Background
Anopheles gambiae s.s.,
Anopheles arabiensis,
Anopheles mascarensis,
Anopheles funestus,
Anopheles merus and, recently,
Anopheles coustani are the most important vectors of malaria in Madagascar [
1‐
5]. Malaria vector control constitutes one of the major malaria control strategy, to target a reduction in
Anopheles vector density and prevent parasite transmission [
6] by using insecticide through indoor residual spraying (IRS) and by implementing insecticide-treated bed net (ITN) mass distribution. In sub-Saharan Africa, malaria vector control programmes continue to rely heavily on IRS and [
6,
7], both of which depend on vector susceptibility to the insecticides used [
8]. ITN and IRS have been proven to be effective in reducing the risk of infection with malarial parasites, clinical disease and child mortality [
9‐
11]. In Madagascar, vector control interventions avoided over 100,000 clinical cases of malaria in 2012 and 2013 [
12].
The World Health Organization (WHO) advises national programmes to evaluate insecticidal activity on nets and on treated walls [
13]. Indeed, essential to the success of these vector control campaigns is the implementation of strong quality control procedures that monitor programmatic effectiveness [
14‐
16]. Long-lasting, insecticidal-treated nets’ (LLINs) useful life may vary considerably from region to region [
17,
18]. A net that is used year-round is likely to lose insecticide more rapidly due to handling and cleaning than a net that is used only seasonally [
17,
19]. The efficacy of IRS may decay with time and must be re-applied frequently and it is important to know the optimal application interval in the field depending on the residual life of the insecticide [
10]. Previous studies have reported that insecticide residual life depends on the substrate to which it is applied [
20,
21]. Evaluation of the residual activity of insecticide applied on treated substrates becomes a necessity when aiming for long-term efficacy of an IRS implementation campaign. The World Health Organization Pesticide Evaluation Scheme (WHOPES) recommends the use of a susceptible mosquito strain, whether to evaluate LLIN bio-efficacy or to determine efficacy of the residual insecticide deposited on a wall over time. In both cases, cone bioassays are used [
13,
22].
Rresults of a study is aiming to determine the susceptibility status of An. arabiensis which is the only laboratory strain used for assessing quality control of malaria vector control tools across Madagascar.
Methods
Insectarium
The insectarium is composed of a breeding room divided into a rearing-larvae box of 25 sq m and an adult-maintaining box of 15 sq m. The larvae box is sustained at a temperature of 29 °C ± 2 and adult mosquitoes are maintained at 27 °C ± 2 with a humidity of 80 %. The insectarium uses a 12:12 light:dark schedule. This is accomplished by using a simple light timer.
Mosquitoes
The An. arabiensis strain has been grown at the Institut Pasteur de Madagascar since April 2010. It comes from Ambohimanambola (18°57′35.38″S; 47°35′53.91″E), southeast of Antananarivo in the Central Highlands of Madagascar. Adult mosquitoes were caught, in stables in the stage of digesting their blood meal, using manual aspirators and put into paper cups. Females were placed in cages made of netting, and their eggs were conducted into petri dishes containing cotton covered with a wet filter paper.
Anopheles arabiensis rearing and colony maintaining
Eggs from wild females were reared in the insectarium. A method which allows mosquitoes to lay eggs on wet filter paper was used. The eggs were harvested every morning. Once the eggs hatched, larvae stage I were removed using a dropper and distributed in batches into white plastic trays 9 cm high × 35 cm long × 25 cm wide, containing tap water 1-cm deep. The larvae were fed with laboratory animal diet powder. To avoid water evaporation, batches were covered with a Plexiglas plate.
At emergence, mosquitoes were placed in cages 23 × 23 cm made with plastic netting. One side of the cage had an opening for allowing the arm to perform various manipulations inside the cage. During the first 20 generations, female mosquitoes were fed directly using a live rabbit. Due to restrictions on use and the difficulty of live animals in a research setting, artificial membrane methods were used: successively, pig bladder, chicken skin membrane and Parafilm M ®. From the 70th generations, female mosquitoes were blood-fed with healthy sheep blood by using an artificial blood-feeder (Hemotek®) and they received a 10 % sucrose solution.
Insecticide susceptibility test
WHO bioassay tests
For each insecticide, 400 female mosquitoes 2–5 days old were exposed to diagnostic doses of various insecticides for susceptibility tests, using insecticide-impregnated papers, as described by standard WHO testing protocol [
23].
Mortality resulting from tarsal contact with insecticide-treated filter papers was measured using WHO test kits [
23]. The tests were carried out using malathion 5 %, fenitrothion 1 %, deltamethrin 0.05 %, permethrin 0.75 %, alphacypermethrin 0.05 %, bendiocarb 0.1 %, propoxur 0.1 %, and DDT 4 %. Insecticide-impregnated papers were obtained from the Malaysian WHO Collaborating Centre at standard concentrations for determining resistance of adult mosquitoes. Four batches of 25 unfed females were exposed to impregnated papers for 1 h. The number of knock-down mosquitoes was recorded every 10 min. Tests with untreated papers that served as control were run in parallel. At the end of the exposure period, mosquitoes were transferred into tubes with untreated white filter papers (known as holding tubes) and allowed a 24-h recovery period. All mosquitoes were provided with 10 % glucose water during the 24-h recovery period. Mortality rate was recorded after 24 h.
CDC bottle test
The principle of CDC bottle bioassay is to determine the time it takes an insecticide to penetrate an arthropod, traverse its intervening tissues, get to the target site, and act on that site relative to a susceptible control. Anything that prevents or delays the compound from achieving its objective of killing the arthropods contributes to resistance.
Diagnostic doses that were applied in the present study were the doses recommended by CDC [
24]. For
An. gambiae s.l., diagnostic doses were 12.5 μg per bottle for deltamethrin and bendiocarb and 21.5, 100, 50 μg, respectively, for permethrin, DDT and malathion. The diagnostic time was 30 min except for DDT (diagnostic time = 45 min). The solutions were prepared and the bottles coated according to CDC protocol [
25]. Fifteen to 25 unfed female mosquitoes aged two to five days were introduced into four 250-ml Wheaton bottles coated with insecticide and one control bottle coated with acetone only. The number of dead or alive mosquitoes was monitored at different time intervals (15, 30, 35, 40, 45, 60, 75, 90, 105, 120 min).
PCR detection of the kdr mutation
One-hundred mosquitoes were used for PCR assays. Each mosquito was extracted using two or three legs following the protocol described by Cornel and Collins [
26]. Leg extractions were used to genotype samples for the
kdr allele, using a PCR diagnostic test for detection of
kdr ‘Leu-phe’ mutations following the protocol described by Martinez-Torres [
27]. Thermocycler conditions consisted of an initial denaturation step of 94 °C for 5 min, 30 cycles of 94 °C for 30 s, 50 °C for 30 s, 72 °C for 30 s, followed by a final extension of 72 °C for 5 min.
Data interpretation
If the mortality in control batches was greater than 5 %, observed mortality rates were corrected by using Abbot’s formula [
28]. Susceptibility status of
An. arabiensis laboratory strain was determined according to the standards of WHO [
24]. A mortality ranged between 98 and 100 % indicates susceptibility. An observed mortality between 90 and 97 % may indicate a resistance and resistant genes should be confirmed. If mortality is less than 90 %, the population is considered as resistant and the resistance mechanisms must be identified.
Discussion
This study describes a successful colonization of
An. arabiensis in the laboratory. At first authors managed to establish a colony of
An. arabiensis in Dakar (Senegal) [
29]. Then, many studies focused to the improvement of
An. arabiensis rearing, from several localities. All of these studies focused on larval development rate and wing length by studying the best larval breeding condition that would allow larval growth and survival for mass mosquito rearing [
30‐
35]. In the current observation, the breeding productivity of
An. arabiensis showed important difficulties to adapt in laboratory conditions. In the insectarium of Institut Pasteur de Madagascar, the percentage of hatched eggs was 40 %, which is relatively low compared to the average rate obtained with
An. arabiensis (Dakar’s strain) in insectarium, estimated at 54.4 % [
29] and increasing from generation to generation. Regarding emergence rate, results in this current study are similar to those reported by Diop et al. [
29] with 95 %, allowing obtaining enough adults for the next generations.
The results of WHO bioassay test on
An. arabiensis laboratory strain in the present study highlight the full susceptibility of this strain to insecticides. Compared to laboratory-reared
An. arabiensis adults (KGB strain, originated from the Zambezi Valley, Zimbabwe) known to be susceptible to deltamethrin 0.05 % and bendiocarb 0.1 % [
23], both populations have a mortality rate of 100 %. Using DDT 4 %, permethrin 0.75 %, the mortality rate was 100 % showing the fully susceptible status of
An. arabiensis Institut Pasteur de Madagascar strain. The same results were obtained with the main susceptible reference strain
An. gambiae KISUMU strain in the Republic of Cameroon [
36] and in Tanzania [
37].
With propoxur 0.1 % and fenitrothion 1 %, current results corroborate with results obtained with the reference strain
An. gambiae (KISUMU strain) in Côte d’Ivoire [
38] with 100 % mortality rate. No resistance was detected for the organophosphorus insecticide malathion 5 %. The mortality rate of
An. arabiensis Institut Pasteur de Madagascar strain showed 100 % mortality just as susceptible as
An. arabiensis Durban strain in Mozambique, with lambda-cyhalothrin 0.05 %, deltamethrin 0.05 %, permethrin 0.75 %, bendiocarb 0.01 %, propoxur 0.01 %, malathion 5 %, and DDT 4 % [
39]. High mortality rates obtained with CDC bottle test corroborate the 100 % mortality rate of
An. gambiae KISUMU strain exposed to permethrin, deltamethrin and bendiocarb [
40,
41]. All in all,
An. arabiensis Institut Pasteur de Madagascar strain shows the same susceptibility patterns as the most used susceptible
Anopheles strains.
As preconized by WHOPES, when a compound is submitted for an evaluation, it should be tested against a susceptible reference strain, i.e., a strain which is considered to present the highest susceptibility level to the main classes of insecticides [
22]. Such reference-susceptible strains exist for regionally important
Anopheles species:
Anopheles albimanus [
42],
Anopheles darlingi [
43],
Anopheles culicifascies,
Anopheles stephensi [
44,
45],
Anopheles quadriannulatus [
46],
Anopheles minimus [
47],
An. arabiensis with different strains depending on the region [
46,
48,
49], and
An. gambiae Kisumu strain [
50]. Considering bioassay results with
An. arabiensis Institut Pasteur de Madagascar strain, its high susceptibility to all tested insecticides within four classes corroborate the definition of a susceptible reference strain [
13,
22].
Authors’ contributions
SR and SB drafted the manuscript. SR, SB and HJV participated in mosquito rearing, strain maintaining and bioassay tests. All authors read and approved the final manuscript.