Uranotaenia unguiculata Edwards, 1913 are attracted to sound, feed on amphibians, and are infected with multiple viruses

Background Uranotaenia unguiculata Edwards, 1913 is a species of mosquito (Diptera: Culicidae) native to central Europe. Recently a novel lineage of the West Nile virus (WNV-lineage 4c) was identified in pools of adult female Ur. unguiculata. To increase the body of knowledge about this species, various trapping methods were evaluated to determine the most efficient method for capturing adult female Ur. unguiculata. Results Sound traps collected equivalent numbers of female Ur. unguiculata as low-hanging light-baited downdraft traps. Hosts were identified as Pelophylax lessonae and P. ridibunda (Anura: Ranidae) species group frogs from the blood found in engorged females. In addition to confirming infection by WNV-lin. 4c, a potentially integrated flavivirus sequence was detected in male mosquitoes. A novel Alphamesonivirus 1 (Nidovirales: Mesoniviridae) was found to be widespread in the Ur. unguiculata population and is herein described. Conclusions Efficient collection methods for Ur. unguiculata for arbovirus surveillance reflect mosquito questing behavior. Uranotaenia unguiculata targets frog species which call from the water, and it is likely that the novel WNV-lin. 4c is maintained in a frog-mosquito transmission cycle. The improved trapping methods listed here will assist future studies of the vector status of Ur. unguiculata for WNV and other arboviruses. Electronic supplementary material The online version of this article (10.1186/s13071-018-3030-2) contains supplementary material, which is available to authorized users.


Background
Uranotaenia unguiculata Edwards, 1913 (Diptera: Culicidae) is a species of mosquito native to the Western Palaearctic with species abundance highest in the Mediterranean biogeographical region [1,2]. European populations are infrequently collected during arbovirus surveillance programs using conventional mosquito trapping methods (e.g. CO 2 -baited light traps), often comprising less than 0.5% of the total collections [3][4][5][6]. It is often reported that Ur. unguiculata feeds exclusively on amphibians [1], similar to other members of the genus Uranotaenia [7,8], although what little evidence exists for this behavior in Ur. unguiculata is conflicting [9][10][11]. Comparatively little is known about the mosquito, particularly its importance as a vector of zoonotic viruses.
In 2013, our group reported the existence of a novel lineage of West Nile virus (Flaviviridae, "WNV") in Ur. unguiculata from Austria [5], and a similar virus was reported from Ur. unguiculata populations in Romania [6] and Hungary [4]. The virus was closely related to WNV-lineage 4 (WNV-lin. 4a) found in Russia in Ur. unguiculata [12] and in Spain in Culex pipiens (Linnaeus, 1758) (Diptera: Culicidae) (WNV-lin. 4b) [13]. Investigations at a study site in Volgograd, Russia, identified virus nucleic acid (WNV-lin. 4a) in both the frog population [Pelophylax ridibundus (Pallas, 1771) (= Rana ridibunda Pallas, 1771)] (Anura: Ranidae) as well as the Ur. unguiculata population [14]. However, no study has conclusively determined that Ur. unguiculata feed on frogs. Furthermore, nucleic acid from a potentially unique flavivirus has been identified from a population of Ur. unguiculata in Turkey [15]. Therefore, the potential of Ur. unguiculata to vector arboviruses to humans and other animals remains unknown.
Herein we describe improved trapping methods to target the collection of adult Ur. unguiculata at a site in the Pannonian biogeographical region of central Europe. We sought to improve upon standard mosquito trapping methods, using both modified traditional and non-conventional mosquito traps, to collect adult females. A longitudinal study was performed using the improved method over a single collection season, yielding many individuals, including males and blood-engorged female specimens. As a result, we provide further support to the hypothesis that WNV-lin. 4c is transmitted to frogs by Ur. unguiculata, and describe a novel alphamesonivirus isolated from a pool of male Ur. unguiculata.

Study site
The majority of mosquito collections were performed at Lake Neusiedl, the largest endorheic lake in central Europe. Mosquito trapping was focused at the Biological Station Lake Neusiedl, Illmitz ("BSI," 47°46. 12

Mosquito collection
Adult mosquitoes were collected with modified CDC Light Traps (John W. Hock Co. Gainesville, FL, USA) using either fluorescent or ultraviolet lights. Traps were placed 1 m from the water edge and the trap intake was 0.5 m from the water surface, and run from 1 h before sunset until 1 h after sunrise. The sampling session in Hungary was performed with a strong mercury lamp over a one hour period approximately 1 h after sunset (21:00-22:00 h). Resting adults were collected using a backpack aspirator (John W. Hock Co, Gainesville, FL, USA) from fixed sites at BSI sampled routinely in the morning and evening: pathways through the reeds cleared by semiaquatic rodents, a man-made wooden boardwalk extending above water into the reeds from shore, and four black plastic refugia (30 × 30 cm boxes, 15 cm tall, lacking a western-facing side, similar to [16]) which were placed at various sites near the water.
Sound traps were modified from gravid traps (John. W. Hock Co. Gainesville, FL, USA): a black plastic basin was filled with 2 cm lake water and an updraft fan was positioned above the water. A small 3 cm speaker was placed at the mouth of the fan intake and broadcast the recorded call of individual Dryophytes gratiosus (LeConte, 1856) (Anura: Hylidae), a species of tree frog native to the southeastern United States whose call is attractive to Neotropical Uranotaenia species [17]. The sound of the calling male frog consisted of approximately one call per s for 14 s, and was broadcast repeatedly for 2 h beginning 1 h after sunset, setting the volume at maximum each night (Additional file 1: Figure S1). Mosquitoes were anesthetized by 5 min incubation at -20°C and sorted to species on an ice-cold plate according to morphologic characters described in [1]. Samples were pooled (n < 50 per pool) by species, sex, and date and stored at -80°C until analysis.

Vertebrate host identification
DNA was extracted from individually separated abdomens of blood-fed specimens (the remaining body parts were pooled by date for virus analysis) using a commercial kit (DNEasy, Qiagen GmbH, Hilden, Germany). Hosts were identified by PCR following published methods which use vertebrate-specific primers designed to amplify portions of the mitochondrial gene 16S rRNA ("L2513", 5'-GCC TGT TTA CCA AAA ACA TCA C-3'; "H2714"; 5'-CTC CAT AGG GTC TTC TCG TCT T-3') [18] or cytochrome b (5'-CCC CTC AGA ATG ATA TTT GTC CTC A-3'; 5'-GCH GAY ACH WVH HYH GCH TTY TCH TC-3') [7]. The amplicons were subjected to Sanger sequencing (Microsynth AG, Balgach, Switzerland), and sequences were compared to voucher specimens collected from the study site (kindly provided by Silke Schweiger, curator of the herpetology collection of the Austrian Museum of Natural History, Vienna, Austria).

Virus detection using RT-qPCR
A single copper-coated steel bead was added to each pool of mosquitoes, and the pools were homogenized in virus growth media [VGM, composed of Dulbecco's minimum essential medium (DMEM), supplemented with 10% fetal calf serum (FCS), penicillin/streptomycin, and 0.25 μg/ml amphotericin B, all cell culture reagents from Gibco, Ther-moFisher Scientific, Paisley, UK] using a TissueLyzer bead mill with a pre-cooled rack set to 30 Hz for 1 min (Qiagen GmbH, Hilden, Germany). Homogenate was cleared by centrifugation at 8000× g for 4 min at 4°C, and supernatant was stored at -80°C. Total RNA was extracted from the pellet using a commercial kit (Zymo Research Corp., Irvine, CA, USA). A one-step RT-qPCR assay was performed with universal flavivirus primers (PF1S and PF2) targeting a portion of the flavivirus NS5 [19] using a commercial kit (Luna®, New Enlgand Biolabs, Inc., Ipswitch, MA, USA, "NEB"). A second RT-qPCR was used to confirm putative identifications, using pan-flavivirus primers (100F and 200R) and a commercial kit (NEB) [20]. Using a probe-based RT-qPCR kit (NEB) alphamesonivirus nucleic acid was detected in mosquito pools with primers designed to match a conserved portion of the ORF1b putative replicase domain (MesoF,

Virus rescue and identification of unknown virus
Virus was rescued from putative positive homogenates on C6/36 insect cells (ATCC #CRL-1660). Briefly, C6/36 cells were incubated with 100 μl of homogenate on a 6-well plate. After 1 h, DMEM with 2% FCS, antibiotics, and antimycotics were added to each well. On day 6 post-infection, cell culture supernatant was blind-passaged into new C3/63 cells and to Vero cells (ATCC #CCL-81). When cytopathic effect (CPE) was observed, supernatant was filtered through 0.2 μm filter and purified through a 36% sucrose cushion at 28000× rpm in a cooled ultracentrifuge. The pellet was treated with RNase and DNase (Promega) for 1 h at 37°C and RNA was extracted from the pellet as described above. First and second strand cDNA were synthesized with 40U AMV reverse transcriptase (Promega, Mannheim, Germany) followed by treatment with 1U RNase H and 20U Klenow fragment DNA polymerase (Promega) using non-specific primers with a known sequence at the 5' end (5'-GAC CAT CTA GCG ACC TCC ACN NNN NNN N-3') as described by others for the sequence-independent amplification of virus particle-associated nucleic acids (PANA) [21]. The cDNA was used as a template for PCR using primers for the known sequence (5'-GAC CAT CTA GCG ACC TCC AC-3'), and the resulting amplicons were TA-cloned into a pGEM vector (Promega). Cloned inserts ≥ 500 bp were detected by colony PCR using M13 primers and Taq polymerase (GoTaq G2® DNA polymerase, Promega) and amplicons were sequenced. These sequences were compared to sequences in the GenBank database using the basic local alignment search tool (BLAST), and primers were designed from the closest-matching sequences to produce a near full-length viral sequence by primer-walking (Additional file 2: Table S1). The sequence was deposited in the GenBank database under the accession number MH215275.

Sequence characterization of Alphamesonivirus 1 isolate
The near full-length sequence (missing portions of the 3' and 5' sequence) of the alphamesonivirus isolate was aligned to reference sequences from the family Mesoniviridae using the MUSCLE algorithm, and sequence analyses were performed in MEGA 6.06 [22,23]. Percent sequence identity for aligned nucleotide and amino acid sequences were calculated with the "Sequence Manipulation Suite" [24]. A maximum likelihood (ML) tree was constructed from the amino acid sequence alignment for the open reading frame encoding the conserved putative spike protein (ORF 2a). The initial tree was obtained by the neighbor-joining method. The final tree was generated using the Jones-Taylor-Thornton matrix-based model with a very strong branch swap filter, and ML estimates are based on bootstrap resampling of 1000 replicates.

Determination of mosquito infection and virus transmission
In June 2018, Ur. unguiculata mosquitoes were collected using sound traps. Individuals were held for 2-5 days at ambient temperature and natural light in humidified chambers and provided 25% solution of local honey in water on Whatman® FTA® cards. The honey cards were changed daily and stored at -80°C thereafter. The legs and wings were removed from mosquitoes and stored in 250 μl VGM in pools of 1-10 individuals. The rest of the mosquito (head, abdomen and thorax) was stored in 500 μl VGM in pools of 2-50 individuals. Pooled mosquito parts were homogenized using a bead mill, and RNA was extracted as described above. If virus nucleic acid was detected in a pool of mosquito bodies by RT-PCR methods described above, then the corresponding pools of legs and wings were similarly tested for the presence of virus nucleic acid. The presence of virus nucleic acid in the legs and wings indicates a disseminated infection. To test for virus transmission, RNA was extracted from the FTA honey cards by first soaking the card in 500 μl Tris-EDTA buffer for 1 h with shaking, then extracting RNA from 200 μl of the Tris-EDTA solution as described above.

Statistical analysis
A two-tailed binomial test was used to compare the collection efficiency of trap methods with the null hypothesis that traps collect equal numbers of mosquitoes. A sign test was used to compare between methods over paired trap-nights. The minimum field infection rate (MFIR) was calculated with ML estimator statistics using "Pooled infection rate 7.0" Microsoft Excel plug-in available from the United States Centers for Disease Control and Prevention, according to methods described therein [25]. Figures were prepared in GraphPad Prism5.

Summary of collection methods for Uranotaenia unguiculata
From 9 August 2016 to 15 September 2016, miniature CDC light traps were used at BSI to collect Ur. unguiculata in order to establish a baseline collection rate.
Traps were baited with a fluorescent light (n = 4 trap-nights), UV light (n = 6 trap-nights), or fluorescent light with dry ice as a source of CO 2 (n = 2 trap-nights). In total, 3347 mosquitoes (3025 females) were collected over 12 trap-nights. Both males (9.6% of the total collection) and females of Anopheles sp. (Diptera: Culicidae), Coquillettidia richiardii Ficalbi, 1899 (Diptera: Culicidae), Culex sp. (Diptera: Culicidae), and Ur. unguiculata were captured in all light traps. Culex pipiens, Cx. torrentium Martini, 1925 (Diptera: Culicidae) (46.7%, Cx. pipiens were not differentiated from Cx. torrentium) and Cx. modestus Ficalbi, 1889 (Diptera: Culicidae) (12.5%) were the dominant culicine mosquito species collected at the site, whereas An. hyrcanus (Pallas, 1771) (30.5%) and An. maculipennis Meigen, 1818 (s.l.) (Diptera: Culicidae) (5.9%) were the dominant anopheline species (Fig. 1a). More male Ur. unguiculata (n = 274) were collected than females (n = 108, average 8.5/trap-night, SD = 12.1). Significantly more Ur. unguiculata were captured at fluorescent-baited traps than UV (39%) traps (binomial test, P = 0.011; sign test for trap-night, P = 1.00), although trap success was low until mid-September. Due to low collection size, the difference in collection efficiency of Ur. unguiculata between traps baited with and without CO 2 could not be inferred. However, the addition of CO 2 appeared to have an effect on other species (e.g. fewer Cq. richiardii and more Anopheles sp. were collected in traps with CO 2 than without, Fig. 1a). No Ur. unguiculata were collected from artificial resting boxes nor from natural resting sites in reeds. On 12 September 2017, 13 male and 2 female Ur. unguiculata, which appeared to be newly emerged imagoes, were captured by aspiration resting under a boardwalk that extended over shallow water into the reeds. Larvae were present in the water beneath this collection site.
These preliminary findings represented a substantial increase in the number and proportion of Ur. unguiculata in comparison to previous similar trapping methods: here we report 3.6% of total female mosquitoes collected were Ur. unguiculata, whereas others report Ur. unguiculata made up < 1% of total collections in this region [5,26]. Therefore bi-weekly trapping was performed with a single low-hanging fluorescent light trap placed as before at BSI beginning 31 May 2017. A single female Ur. unguiculata was captured on 14 June 2017 and a single male Ur. unguiculata was captured on 22 June 2017. Following that, no Ur. unguiculata were captured until August, and the peak collection period began on 2 August 2017 and continued until 7 September 2017 (Fig. 1b).
To test the hypothesis that Ur. unguiculata are attracted to sound, sound traps were used at several locations around the lake. Each night a sound trap was used, a 'mock' sound trap (updraft trap with no sound) was placed 3-10 m away, and a fluorescent light trap was placed at the same site > 10 m from the sound trap and out of sight from the sound trap (n = 5 nights). No Ur. unguiculata were captured in 'mock' sound traps, whereas 86 female Ur. unguiculata were captured in the sound traps (average 12.2 per trap-night; range 0-36) ( Table 1). The trap success of the sound traps was not different from light traps (compared on n = 5 nights, average 12.4 per trap-night in light traps; range 1-27) (binomial test, P = 0.06; sign test for differences in trap night, P = 1.00) ( Table 1).

Hosts of Uranotaenia unguiculata
Eight blood-engorged female Ur. unguiculata were collected from 8 August 2017 through 7 September 2017: five individuals from sound traps, and three individuals from light traps (including two from Hungary captured using a mercury lamp). Hosts were identified from the blood meal using 16S rRNA PCR [18], and amplicons were compared to a DNA library made from voucher specimens. All were identical to Pelophylax lessonae/ ridibundus species group voucher specimens collected from the site. These identifications were confirmed using cytb PCR protocol [7]. Although voucher specimens exist for P. lessonae, P. ridibundus and P. esculentus (which make up the species group), these species could not be differentiated by the sequenced amplicons.

Flavivirus identification
In 2016, 108 female and 274 male Ur. unguiculata were captured and divided into 11 and 10 pools, respectively; and in 2017, 185 female Ur. unguiculata and 107 males were captured and divided into 14 and 7 pools, respectively, for flavivirus screening. Two pools of females and one pool of males from 2017 tested positive for the presence of flavivirus nucleic acids (NS5 gene) by both RT-qPCR methods ( Table 2). Sequencing of these amplicons showed that the pools of females (2017, MFIR = 12; 95% CI: 2.2-40.8) were positive for WNV-lin. 4c with 99% sequence identity to published sequences from 2013 (KJ891223 "WNV Uu-LN-AT-2013") [4,5], differing in only 3 synonymous nucleotide substitutions across the 205 bp product of the NS5 gene; and 99% sequence identity to an 800 bp portion of the E gene, differing at 3 synonymous nucleotide substitutions. A bias-corrected ML estimator calculation for the MFIR was 12.05 (95% CI: 2.20-40.76) for female Ur. unguiculata over both years.
The flavivirus RNA-positive pool of males displayed closest sequence identity (100%) to a published sequence that was detected in Ur. unguiculata from Turkey (GenBank: KU958167) [15]. The presence of the DNA form of the  sequence was confirmed by PCR amplification from the RNA extract (i.e. without reverse transcription).

Alphamesonivirus isolation and characterization
Two pools of male Ur. unguiculata had putative positive amplification by one flavivirus RT-qPCR (where Ct > 30 but melting curve analysis did not match positive controls) [19]. Therefore the pool homogenates was inoculated onto C6/36 cells. One pool caused CPE at 6 days post-infection, and was then filtered and passed to flasks of C6/36 cells. This passage (p2) was used for sequence characterization by PANA [21], as it did not produce amplicons by flavivirus-specific RT-qPCR. This passage did not produce CPE on Vero cells grown at 37°C. Following PANA PCR cloning, the virus was determined to be an alphamesonivirus, based on the sequence of 6 unique gene products approximately 500-2000 bp long distributed throughout the genome. Primers were designed based on sequence similarity to previously characterized alphamesoniviruses (Additional file 2:  Table 3). An RT-qPCR assay was designed to screen the other pools of male and female mosquitoes for the presence of alphamesonivirus. Ten pools from 2016 (five pools of females) and nine pools from 2017 (seven pools of females) were positive for alphamesonivirus (

Mosquito infection and virus transmission
A total of 362 female Ur. unguiculata mosquitoes were collected over four nights around Lake Neusiedl in June 2018. The legs and wings were dissected and the remaining bodies were pooled in 44 pools for the detection of virus (Table 4). The presence of WNV-lin. 4c was detected in nine of these pools, corresponding to 225 mosquitoes from which legs and wings had been pooled into 39 pools. WNV-lin. 4c was detected in six of the 39 pools. The potential for virus transmission was determined by detecting virus nucleic acid on honey-soaked FTA cards which had been placed into chambers with mosquitoes for feeding purposes prior to their dissection. WNV-lin. 4c nucleic acid was detected Fig. 2 Phylogenetic tree of the amino acid sequence of the putative spike protein (complete ORF2a) from selected species of Mesoniviridae, including a newly described isolate from Uranotaenia unguiculata in Austria (MH215275). Node support is based on 1000 bootstrap replicates on one of nine honey cards, suggesting that Ur. unguiculata are capable of transmitting the virus. Alphamesonivirus was detected in three pools of mosquito bodies, corresponding to 11 mosquitoes, from which the legs and wings had been placed into tubes individually. From these 11 mosquitoes, alphamesonivirus was detected in the legs and wings of two individuals, indicating a disseminated infection. The presence of alphamesonivirus nucleic acid was detected on three of the nine honey cards, suggesting the presence of the virus in saliva.

Discussion
Herein we report the first molecular identification of the hosts of Ur. unguiculata from the guts of blood-engorged flies. The hosts were identified as anurans, and a similar host preference is known for other members of the genus Uranotaenia [7,8]. Commonly encountered species of anurans at BSI during the study period included Pelophylax sp., as well as Hyla arborea (Linnaeus, 1758) (Anura: Hylidae), Bufo bufo (Linnaeus, 1758) (Anura: Bufonidae) and Bombina bombina (Linnaeus, 1761) (Anura: Discoglossidae) (via visual encounter during trap setup). It is unknown if Ur. unguiculata takes blood from animals other than frogs. Previous attempts to identify the hosts of Ur. unguiculata have relied on serological testing, wherein amphibian antiserum was not used or was unavailable, and the host identities were determined to be from reptiles [10] or a horse [11]. It has been reported that Ur. sapphirina (Osten Sacken, 1868) (Diptera: Culicidae), a Nearctic species, may also feed on mammals in addition to amphibians [7,29]. Furthermore, landing captures and captures from host-baited traps suggest that Ur. unguiculata may be attracted to mammals including humans [9,11,30] but not birds [3]. The relatively low efficiency of common mosquito collection methods (e.g. CO 2 -baited light traps) for the collection of Ur. unguiculata has left many gaps in the knowledge of the behaviors of this species.
Efficient collection methods for a mosquito species reflect its host preference and common methods (e.g. CO 2 -baited light traps) are designed to collect mosquitoes based on foraging behavior during appetential flight [31]. For example, trap height is an important factor for collecting ornithophilic versus mammal-biting mosquitoes [32][33][34]. Sebesta et al. [3] collected Ur. unguiculata in 1 m high CO 2 -baited CDC light traps, and none in 5-m high traps nor in pigeon-baited traps. We reasoned that Ur. unguiculata foraging preference would reflect host behavior, and therefore placed our traps near the water surface (0.5 m height). Although we did not compare the importance of trap height to collection efficiency of Ur. unguiculata directly, this trap placement was an improvement compared to other published records of Ur. unguiculata in the same trapping  Legs and wings were stored separately from body, and samples were pooled into tubes of 2-50 (bodies) or 1-10 (legs and wings). Each honey card sampled between 20-50 mosquitoes c Pools were tested for the presence of virus by RT-PCR locales [5,26] as well as in the broader surrounding biogeographical regions [35] using common mosquito collection methods. Importantly, we collected both male and female Ur. unguiculata; the efficient collection of males to our knowledge has not yet been reported.
Although we provide evidence that Ur. unguiculata females are attracted to sound, it is unknown if sound is used exclusively to locate hosts. The host species identified here, Pelophylax sp. and B. bombina were the only two species of anurans heard calling during the collection period. Sound attraction is known from Ur. lowii Theobald, 1901 (Diptera: Culicidae), a Neotropical species of mosquito [17], and several species of Uranotaenia from Japan [8]. Acoustic location of hosts by hematophagous dipterans is best known from the Corethrellidae (Wood & Borkent 1989), a family closely related to mosquitoes which feed on frogs [36][37][38]. The sound of the calling male D. gratiosus, a Nearctic species of frog, is attractive to Ur. lowii as well as to Neotropical and Australian corethrellids. Therefore it has been hypothesized that acoustic location in corethrellids is performed by a sensory organ that detects frequencies that are similar to wing beat frequency (approximately 420-450 Hz), which match the dominant frequency of the call of D. gratiosus (Additional file 1: Figure S1) [37,39,40]. The Johnston's organ is known to be the auditory organ of mosquitoes, and is used to identify the wing beat frequency of conspecifics during mating, though may be sensitive up to 2 kHz in some species [41,42]. Further studies on acoustic location and sound preference of Ur. unguiculata are underway, and the attractiveness of native anuran calls will be evaluated.
Knowledge of mosquito host feeding behavior is very important for understanding the epizootic potential of arboviruses. The presence of WNV-lin. 4c nucleic acid was recently reported in Ur. unguiculata from the study location here, as well as other sites in central Europe [4][5][6].
Here we provide evidence that Ur. unguiculata are feeding on Pelophylax sp. at a site where WNV-lin. 4c was detected in pools of conspecifics, including evidence that suggests the mosquitoes are both infected with the virus and are capable of transmitting the virus. Taken together with the detection of virus nucleic acid present in both Ur. unguiculata and also frogs (P. ridibundus) collected from a site in southern Russia [14], it is likely that this virus is maintained in a frog-mosquito transmission cycle. The first identification of WNV-lin. 4 was from a Dermacentor marginatus (Sulzer, 1776) (Acari: Ixodidae) tick in the Volgograd region, southern Russia, in 2003 (WNV-lin. 4a; GenBank: AY277251) [12], and a similar virus has also been isolated from Cx. pipiens in Spain 2011 (WNV-lin. 4b; GenBank: GU047875) [13]. In sum, there is further support for WNV-lin. 4c being ecologically and genetically distinct from other WNV lineages [43]. Since WNV-lin. 1 and WNV-lin. 2 are known pathogens to humans and animals, it is important to understand the epizootic potential of the WNV-lin. 4c. Initial efforts have been successful in isolating this virus on C6/36 cells, and future efforts should characterize the pathogenicity of the virus. Additionally, the vector status of Ur. unguiculata for WNV-lin. 4c must be determined in controlled experiments.
The genus Uranotaenia has few reports of infection with arboviruses. Eastern equine encephalitis virus was discovered in Ur. sapphirina in the southern USA [44], and a cyprovirus (Reoviridae) has also been isolated from this species [45]. A novel flavivirus, Nounane virus, was reported from Ur. mashonaensis Theobald, 1901 (Diptera: Culicidae) in Côte d'Ivoire [46]. Nounane virus bears closest similarity to Barkedji virus, a virus found in Cx. perexiguus Theobald, 1903 (Diptera: Culicidae) mosquitoes in Israel [47], and Nhumirim virus, a virus found in Cx. chidesteri Dyar, 1921 mosquitoes from Brazil [48]; the vertebrate host is unknown for these viruses, although all are genetically similar to mosquito-borne zoonotic flaviviruses and not to insect-specific flaviviruses. Herein we report a potentially endogenous flavivirus-derived genomic sequence, identical to the sequence reported by others in Ur. unguiculata [15], possibly reflected an ancient association between Uranotaenia and flaviviruses [49,50]. In addition, we isolated and sequenced the genome of an alphamesonivirus which is widespread in the population at BSI. Another member of the family Mesoniviridae, Meno virus, was isolated from Côte d'Ivoire, 2004, where it was found in Ur. chorleyi Edwards, 1936 (Diptera: Culicidae) along with Cavally virus, the first insect-associated nidovirus [27,51]. Much remains unknown about this newly discovered family of insect viruses, which are within the Nidovirales [27,28]. Future efforts will further characterize the virus isolate reported herein, and the presence of this or another alphamesonvirus within other mosquito species in the region will be tested.
In general, the comparatively low efficiency of collection and lack of human-biting behavior have likely contributed to the gaps in knowledge about this mosquito species in the Western Palaearctic. The optimized sampling conditions reported here increased trapping success compared to previous methods. This will aid in future studies of the habits of this elusive mosquito, and the transmission of arboviruses.

Conclusions
Improved collection techniques have yielded this first definitive report of the hosts of Ur. unguiculata using molecular methods, and have revealed the presence of a novel insect-specific flavivirus. The mosquitoes take blood from frogs, Pelophylax spp., and may transmit WNV-lin. 4c to frogs, although vector competence has not yet been established. It was discovered that Ur. unguiculata are attracted to sound, potentially as a method of acoustic location of hosts. Further research will focus on the ecological association between the mosquitoes and their hosts, as well as