Journal of Ethnopharmacology 103 (2006) 433–438
Chemical and biological investigations of a toxic plant from Central
Africa, Magnistipula butayei subsp. montana
C. Karangwa a,b , V. Esters a , M. Frédérich a , M. Tits a , J.N. Kadima b , J. Damas a ,
A. Noirfalise a , L. Angenot a,∗
a
Natural and Synthetic Drugs Research Centre (C.P.S.N.S.), Department of Pharmacy, Faculty of Medicine,
University of Liège, Avenue de l’Hôpital 1, B36, 4000 Liège 1, Belgium
b Laboratory of Pharmacology and Toxicology, Department of Pharmacy, Faculty of Sciences and Technology,
National University of Rwanda, BP 117 Butare, Rwanda
Received 26 May 2005; received in revised form 10 August 2005; accepted 16 August 2005
Available online 19 September 2005
Abstract
Magnistipula butayei subsp. montana (Chrysobalanaceae) is known, in the Great Lakes Region, to possess toxicological properties. In this
paper, we investigated the acute toxicity (dose levels 50–1600 mg/kg) of its aqueous extract, administered orally to adult Wistar rats.
This study demonstrated that the freeze-dried aqueous extract (5%, w/w) possesses high toxicity. The extract caused hypothermia, neurological disorders, including extensor reflex of maximal convulsive induced-seizures at about 2 h after the administered dose, and death occurred
(LD50 = 370 mg/kg) in a dose dependent manner.
Blood parameter evaluation revealed slight variations, but these might not have clinical relevance. Histological examination of internal organs
(lungs, liver, heart and kidneys) did not reveal any abnormality in the treated group compared to the control. Therefore, it can be concluded that
Magnistipula butayei subsp. montana aqueous extract, given orally, is toxic and that its target is the central nervous system.
General phytochemical screening revealed that the plant did not contain significant amounts of products known to be toxic, such as alkaloids
or cardioactive glycosides, but only catechic tannins, amino acids, saponins and other aphrogen principles in the three parts of the species (fruit,
leave and bark).
© 2005 Elsevier Ireland Ltd. All rights reserved.
Keywords: Magnistipula butayei subsp. montana; Chrysobalanaceae; Convulsions; Acute toxicity; Hypothermia; Blood parameters
1. Introduction
Magnistipula butayei subsp. montana (Hauman) F. White
(Chrysobalanaceae) is an evergreen and perennial tropical rainforest tree, which induces severe poisoning of animals and
humans in South West Rwanda, North Burundi and East Congo
(Desouter, 1991).
According to our ethnobotanical investigations in three
Rwandan provinces, people in the Nile-Congo Crest (Cyangugu
and Kibuye: 2100–2200 m) use a decoction of tree trunk bark
and root, while in the Crest borders (Butare: 1500–1900 m),
Abbreviations: DW, distilled water; MBMAE, Magnistipula butayei subsp.
montana aqueous extract; RBC, red blood cells; WBC, white blood cells
∗ Corresponding author. Tel.: +32 4 366 43 30; fax: +32 4 366 43 32.
E-mail address: L.Angenot@ulg.ac.be (L. Angenot).
0378-8741/$ – see front matter © 2005 Elsevier Ireland Ltd. All rights reserved.
doi:10.1016/j.jep.2005.08.019
they widely use the leaf and fruit for killing wild animals
(rats, dogs and other predators) and for poisoning humans
(Karangwa, 2002). The plant is locally named Umutamasha,
Intambasha, Ururamba (Kirundi) (Karangwa, 2002) Umuganza
or Umusarwe (Tervuren Museum, Brussels, Belgium). However, its toxicity has not yet been studied; only reports from some
ethnobotanists (Troupin, 1978; Desouter, 1991) have related its
toxicity.
Indeed, in the Congolese equatorial forest (Central Africa),
local people use the tree bark of an other species, Magnistipula
sapinii De Wild., in ordeal poison (Staner and Boutique,
1937).
The present study was initiated to evaluate the toxicity of the
aqueous extract from Magnistipula butayei subsp. montana to
substantiate the folklore claims and to detect active principles in
order to find an antidote.
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C. Karangwa et al. / Journal of Ethnopharmacology 103 (2006) 433–438
2. Materials and methods
2.1. Plant material
Mature tree trunk bark from Magnistipula butayei subsp.
montana was collected in Binogo (Rusenyi district, Kibuye
province, Rwanda) in August 2001. Binogo is a village located
in the mountains of the Nile-Congo Crest near the National
Reserve of Nyungwe. The Belgian taxonomist, Georges Troupin
(1978), had previously botanically authenticated and deposited
some specimens (voucher numbers 15981, 16319, 924, 16035)
at the Herbarium of the Institute of Scientific and Technological
Research, Butare, Rwanda. Referring to these specimens, we
collected and deposited other voucher specimens (Karangwa,
5108) of this plant at the same institute, as well as at the National
Botanic Garden of Belgium (Meise) and at the Laboratory of
Pharmacognosy, Department of Pharmacy at the University of
Liège.
test sheet by Malone and Robichaud (1962). The Hippocratic
screening test is commonly used in the preliminary screening of medicinal plants to detect interesting pharmacological
activity. Fourty-two adult Wistar rats were utilised and grouped
into seven groups. Six rats constituted each group. They were
deprived of food, but not water, 12 h before starting the experiments. Six groups were respectively treated with six doses (50,
100, 200, 400, 800 and 1600 mg/kg per os (p.o.) of the MBMAE.
The one control group received an equal volume of the distilled
water vehicle (4 ml/kg).
Observations of toxic symptoms were made and recorded
systematically at 1, 2, 4 and 6 h after administration. Finally,
the number of survivors was noted after 12 h and these animals
were then maintained for a further three days, with observations
being made daily. All surviving animals were euthanized with a
large dose injection of pentobarbital (100 mg/kg) (Sigma).
2.5. Monitoring of body temperature
Mature bark was dried in an air-conditioned room and
crushed to obtain a coarse powder (sieve: 1 mm). The extraction was performed by macerating 500 g of crude powder of
MBM in 5 l distilled water (DW) and percolating through a
fresh cotton bed at room temperature for 24 h. The percolate
was freeze-dried (Alpha Chriss® ) for 36 h and the resulting powder (yield ±5%, w/w) was immediately stored in polyethylene
containers.
The lyophilised residue was extemporaneously dissolved in
water for biological assays.
Twenty-four adult male Wistar rats were utilised and grouped
in four experimental groups. Each group consisted of three
treated and three control rats. The treated rats respectively
received four doses (50–1600 mg/kg) of the MBMAE and the
controls received the vehicle (4 ml/kg). The rectal temperature of
each animal was registered immediately before and after administration of an oral single dose of either the extract or the solvent
(Table 2).
The probe of a digital thermometer (Ama-Digit® ) was introduced into the rectum of the rat to a constant depth of 2.5 cm.
Controls served as a reference point for the determination of
temperature changes.
2.3. Animal tests
2.6. Parameters: blood analysis
All experimental procedures were carried out in strict accordance with the European Commission Directive (86/609/EEC)
for Guidelines in the Care and Use of Laboratory Animals and
were approved by the Ethical Committee for protection of animals at the University of Liège, Belgium.
Adult Wistar rats, weighing between 200 and 300 g, were
utilised in various experiments. The animals were all purchased
from the Animal Centre of the University of Liège, Belgium.
The animals were kept in an animal room where they were maintained under a controlled temperature (23 ± 1 ◦ C), as well as on
a 12 h light/12 h dark cycle, and were provided with food and/or
water ad libitum. All treated animals received the Magnistipula
butayei subsp. montana aqueous extract (MBMAE) in a single
oral dose (expressed as milligrams of the extract per kilogram
of rat) by gavage using a feeding needle. Controls received the
same solvent.
The adult male Wistar rats group, fasted overnight, were
treated with 800 mg/kg of the MBMAE; the other group (control) received the solvent (4 ml/kg). Two hours later (considered
as an elapsed-time of convulsions according to our primary
tests), they were anaesthetised for blood collection from a common carotid artery. Blood samples were collected into:
2.2. Preparation of the aqueous extract for biological tests
2.4. Acute toxicity study
The acute toxicity profile was assessed by monitoring convulsions, mortality (determined as LD50 by statistical software
Graph Pad Prism, Version 3.0) and other behavioural variations
in the same animals, as described in the Hippocratic screening
• centrifuge tubes with 2 ml of 20% EDTA for white blood cell
(WBC) and red blood cell (RBC) counts and for haemoglobin
estimation;
• centrifuge tubes with 3 ml of citrate for coagulating testing;
• heparinised tubes (5 ml) for biochemical determination of
electrolytes (Na, K, Cl and Ca), glucose and albumin concentration in rats.
A blood analysis (for both haematology and biochemistry
purposes) was carried out within 2 h.
The haematological parameters (total red blood cells and
leukocytes (Potron et al., 1990) and haemoglobin (International
Committee for Standardization in Haematology, 1978)) were
determined by using an autoanalyser (ADVIA 120 Haematology System, Bayer Diagnostics), and coagulation testing (Quick,
1935) by using an automated BCS BEHRING-DADE.
C. Karangwa et al. / Journal of Ethnopharmacology 103 (2006) 433–438
435
Table 1
Percentage of mortality, toxicity signs and symptoms observed in rats after the oral administration of MBMAE (N = 6, number of rats per set)
Doses
Tonico-clonic convulsive seizures
Mortality
n
Intensity (%)
Latency (h)
Episode duration
(min)
n′
Other toxic symptoms
Percent
DW (control) 4 ml/kg
MBMAE 50 mg/kg
MBMAE 100 mg/kg
MBMAE 200 mg/kg
0/6
0/6
0/6
1/6
0
0
0
+
0
0
0
100
0
0
0
±3.0
0
0
0
0.5–2
0
0
0
1/6
0
0
0
16.7
0
0
0
12–72
MBMAE 400 mg/kg
6/6
++
100
±2.5
0.5–2
3/6
50.0
6–72
MBMAE 800 mg/kg
6/6
+++
100
±2.0
0.5–2
6/6
100.0
5–48
MBMAE 1600 mg/kg
6/6
+++
100
±1.5
0.5–2
6/6
100.0
2–48
Latency (h)
None
None
Asthenia
Imm. star., trem., LMS,
T/C conv.seiz.
Imm. star., trem., LMS,
T/C conv.seiz.
Imm. star., trem., LMS,
T/C conv.seiz.
Imm. star., trem., LMS,
T/C conv.seiz.
LD50 = 370 mg/kg. Imm.: immobilisation; star.: staring; trem.: tremor; LMS: limbic motor seizures (automatisms: bobbing, nodding, chewing; rearing and loss of
balance); T/C conv. seiz.: tonico-clonic convulsive seizures; n = ratio of convulsing rats; n′ = ratio of dead rats. 0, +, ++, +++: the rating marks, 0: negative; +: weak;
++: strong; +++: very strong; ±: approximate. MBMAE: Magnistipula butayei subsp. montana aqueous extract; DW: distilled water.
The biochemical parameters, including glucose (Banauch et
al., 1975), albumin (Meites, 1989) and electrolytes (Meyerhoff
and Opdyke, 1986), were determined enzymatically using specific kits and measurement of optical density at the corresponding wavelength with a spectrophotometer [MODULAR: module
ISE (electrolytes) and Module P (glucose, albumin and P)].
2.7. Tissue analysis
Two adult male Wistar rats, fasted overnight, were treated
with 800 mg/kg of the MBMAE; two controls received the
solvent. Two hours later, they were anaesthetised (Nembutal®
100 mg/kg) and euthanised for tissue studies. Liver, lungs, heart
and kidneys were removed and blotted free of blood in buffered
formalin.
2.8. Phytochemical screening
Standard screening tests using conventional protocol
(Angenot, 1970; Evans, 1996; Wagner and Bladt, 1996) were
utilised for detecting the major components (alkaloids, tannins,
flavonoids, amino acids, etc.).
2.9. Statistical analysis
The results were expressed as mean ± standard deviation
(S.D.). Differences between control and experimental groups
were assessed by the Student’s t-test. P-values of less than 0.001,
0.01 and 0.05 were respectively considered to be highly significant, very significant and significant.
3. Results
3.1. Acute toxicity and behavioural observations
3.1.1. Acute toxicity
Magnistipula butayei subsp. montana aqueous extract
(MBMAE) administered to rats provoked convulsive seizures
prior to death in a dose dependent manner. The doses of 50
and 100 mg/kg did not induce any visible seizures or death. On
the other hand, the doses of 200–1600 mg/kg were lethal and
caused death with variable latency from 2 to 72 h (Table 1).
The LD50 was estimated to be 370 mg/kg body weight (BW).
Extract induced an initial arousing and then prolonged reduction
of motor activities followed by tonic jerks, followed finally by
convulsions. A range of convulsive responses was observed: (i)
tonic or clonic events, mainly confined to the head or the head
and forelimbs, occasionally with nodding and rearing, but with
the animal maintaining its stance (defined herein as a restricted
seizure), (ii) tonic or clonic events involving the head and all
limbs associated, sometimes with a loss of postural control
(defined herein as a generalised seizure). Involvement of the
trunk and hindlimbs, therefore, distinguished a restricted from
a generalised seizure.
Generalised seizures began in the same way as restricted
seizures, with head and forelimb clonic activity, and this
was immediately followed by involvement of the trunk and
hindlimbs, finishing in the opisthotonus position. Restricted
seizures occurred more frequently than generalised seizures.
With the doses of 200 and 400 mg/kg, restricted seizures
were generally observed, whereas generalised seizures occurred
with high doses (800 and 1600 mg/kg). The episode duration of generalised seizures was 30 s–2 min. The intensity and
latency of convulsions depended on the administered dose
(Table 1).
3.1.2. Behavioural observations
The MBMAE was found to provoke neurological disorders in
a dose dependent manner. Besides convulsive seizures and death,
the doses of 200–1600 mg/kg BW caused dose-related immobilisation, staring, irregular breathing, tremor, automatisms (bobbing, nodding, chewing), loss of screen grip and righting reflex
and convulsive seizures prior to death (Table 1). The intensity and elapsed time of signs and symptoms were respectively
dependent on the administered dose. Thus, the small doses of
50 and 100 mg/kg did not show any visible change.
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C. Karangwa et al. / Journal of Ethnopharmacology 103 (2006) 433–438
Table 2
Effect of MBMAE on body temperature in rats (N = 3, number of rats per set)
Rectal temperature (◦ C) before and after treatment
Treatment
0 min
30 min
60 min
120 min
(A) DW (control) 4 ml/kg
MBMAE (50 mg/kg)
Control (4 ml/kg)
MBMAE (100 mg/kg)
Control (4 ml/kg)
MBMAE (800 mg/kg)
38.13 ± 0.15
37.73 ± 0.46
38.77 ± 0.64
38.30 ± 0.64
38.43 ± 0.21
37.27 ± 0.12
38.7 ± 0.17
38.33 ± 0.42
38.03 ± 0.31
37.77 ± 0.68
38.77 ± 1.12
38.17 ± 0.47
37.7 ± 0.26
37.40 ± 0.10
37.30 ± 0.26
36.23 ± 0.83
38.80 ± 0.26
37.17 ± 0.15
38.47 ± 0.15
37.53 ± 0.32
37.13 ± 0.15
35.93 ± 0.32b
38.97 ± 0.76
34.87 ± 0.58a
(B) Control (4 ml/kg)
MBMAE (1600 mg/kg)
38.77 ± 0.60
38.33 ± 0.06
38.60 ± 0.17
37.57 ± 0.55
38.47 ± 0.06
34.73 ± 0.10a
37.93 ± 0.81
33.10 ± 0.10a
240 min
360 min
37.87 ± 0.32
31.93 ± 0.12a
38.03 ± 0.15
31.83 ± 0.55a
Each value represents mean ± standard deviation. (n = 3) of body temperature measurement in rats. MBMAE: Magnistipula butayei susp. montana aqueous extract.
(A) First measurement of body temperature (0–120 min). (B) Second measurement of body temperature (0–360 min). DW: distilled water.
a P < 0.001 compared with control values for the corresponding minutes.
b P < 0.01 compared with control values for the corresponding minutes.
3.2. Evaluation of body temperature
was a significant increase in phosphorus (P < 0.05) and glucose
(P = 0.05) detection.
Our experimental pharmacology study demonstrated that the
MBMAE caused a significant lowering effect on body temperature in treated rats compared with respective controls. This
effect occurred in a dose dependent manner. It was found
that MBMAE at a dose of 100 mg/kg BW caused significant hypothermia (P < 0.01) at 2 h following its oral administration (Table 2). This effect was early maximal at a dose
of 1600 mg/kg (P < 0.001), at 1 h following its administration and remained for at least 6 h (while the animal was still
alive).
3.4. Histological evaluation
Organs from rats treated with the MBMAE were macro- and
microscopically comparable to the controls.
Histopathological examination of tissues (liver, lungs, heart
and kidneys) from the Wistar rats indicated that there was no
detectable abnormality. No pathological alteration was detected.
The architecture of the internal organs was examined and their
cellular appearance was comparatively similar in both treated
and control groups.
3.3. Haematological and biochemical observations
3.5. Phytochemical screening
Haematological and biochemical results are respectively
described in Tables 3 and 4.
The haematological values of rats treated with the MBMAE
showed a slight significant increase in red blood cells (P < 0.05)
and white blood cells (P < 0.05) (Table 3). But, there were no significant differences in haemoglobin (HGB) estimation (P > 0.05)
from the controls.
In the blood chemistry analysis, including glucose, albumin,
coagulation time and electrolyte determination, no significant
changes occurred in the parameters (Table 4). However, there
Table 3
Haematological observations
Blood elements
Control
(NaCl 0.9%),
M ± S.D.
MBMAE
(800 mg/kg),
M ± S.D.
P-value
Significance
RBC (106 /l)
HGB (g/dl)
WBC (103 /l)
7.25 ± 1.22
13.0 ± 2.65
0.88 ± 0.44
7.58 ± 0.25
14.48 ± 0.35
2.16 ± 0.89
0.03
0.52
0.03
S
NS
S
Haematological values of rats treated with MBMAE (Magnistipula butayei
subsp. montana aqueous extract) in an acute toxicity; S: Significant values from
the control (P < 0.05). NS: non significant (P > 0.05). Data are expressed as
mean ± standard deviation. (n = 6). RBC: red blood cells; HGB: haemoglobin
and WBC: white blood cells.
The phytochemical tests revealed that Magnistipula butayei
subsp. montana contained neither cyanogenetic nor cardioactive
glycosides nor alkaloids. No significant amounts of terpens or
anthraquinones were detected. However, catechic tannins, leucoanthocyanins, amino acids and saponins (foam value) were
found in the three parts of the plant, with a high concentration
in leaves (Table 5).
Table 4
Biochemical observations
Blood elements
Control
(NaCl 0.9%),
M ± S.D.
Glucose (mg/dl)
Sodium (mmol/l)
Potassium (mmol/l
Calcium (mmol/l
Chlorides (mmol/l
Phosphorus (mg/dl)
Albumin (g/dl)
Prothrombin
time (inr)
0.85
157
3
1.53
130
31
21.5
1.36
±
±
±
±
±
±
±
±
MBMAE
(800 mg/kg),
M ± S.D.
0.18
1.35 ± 0.24
2.25
157.5 ± 3.26
0.57
3.2 ± 0.33
0.20
1.7 ± 0.20
11.86 123.16 ± 3.86
6.40
58.5 ± 26.26
5.68
24.3 ± 3.56
0.76
0.96 ± 0.03
P-value Significance
0.05
1.00
0.44
0.18
0.21
0.04
0.52
0.23
NS
NS
NS
NS
NS
S
NS
NS
Blood chemistry values from rats treated with MBMAE (Magnistipula butayei
subsp. Montana aqueous extract), controls: 4 ml/kg NaCl 0.9% in an acute toxicity. Data are expressed as mean ± standard deviation (n = 6) S: significant value
from the control (P < 0.05) and NS: non significant (P > 0.05).
C. Karangwa et al. / Journal of Ethnopharmacology 103 (2006) 433–438
Table 5
Phytochemical components
Chemical components
Leaf
Fruit
Bark
Alkaloids
Catechic tannins
Gallic tannins
Flavonoids
Anthocyanins
Leucoanthocyanins
Saponins (foam value/French Pharmacopoeia)
Cardiactive glycosides
Cyanogenetic glycosides
Anthraquinones
Amino-acids
−
++
−
++
+
++
++
−
−
−
+
−
+
−
−
−
+
++
−
−
−
+
−
+
−
−
−
+
+
−
−
−
+
Phytochemical screening of three parts of Magnistipula butayei subsp. montana
collected in August 2001 in mountains bordering the Congo-Nile Crest, West
Rwanda; −; +; ++: the rating marks, −: negative; +: weak; ++: positive.
4. Discussion and conclusion
Chemical products that act upon the central nervous system
(CNS) influence the lives of everyone, every day. These products
are invaluable therapeutically because they can produce specific
physiological and psychological effects (Goodman and Gilman,
1996). We tried here to elucidate the toxicity of a plant, Magnistipula butayei subsp. montana, traditionally used as a poison in
Great Lakes Region for its “inducement of tremor and death”.
The aqueous extract was used in these tests, since this form is
traditionally used by the local population.
The present study has shown that MBMAE elicits immobilisation, staring, tremor, facial and jaw clonus, loss of balance
and tonic and/or clonic convulsive seizures prior to death in Wistar rats. The convulsive seizures appeared in a dose dependent
manner, as did death. In addition to the behavioural alterations,
hypothermia was also observed. This probably indicates that
the aqueous extract contains substances that act upon the neurones of the hypothalamic area involved in body temperature
regulation (Bastidas Ramirez et al., 1998; Devi et al., 2003).
The loss of screen grip can be taken as an indication of skeletal muscle relaxant activity. The site of action of this activity
could be peripheral (at the neuromuscular junction) or central
(Kanjanapothi et al., 2004). It is possible that the CNS depression and paralysis of skeletal muscle, which are caused by the
MBMAE, tend to modify the response to neuronal disruption
and, as a result, hypothermia occurs (Kanjanapothi et al., 2004).
Although the hypothermia was statistically significant, it might
not have clinical relevance regarding convulsive seizures. Normally, there is a close relationship between seizures and body
temperature. High fever frequently induces febrile convulsions
in children (Lennox-Buchtal, 1974; Nelson and Ellenberg, 1990)
and hyperthermia-induced seizures have been reported in experimental models (McCaughram and Schetcher, 1982; Johnson et
al., 1985; Tancredi et al., 1992; Morimoto et al., 1996; Ahlenius et al., 2002). However, hypothermia is known to prevent or
reduce nervous damage (Traynelis and Dingledine, 1988; Maeda
et al., 1999; Sanchez-Mateo et al., 2002; Takei et al., 2004; Yager
et al., 2004). By contrast, the MBMAE acted by inducing convulsive seizures and lowering body temperature.
437
The respiratory failure and irregular breathing could also be
due to central or peripheral action. Centrally, the irregular breathing could be due to a CNS depression leading to convulsions,
whereas, peripherally, the failure could possibly be due to an
inhibitory action at the neuromuscular junction. The literature
shows that variations in some blood parameters can induce convulsive seizures: hypernatraemia (Türk et al., 2005), hypoglycaemia (Hogan et al., 1985) hypocalcaemia and, hypokalaemia
(Astrup et al., 1979; Traynelis and Dingledine, 1988). In
our results, haematological and biochemical blood parameters
showed values that lacked clinical relevance. The histopathological evaluation failed to reveal any abnormality that would
cause convulsive seizures. Nevertheless, behavioural alterations
supracited are good evidence that the MBMAE target is the central nervous system (Mraovitch and Calando, 1999). Therefore,
it can be concluded that MBMAE, given orally, is toxic with
LD50 = 370 mg/kg and its target is the central nervous system.
The general phytochemical screening revealed that the plant
did not contain significant amounts of products known to be
toxic, such as alkaloids or cardioactive glycosides, but only
catechic tannins, amino acids, saponins and other aphrogen principles in the three parts of the plant (fruit, leaf and bark).
Further toxicological tests are in progress in order to establish
the real target, how the toxin acts, and phytochemical studies
are being conducted in order to identify the active substance
responsible for the toxicity. Non protein amino acids will receive
attention because of their possible physiological and toxicological significance (Evans, 1996).
Acknowledgements
The authors are grateful to Professor J.P. Chapelle, Head of
the Medical Chemistry Laboratory, CHU Liège for providing
necessary biochemical research facilities. Acknowledgement is
extended to the Belgian Development Cooperation (DGDC) for
its financial support. Michel Frédérich is a Research Associate
from the Belgian National Fund for Scientific Research. Histological examinations were performed by Dr. D. Cassart in the
Clinical Laboratory for Small Animals (Faculty of Veterinary
Medicine, University of Liège, Belgium).
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