Aedes albopictus in Lebanon, a potential risk of arboviruses outbreak

Aedes albopictus specimens were sampled during the months of September and October of 2009 and 2010. Eggs were collected using ovitraps from Sarba, a coastal agglomeration located at 20 km north of Beirut, and from Fanar, an agglomeration at 250 m of altitude on the hills of the Mount Lebanon chain east of Beirut (Figure 1). Wooden strips were removed weekly from ovitraps, then dried for at least 3 days. Eggs were carefully removed and stored in humid chambers before hatching. Resulting F0/F1 adults were used for vector competence studies. Adults were collected by manual aspiration or using BG-sentinel traps or CDC miniature light traps coupled with dry ice as attractant. Traps were left in outdoor microhabitats for 18–24 hours and collected adults were stored at −20°C for further processing (blood-meal identification and phylogenetic analysis).

Mosquitoes were individually ground in wells of polystyrene plates previously saturated with a blocking buffer (3% fat free milk in PBS). The grinding was performed in 150 μl of PBS containing 3% fat free milk and 0.05% Tween 20, using an electric grinder (Micro Motor Escort®). Aliquots of each mosquito lysate were then stored at −20°C for later use.

To determine the animal species from which blood-meals originated, serum immunoglobulins specific to the most common urban hosts (poultry, dog, cat or human), were detected using a standard sandwich ELISA [18]. Briefly, plates were coated overnight at +4°C with 50 μl of capture antibodies, then saturated with 200 μl PBS containing 3% fat free milk. Mosquito lysates, diluted at 1/100, were added in duplicates and incubated for 1 hour at room temperature, followed by conjugated antibodies. Mosquito lysates and secondary antibodies were diluted in PBS buffer containing 3% fat free milk and 0.05% Tween 20. The immune complex was revealed by adding TMB substrate. The reaction was stopped after 15 min by adding 3 N HCl and the optical density was measured at 450 nm. All incubation steps were separated by 4 washes with PBS containing 0.05% Tween 20. Lysates obtained from males and females artificially fed on blood of the four host species tested were used as negative and positive controls respectively.

Capture antibodies were used at the following optimal concentrations: 4 μg/ml for rabbit anti-chicken IgY and goat anti-human IgG, and 2 μg/ml for rabbit anti-dog IgG and goat anti-cat IgG. Secondary peroxidase-conjugated antibodies were used at the following optimal concentrations: 0.05 μg/ml for goat anti-human IgG and rabbit anti-dog IgG and 0.2 μg/ml for goat anti-cat IgG, and rabbit anti-chicken IgY. All captures and secondary antibodies were affinity-pure and Fc fragment specific (Jackson ImmunoResearch Laboratories, Inc).

DNA was extracted from adults using the CTAB protocol [19]. Briefly, each specimen was ground in 200 μl CTAB lysis buffer (2% CTAB, 1.4 M NaCl, 10 mM EDTA, 100 mM Tris pH 8). The homogenate was incubated at 65°C for 5 min, then 200 μl chloroform were added and the mixture was centrifuged at 12,000 rpm for 5 min. The upper phase containing the DNA suspension was transferred into another tube, mixed with 200 μl isopropanol and centrifuged again at 12,000 rpm for 15 min. The DNA pellet was mixed with 200 μl of ethanol 70% and centrifuged at 12,000 rpm for 5 min. The supernatant was discarded and the pellet was dried for 30 min, then resuspended in 20 μl double distilled (dd) H₂O. Extracted DNA was used as template for amplification of three mtDNA genes: a 360 bp fragment for cytochrome b (cytb), a 600 bp fragment for cytochrome oxidase I (COI) and a 450 bp fragment for NADH deshydrogenase 5 (ND5). Three sets of primers were used: for cytb, L14841 (5’-AAAAAGCTTCCATCCAACATCTCAGCATGATGAAA-3’) and H15149 (5’-AAACTGCAGCCCCTCAGAATGATATTTGTCCTCA-3’) [20]; for COI, CI-J-1632 (5’-TGATCAAATTTATAAT-3’) and CI-N-2191 (5’-GGTAAAATTAAAATATAAACTTC-3’) [21] and for ND5, ND5FOR (5’-TCCTTAGAATAAAATCCCGC-3’) and ND5REV (5’-GTTTCTGCTTTAGTTCATTCTTC-3’) [22]. Each reaction was performed in a DNA Engine Peltier thermal cycler (Bio-Rad®), in a final volume of 30 μl. The PCR mixture contained 5U Promega Taq polymerase, 3 μl Taq polymerase buffer (10X), 0.5 μl of dNTPs (25 μM), 1 μl of each primer (10 μM), 1 μl of DNA, and 22.5 μl of water-free nuclease. The amplification reaction was performed under the following conditions: denaturation at 95°C for 4 min followed by heating at 95°C for 40 seconds; annealing for 1 min, at 46°C for cytb, 40°C for COI and 44°C for ND5; elongation for 1 min, at 66°C for cytb and COI, and at 70°C for ND5. The mixture was submitted to 35 cycles and to a final extension step of 7 min, at 66°C for cytb and COI and at 70°C for ND5. PCR products were separated by electrophoresis in a 1% agarose gel and purified using the Illustra GFX PCR DNA and gel band purification kit (GE Healthcare®). Genes were sequenced in an automated DNA sequence (ABI PRISM® 3130). Sequences were read using ChromasPro software.

Gene sequences were aligned using ClustalW software. A phylogenetic tree based on combined analysis of the three genes was constructed using Lebanese specimens as well as 13 other Ae. albopictus specimens described in [23]. A Maximum Likelihood tree was built using PHYML [24]. The significance of internal branches was evaluated using 1000 bootstrap replicates. Aedes aegypti from Hawai was used as outgroup.

At different days pi, total nucleic acids were extracted from individual mosquitoes and from dissected organs (midguts, wings, and salivary glands) and analyzed as follows: material was ground in 350 μl of RA1 solution and RNA was extracted using NucleoSpin® RNA II kit. Total RNA was resuspended in 40 μl dd H₂O, then a volume of 1 to 5 μl was used in a one-step RT-PCR reaction performed with a Power SYBR® Green RNA-to-CT™ one step kit (Applied Biosystem). The reaction in a volume of 25 μl contained: 1 to 5 RNA templates, 12.5 μl 2X Power SYBR® Green I RT-PCR Mix, 100–250 nM sense primer, 100–250 nM anti-sense primer, 0.2 μl RT enzyme mix and ddH₂O. Primers were selected in an encoding region (Table 1). The PCR program was: 48°C for 30 min, 95°C for 10 min; 40 cycles of 95°C for 15 s, 60°C for 1 min, 72°C for 30 s and 90°C for 15 s. A standard curve was generated using duplicates, from 10² to 10⁸ copies of RNA synthetic transcripts per reaction. Quantification of viral RNA was achieved by comparing the threshold cycle (Ct) values of samples to those of standards, according to the ΔC_t analysis.

After exposure to an infectious blood-meal, mosquitoes were tested for viral transmission potential at days 10 and 21 pi, by collecting saliva using the forced salivation technique [14]. Briefly, mosquitoes were anesthetized on ice and legs and wings were removed. The proboscis was then inserted into a pipette tip containing 5 μl of fetal bovine serum (FBS). After 45 min, the tip content was transferred in 45 μl of L15 medium.

Saliva suspensions were titrated by focus fluorescent assay on C6/36 cells of Aedes albopictus[34]. Samples were serially diluted and inoculated into C6/36 cells in 96-well plates. After an incubation of 3 days for CHIKV or 5 days for WNV and DENV-2 at 28°C, cells were stained using hyper-immune ascetic fluid specific to each virus as the primary antibody and conjugated goat anti-mouse as the secondary antibody.

The Fisher’s exact test was used for comparisons of rates (DIR and TR) and the Kruskall-Wallis test for comparisons of means from the STATA software (StataCorp LP, Texas, USA).

A total of 333 Ae. albopictus specimens were collected, including 136 females. Among those, 32 were obviously engorged (Table 2). The origin of the blood-meal was detected in 71.9% of them and was as follows: 46.8% of Ae. albopictus fed on humans, 15.7% on poultry, 6.3% on cats and 3.1% on dogs, suggesting that Ae. albopictus is preferentially anthropophilic (Fisher’s exact test: p < 0.05). All tested blood-meals came from a single host i.e., no mixed blood-meal was detected.

The alignment of the sequences corresponding to the three mitochondrial genes cytb, COI and ND5 from two specimens originating from each of the 6 localities sampled revealed no sequence polymorphism. Consequently, only specimens from one locality, Sarba, were considered for the phylogenetic analysis. The Lebanese Ae. albopictus sequences are identical to sequences obtained from specimens circulating in France, Madagascar and USA and La Providence (La Reunion). They were distantly related to the Asian and Brazilian specimens included in this study, which formed a distinct subgroup on the phylogenetic tree (Figure 2).