200 g/ml in mixture
human lymphocytes in vitro and the micronucleus test
treatments. Mitomycin-C (Sigma) at a final concentration of
0.1 g/ml served as positive control. Cultures were incubated
G. Demsia et al. / Mutation Research 634 (2007) 32–39
in the dark at 37 ◦C for 72 h and demecolcine (Gibco) at a final
reason they can be distinguished from mature, norchromatic
concentration of 0.3 g/ml was added 2 h before harvesting
erythrocytes (NCEs) by selective ribosome staining. In addi-
slight modification of the original Moorhead et al.
tion, 200 total (immature and mature) erythrocytes were
protocol was used for cell harvesting and chromosomal prepa-
scored for PCE frequency per animal and for each treatment
ration. Chromosome staining was performed according to the
fluorescence-plus procedure with minor modifications. Briefly, air-dried slides were immersed for 15 min in a solu-
tion of 0.5 g/ml Hoechst 33258 (Sigma) in Sorensen’s buffer,exposed for 30 min to UV radiation, washed and finally stained
The one-way ANOVA test and the Student’s t-test of the Ori-
with Giemsa (Fluka) solution in Sorensen’s buffer, pH 6.8, for
gin 7.0 software (OriginLab Corporation, Northampton, USA)
were applied to statistically analyse the results obtained with
The frequency of SCE was evaluated in 50 second-division
metaphases for each treatment. Calculating the replicationindex (RI) from 200 metaphases was the criterion for thedetermination of possible cytotoxic effects. The RI was given
3. Results
by equation: RI = M1 + 2M2 + 3M3/N, where M1, M2 and M3denote those metaphases corresponding to first, second and
Cytogenetic end-points such as CBMN and SCE
third or subsequent divisions, and N is the total number of
induction in human lymphocytes in vitro and the in vivo
MN formation in rat bone-marrow were used to evaluatethe genotoxic effects of imidacloprid and metalaxyl. 2.4. Micronucleus (MN) test in rat bone-marrow in vivo3.1. Micronucleus test in human lymphocytes in
Healthy male Wistar rats, 6 weeks of age and weighing
138 ± 1.54 g were obtained from the Pasteur Institute, Athens,Greece and housed in groups of five in plastic chambers under
shows the results obtained with peripheral
controlled temperature and light conditions, having free access
blood lymphocyte cultures treated with imidacloprid and
to standard rodent chow and water. The rats were treated orally
metalaxyl, separately or in combination.
either with separate or combined doses of imidacloprid and
Neither separate nor mixed imidacloprid and met-
metalaxyl. The Student’s t-test did not reveal statistically sig-
alaxyl treatments were able to induce a statistically
nificant differences in animal weights between study groups.
The pesticides were tested at three different doses, cor-
significant increase in the frequency of MN and BNMN,
responding to 22, 45 and 67% of the published LD
except the concentration 50 g/ml of metalaxyl. Anal-
for imidacloprid (450 mg/kg) and 11, 22 and 45% of the pub-
ysis of the CBPI indicated a minor decrease at all test
concentrations (except the imidacloprid concentration of
received either imidacloprid at 100, 200 and 300 mg/kg b.w. or
0.1 g/ml) compared with the controls, but the level of
metalaxyl at 75, 150 and 300 mg/kg b.w., or the 1:1 mixture of
significance was not reached. In addition, in the case of
these two agents at 150, 200 and 400 mg/kg b.w. Cyclophos-
mixed pesticide treatments, a twofold increase in MN
phamide (Sigma) at 20 mg/kg b.w. was used as the positive
and BNMN frequencies was observed at concentrations
control. At 24 h after the treatment, animals were anaesthetized
of 100 and 200 g/ml. However, these effects were also
with CO2 and sacrificed by cervical dislocation in accordance
with the approved procedure of the Ioannina University Insti-tutional Animal Care and Use Committee.
The micronucleus (MN) test was performed as described by
3.2. Sister-chromatid exchange analysis in human
Schmid with minor modifications. Bone-marrow, from
both epiphyseal cartilage-decapitated femurs, was collectedby mild centrifugation in 5 ml centrifuge tubes containing
2 ml of foetal calf serum (Invitrogen). Pelleted marrow cells
blood lymphocyte cultures treated with imidacloprid and
were washed by centrifugation at 1000 rpm for 3 min in 4 ml
metalaxyl in separate or mixed treatments.
foetal calf serum, resuspended in a small amount of serum,
The results of SCE analysis showed that imidacloprid
spread on clean microscope slides, air-dried, methanol fixed,
did not significantly alter SCE frequencies compared
and finally stained with May-Grunwald (Fluka) followed by
with the control. Statistically significant differences
To determine MN frequencies, 2000 polychromatic ery-
(p < 0.05) – without a dose–response pattern – in compar-
throcytes (PCEs) were analysed per animal and for each
ison with the control in the SCE frequencies were seen
treatment. Polychromatic erythrocytes are developmentally
at metalaxyl concentrations of 5, 10 and 100 g/ml, as
immature erythrocytes that still contain ribosomes. For this
well as at the 100 and 200 g/ml mixed treatments. G. Demsia et al. / Mutation Research 634 (2007) 32–39
Table 1Frequencies of binucleated micronucleated cells (BNMN) and micronuclei (MN), as revealed after Giemsa staining, induced in vitro in humanlymphocyte cultures in separate or mixed treatments with imidacloprid and metalaxyl
BN, binucleated cells; BNMN, micronucleated binucleated cells; MN, micronuclei; CBPI, cytokinesis block proliferation index; MF(‰) ± S.E.,mean frequencies (‰) ± standard error; ap < 0.05; bp < 0.05 1, 2, 3; cp < 0.0011, 2, 3 (one-way ANOVA test). 3.3. Micronucleus analysis in rat bone-marrow
PCEs in total erythrocytes (PCEs and NCEs) in cyto-
genetic assays, such as the in vitro cytokinesis-blockmicronuclei and SCE analysis in human lymphocytes
The results obtained with PCEs from orally treated
and the in vivo MN test on rat bone-marrow. Regard-
rats are shown in with different separate or
ing the cytotoxicity index in all cytogenetic end-points
combined doses of imidacloprid and metalaxyl.
considered (no statistically significant dif-
The results of the MNPCE analysis indicate statisti-
ferences were observed between controls and metalaxyl-
cally significant effects up to 300 mg/kg b.w. (p < 0.01)
or imidacloprid-treated cultures or animals.
imidacloprid and metalaxyl when given separately, andup to 200 mg/kg b.w. (p < 0.001) and 400 mg/kg b.w. 4. Discussion
(p < 0.05) when given in combination.
The reported control frequencies of MN, SCEs and
Pesticides form an important group of man-made
MNPCEs are in accordance with the published values for
noxious chemicals. Their potential synergistic or antag-
the cytogenetic end-points used here In addi-
onistic side effects in humans have not yet been
tion, the MN and SCE frequencies after treatment with
extensively investigated. Bolognesi viewed cyto-
mitomycin C as positive control as well as the
genetic biomarkers in pesticide-exposed workers and
MNPCEs frequencies after treatment with cyclophos-
reported indications of dose-dependent effects with
phamide as positive control consistent with the
increasing duration or intensity of exposure. Further-
literature and authenticate our experimental procedure,
test animal response, and treatment observations.
chemicals might be dependent on the dose and dose
The cytotoxic effects of imidacloprid and metalaxyl
rate at which the chemicals reach the target tissues.
were evaluated by the determination of CBPI, RI and (%)
This possible variable response to the level, length and
G. Demsia et al. / Mutation Research 634 (2007) 32–39
Table 2Frequencies of sister-chromatid exchange (SCE) induced in human lymphocyte cultures in vitro in separate or mixed treatments with imidaclopridand metalaxyl
MF ± S.E., mean frequencies ± standard error; RI, replication index; ap < 0.05; bp < 0.00011, 2, 3 (t-test).
Table 3Frequencies of micronuclei in polychromatic erythrocytes (PCEs), induced in rat bone-marrow cells treated in vivo with imidacloprid and metalaxyl
MF(‰) ± S.E., mean frequencies(‰) ± standard error; MNPCEs, micronucleated polychromatic erythrocytes; CP, Cyclophosphamide; ap < 0.01;bp < 0.001; cp < 0.05 (t-test). G. Demsia et al. / Mutation Research 634 (2007) 32–39
frequency of exposure to various pesticides could be
Taking into consideration the suggestions of Bolog-
correlated to the variable response observed in other
mammalian tissues to other environmental stressors
observed genotoxic effects may be the result of either
such as heat treatment or viral infection In
the dose applied to the test system and/or the rate by
an attempt to further address these issues we focused
which the test pesticides reach the target tissue.
on the possible synergistic effect of imidacloprid and
Our results do not indicate a clear-cut genotoxic effect
of imidacloprid and metalaxyl when tested separately
In a study of the potential in vivo genotoxic effects of
on human lymphocytes in vitro or on rat bone-marrow
imidacloprid and metalaxyl on occupationally exposed
in vivo. In treatments with a mixture of these pesticides
farmers, smokers and non-smokers, statistically sig-
we observed statistically significant differences at the
nificant differences were observed in MN frequencies
highest test concentrations for both SCE and MNPCEs.
between controls and exposed smokers, as well as
This effect was not dose-dependent. However, Dolara
between controls and all the exposed farmers
et al. an in vitro dose-dependent induction
observations provided the basis for the idea that the
of SCE in human lymphocytes exposed to a mixture of
observed effects may have resulted from an interaction
four different pesticides, while no significant increase in
SCEs was seen when the various pesticides were tested
Significant differences in MN and SCE frequen-
separately. This latter result is in agreement with our
cies were observed in in vitro studies when 0.1 and
observations when we tested imidacloprid and metalaxyl
0.5 g/ml of imidacloprid were added to human lym-
alone. In addition, Bianchi-Santamaria et al.
phocytes at 24 h after the start of the culture Our
a dose-independent induction of MN in human lympho-
results show that MN and SCE frequencies after treat-
cyte cultures with mixtures of various phytochemicals
ment with imidacloprid are not different from the control
at environmental concentrations. Taking into considera-
values. However, the differences between our MN and
tion that to some extent controversial results have been
SCE control values and those in the above-mentioned
reported on the genotoxicity of the various agrochemi-
study may explain the controversial results in MN and
cals, tested alone or in combination, it appears important
to conduct studies using different genotoxicity tests in
order to reach to a comprehensive understanding of their
1000 g/ml) resulted in a significant dose-dependent
induction of CAs in human lymphocytes Treat-
In conclusion, our study revealed an increase in MN
ments with metalaxyl doses lower than those mentioned
frequency in human lymphocytes as well as in rat bone-
above did not result in a statistically significant increase
marrow cells and an induction of SCEs in cultured human
in MN frequencies. On the other hand, a significant
lymphocytes treated with a mixture of imidacloprid and
increase in SCE frequency – without a dose–response
metalaxyl. These observations are indicative of a possi-
pattern – was observed after treatment with metalaxyl.
ble synergistic effect of these two pesticides.
In our in vivo study no effects were observed in
single pesticide treatments up to the concentration of
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