Sampling took place from June–August, 2007 and April–May 2008 at 20 sites in the lowland forests of Cameroon (Figure 1). Coquillettidia spp. were only found at four of those sites, Mvia (N03.5105° E010.0176°) Nk'leon (N02.3974° E010.0452°), Ndibi (N 03.774897° E12.201532°), and Nkouak (N03.86735° E013.31634°). The majority (95%) of the total numbers of Coquillettidia mosquitoes were collected in Ndibi and Nkouak. The lowland forests of southern Cameroon have a humid equatorial climate with three dry months characterized by alternating two dry seasons and two wet seasons (the big dry season between mid-November to mid-March, the small wet season from mid March to mid June, the small dry season from mid June to mid August, and the large wet season from mid August to mid November) 38. The average annual temperature of the region is about 23°C (22.8°C in July to 24.6°C in April) 39.

Sampling was done at Mvia in June 11–13, 2007; Nk'leon in July 28–31, 2007; Ndibi, in August 21–26, 2007 and May 2–16, 2008; and Nkouak in August 27–31 2007 and again in May 17–29 2008. Nkouak is the most forested with the lowest human population density with fewer than 1000 people. The village is surrounded by swamps, which are the sources of the Nyong and Bomba rivers. Nkouak has three major vegetation types: (1) secondary forest immediately surrounding the village where locals have planted cocoa, coffee, some palms and other cash crops (2) mature secondary forest where very little human activity occurs, (3) mature forest, which is quite distant from the village and contain major wild life. Ndibi is characterized by secondary forest in various stages of degradation and seasonally flooded swamp forest (September to December) with floating grass plant communities along either side of the Nyong river 39. Ndibi has a comparatively higher human population density and is less than 2 km from the city of Akonolinga (pop. 25, 700) across the River Nyong.

Light trapping (mini CDC light traps) effort per site ranged from four to 15 trap nights. No notable changes in the weather occurred during the collection period that might bias comparisons of mosquito abundance.

In 2007, mosquitoes were collected using six Center for Disease Control (CDC) Miniature Light Traps (Figure 2, 40) baited with CO₂ (John W. Hock, Gainesville, FL), following protocols for proper use and assembly provided with the traps. In the 2008 sampling season, a more comprehensive mosquito collection scheme was carried out in Ndibi and Nkouak that included use of six miniature CDC traps, four net traps (Figure 2, 41), four modified bird baited Ehrenberg lard cans (Figure 2, 42) and sweep net collections of resting mosquitoes in forest vegetation (Figure 2). To escape the heat and wind, mosquitoes rest in more humid conditions under leaves in shaded thick clumps of vegetation. At the collection sites, the surrounding forest offered many such resting sites. The use of CO₂ (John W. Hock, Gainesville, FL) and birds (feral pigeons) as bait in the net traps was alternated. CO₂ sachets and birds (confined within a cage) were placed in the middle of the net trap. In 2008 the lights from the CDC traps were switched off in order to reduce damage to mosquitoes (for morphological identification purposes) that would have been caused by thousands of captured moths and other arthropods attracted to light. In order to fully explore microhabitat preference and help broaden the sampling of the mosquito community, traps of each kind were placed along a vegetation gradient from the floating mat community, through the grass sedge meadow and upland forest and plantations to the swamp forest.

Traps were set out each day for at least 12 h (6.00 pm–06.00 am). Following each trapping period, the collection bags were removed from traps and the mosquitoes immobilized with chloroform and/or smoke within two hours of trap closing. On the same day following the collection and immobilization, mosquitoes were sorted by sex and identified to species with the aid of a stereomicroscope (× 90) and morphological keys 2527. Bird baited and CO₂ baited traps collect predominantly blood-seeking females, and in many African mosquitoes, Culicidae closely related species can only be identified by examination of the male genitalia. This was the primary reason an attempt was made to find males in resting vegetation to identify the more cryptic species assuming that the males would give clues to identification of females collected in the baited traps. Sweep net collections were performed for an hour each day (3.00 pm–4.00 pm) in low-lying grasses and shrubs along the edges of foot paths and clearings in the forest floor. Females collected in the sweep nets were also used for Plasmodium spp. DNA isolation.

Collections were made at 20 sites, in the lowland forests of Cameroon, but trapping effort are analyzed for Ndibi and Nkouak only where more than 95% of Coquillettidia spp. were collected. Although resting mosquitoes were also collected, only mosquitoes collected overnight were used to calculate mosquitoes per trap night. For each site, sampling date, trap type and species, whole unfed and recently fed (blood meal still visible) mosquitoes were pooled separately into groups of between three to 20 individuals, and stored in 95% alcohol in the field and later at -20°C in the laboratory until DNA extraction and subsequent testing by PCR. Minimum field infection rates for estimating Plasmodium spp. infection per thousand pooled mosquitoes were calculated using the bias-corrected maximum likelihood estimation (MLE) methodology with 95% confidence skewness-corrected score intervals 43.

Chi-square analysis was applied to compare maximum likelihood infection rates (MLE) for all the Coquillettidia spp. and the number of isolated Plasmodium spp. infections as a function of the number of mosquitoes collected at each site. All statistical analyses were performed using STATA.

In the laboratory the head and thorax of each mosquito was severed from the abdomens and pooled for DNA extraction. Pools varied in size from 3–20 mosquitoes, and DNA extraction followed modified procedures of Pilchart et al 44 and Ishtiaq et al 18 Briefly, sample pools were homogenized with the aid of heat-sealed pipette tips and 200 μL of total DNA was extracted using the DNeasy Tissue Kit (Qiagen) following the manufacturer's protocol except for the addition of 30 ml of 100 mg/ml dithiothreitol to the tissue digestion buffer 45. The primer pairs L1518 and H15730 were used to amplify ~510 bp fragments of cyt b of the parasites. Each PCR cocktail contained 5.0 μL 10× Qiagen PCR buffer, pH 8.3 (10 mM Tris-CH1, pH 8.3 and 50 mM KC1, 0.01% NP-40), 1.5 mM MgCl₂, 5 μL dNTP mix (10 mmol/L each), 0.3 μL Taq DNA polymerase (1.25 U/reaction), 2.5 μL each primer (0.1–0.5 μmol/L), 1 μL of 10% BSA buffer 46, 2 μL template DNA and the remaining volume of ddH₂O up to 27.7 μL. The PCR thermal regime consisted of one cycle of 5 min at 95°C, 44 cycles of 0.5 min at 95°C, 0.5 min at 50°C, 0.45 min at 72°C, and a final cycle of 5 min at 72°C. Each extraction included a negative control (cocktail without the template DNA), which was screened to detect potential contamination, and a positive control. All positive pools were later subjected to nested PCR protocol 47. In the first PCR reaction, the cyt b gene was amplified using primers HaemNF and HaemNR2 in a 25 μl volume reaction. For the second PCR, 2 μl of the first PCR product was used as template in a 25 μl volume with the primers HaemF and HaemR2, including the same reagents and under the same thermal regime as the first PCR, except that 35 cycles were used instead of 20 cycles.

Additionally, to ensure that the positive results were DNA from sporozoites and not from some undigested parasite infected blood cells that might have persisted in the vector digestive system (as remnants of blood meal), all positive samples were screened for vertebrate DNA using the same thermal regimes for the PCR reaction above, but with primers L14724 and H15149.

Finally, to help ensure that failure to detect a parasite was not due to poor DNA extractions, a fragment (650 bp) of vector COI DNA 48 was also amplified using primers LCO1490 and HCO2198 49.

Positive or negative amplifications were evaluated as the presence or absence of bands on 1.5% agarose gels. Samples that showed positive amplification were subjected to dye terminator cycle sequencing reactions (30 cycles, 55°C annealing), and sequenced on ABI 3730 Genetic Analyzer (Applied Biosystems) automated sequencers, using Big Dye vs. 3.1. For all these samples, the mitochondrial cyt b gene was sequenced in two overlapping fragments using the same primer pairs described above.

Sequences were assembled with Sequencher 4.7 (Gene Codes Corporation, Ann Arbor, MI), aligned in ClustalX and manually corrected by eye. Because the sequences are from coding genes, alignment was straight-forward. Lastly, sequences were confirmed by BLASTN (basic local alignment search tool) to be most closely related to avian Plasmodium spp. cyt b (identical or nearly identical matches to lineages posted in GenBank). Potentially new and unique sequences were checked by additional sequencing of the fragments. The electropherograms were also checked for double nucleotide peaks to infer possible cases of mixed infections of two or more different parasite lineages. The new sequences have been deposited in the GenBank International Nucleotide Sequence Database (Accession numbers: GQ150187–GQ150196).

Phylogenetic analyses were carried out in PAUP* 50. The compiled data set, excluding pools that showed indications of multiple infections, four additional species, Plasmodium juxtanucleare, Plasmodium relictum, P. gallinaceum and Plasmodium elongatum, all of which are known to be transmitted by other mosquitoes 2161751 and three outgroup species of positively identified avian haemoproteids, based on the phylogeny in Valkiūnas et al 4 was used. Additionally, four parasite lineages 3652 recorded from numerous avian host species captured within the tropical lowland forests were included. Phylogenetic relationships of the parasite lineages were estimated using MrBayes 3.1 53. The most accurate available model of sequence evolution, the GTR + G model was used because this level of complexity is warranted due to the extreme AT bias in Plasmodium mitochondrial genes 5455. The Markov chain was sampled every 200 generations for 10 million generations. Bayesian posterior branch probabilities were obtained by taking the majority rule consensus of the sampled trees, excluding the first 12,500 trees as burnin. Replicate runs of the software, each with one cold and three heated chains, produced essentially identical results. Nodal support for the final tree was assessed using ML100 nonparametric bootstrap replicates each with TBR branch swapping. Additionally, PAUP* was used to estimate mean pairwise distances between the different Plasmodium lineages using the Kimura 2-parameter (K2P) model with uniform substitution rate among sites.

Nine wild-caught female C. aurites collected from Ndibi in February 2009 were dissected and salivary glands were isolated on glass slides using traditional mosquito dissection methods 56. The head of insects was cut off with a razor and salivary glands were gently pressed out with a slight pressure by a blunt needle on the thorax near the base of the fore-legs. The glands were placed in a small drop of phosphate buffered saline, ruptured by a gentle pressure of a needle, and mixed with a minute drop of the saline to produce a thin film. The preparations were air-dried and fixed in absolute methanol in the field, and then stained with Giemsa in the laboratory, as described by Valkiūnas 2.

An Olympus BX61 light microscope equipped with Olympus DP70 digital camera and imaging software AnalySIS FIVE was used to examine slides, prepare illustrations and to take measurements. Entire films were examined at low magnification (× 400) and recorded sporozoites were studied at high magnification (× 1,000).

Representative preparations of sporozoites (accession numbers 47721, 47722 NS) have been deposited in the collection of the Institute of Ecology, Vilnius University, Vilnius, Lithuania.

In 2007 and 2008, 10,631 mosquitoes of at least 24 species were collected in Ndibi and Nkouak. Species of Coquillettidia accounted for 17% of the total mosquitoes collected (1,802/10,631) with over 76% captured with CDC light traps alone (Table 1). Coquillettidia aurites was by far the most common of the Coquillettidia species collected, comprising 71% of the species collected in Nkouak and only 9% of the total collected in Ndibi. Coquillettidia metallica accounted for 1.2% of the total, collected mostly in Ndibi and only a single blood fed individual was captured in Nkouak. C. pseudoconopas was captured in Nkouak, Mvia and Nk'leon and accounted for 15% of the total species collected (Table 1). Only one individual of C. maculipennis was captured in Ndibi during the entire season, so this species has been excluded from all the analyses. Relative population densities (light trap counts per trap night), for C. aurites, calculated for each site showed that Nkouak had a significantly higher number than Ndibi. The spatial geographic distribution of the Coquillettidia spp. mosquitoes as a function of habitat use is shown in Figure 3. Although no significant associations were demonstrated between the number of Plasmodium spp. isolations made from mosquitoes and any of the four microhabitats that were analyzed, most species showed (except for C. metallica that was mostly captured in open habitats) a strong preference for swamp forest/upland forest and plantations than more open habitats.

Variation in dark apical scaling of sternites was found among female and male C. aurites with some having no dark scales, others with smattering of scales and in others dark scales formed complete apical bands. Males were collected resting in lower forest vegetation and their genitalia confirmed they were all C. aurites although the membranous expansion of gonostylus was not quite as large as that depicted in Service 25. Images of male genitalia and other morphological features of mosquitoes are deposited in 57.

The number of positive pools in the three species is presented in Table 2. No vertebrate DNA was found in any of the pools, which shows that only DNA of Plasmodium spp. sporozoites (but not of blood stages of the parasites) was amplified. Of the 256 (1285 individuals total) pools screened for Plasmodium spp., 85 (33%) were positive for parasites, yielding a maximum likelihood estimates (MLE) of Plasmodium infections of 112.22/1,000 for C. metallica, 84.04/1,000 for C. aurites and 35.4/1,000 for C. pseudoconopas. Within the two sites however, C. aurites showed a significantly higher MLE in Ndibi than in Nkouak (Ndibi = 116.46/1000; Nkouak = 66.76/1000; χ² = 13.49, p < 0.001), although Nkouak had a higher density of C. aurites (Figure 4). Average mosquito densities within the sites ranged from 39.8 mosquito/trap-night in Ndibi to 115 mosquito/trap-night in Nkouak, whereas the average proportion of corresponding Plasmodium isolations ranged from 45.12% in Ndibi to 28.99% in Nkouak.

Parasite lineages based on 750 nucleotides of cyt b sequence were distinguished after checking carefully against the original chromatograms from the sequencing gel. Parasite sequences differing by only a single nucleotide were considered the same phylogenetic species, while numbered lineages differing by more than one nucleotide substitutions, or at least 0.2% genetic distance were considered separate phylogenetic species. At least eight lineages of Plasmodium spp. were found from the positive pools. Two of them were already known lineages (PV11 and PV12) 36 and six were new lineages that were named by assigning a number in sequential order (PlasCoq1- PlasCoq6). The 8 lineages differed from one another by 0.2 and 15.8% sequence divergence. Some of these are small genetic distances, and likely represent intraspecies divergence of avian Plasmodium 4 although in some cases they are well beyond distances corresponding to good species 5. Cytochrome b sequence divergence as low as 1.0% 58 has been observed between named species of malaria parasites of mammals, although biological 'species' boundaries of avian malarial parasite lineages have not been clearly defined. Of the eight Plasmodium lineages found in this genus, C. aurites harboured seven lineages; C. metallica at least two (including an additional co- infection which was not included in the analysis) and C. pseudoconopas harboured one. The most common lineages (PV11 and PV12) were found to be unevenly distributed in both regions (Figure 4) and represent more than 88% of the lineages recovered from these mosquitoes. The other lineages were found in very few mosquitoes in both locations (Figure 4). Lineage PlasCoq6 is widely divergent from the other lineages, and was only recorded once in a pool sampled from Ndibi. These rare lineages were re-sampled.

Sporozoites were observed in salivary glands of two mosquitoes. Up to three sporozoites were observed in each positive salivary gland smear. They were of elongated shape typical for haemosporidian parasites, with nuclei located approximately at the center (Figure 5). Non-deformed sporozoites (n = 3) averaged 9.9 μm in length and 0.9 μm in width.

Identical lineages identified based on sequence similarity as posted on GenBank were found in parasites isolated from birds belonging to different families of the Passeriformes and non Passeriformes by Blastn search. PV11 36 is an identical match to WA15 52, while PV12 36 is identical to lineages WA9 and P46 352. Over 35 species of birds from 11 families have been shown to be infected with these lineages. The other lineages were relatively rare and together comprised less than 12% of the total parasite load in Coquillettidia spp. Lineages PlasCoq2 and PlasCoq5 however showed a close relationship to PV11 (Figure 6). In general, the parasites obtained from Coquillettidia spp. consisted of closely related lineages also found in birds of different families and these lineages do not appear to be shared with lineages found in other mosquito species so far (Figure 6). While further sampling will be necessary, it is possible that these parasites are only transmitted by Coquillettidia spp.

The likelihood estimates of infection rate (MLE) was examined as a function of the sample size of vectors by asking whether less common species had different infection prevalence than more common species, assuming that species were captured in CDC traps in proportion to their relative abundance. Interestingly, the least and most abundantly sampled species, C. metallica and C. aurites respectively, had the highest maximum likelihood estimates of infection rates (Table 2). Because only few C. metallica were collected, it was not possible to determine if these high estimates of the likelihood infection rates truly reflect the infection rates in nature. More sampling is warranted to confirm this.

Figure 6 summarizes the most important phylogenetic results of this study. Of the 85 pools infected with Plasmodium spp., 81 yielded sequence data of sufficient length to be included in the phylogenetic analysis. The remaining cases (n = 4), showed indications of multiple infections as revealed by double peaks in the chromatogram, and were not included in the analyses. However, some double peaks were easily discernable for parasites lineages PV11 and PV12. All parasites were designated as avian Plasmodium spp. by phylogenetic affinity to published avian Plasmodium spp. cyt b sequences. Support for the nodes, judged by the bootstrap analysis is strong. Examination of the tree revealed no reciprocal monophyly of the Plasmodium spp. lineages detected in Coquillettidia spp., but they clustered together as separate clades with lineages recovered from other culicine species nested within the tree. Known avian parasites, P. relictum and P. elongatum, both of which are transmitted by other vector species 1651 tend to show close affinity to lineage PV12. P. juxtanucleare was most closely related to lineages PlasCoq3 and PlasCoq4. Lineage PlasCoq6 was very rare and was only found once, and this lineage is basal to the tree and equally distant to Plasmodium and Haemoproteus.

This study found that over 90% of the pools of Coquillettidia spp. that were positive consistently harboured certain parasite lineages, which were closely associated to lineages isolated from different bird host groups. All the positive pools were screened for vertebrate DNA to confirm that none had contaminant bird DNA, and the absence of vertebrate DNA from all pools suggests that Plasmodium spp. lineages were isolated from sporozoites rather than amplified from blood stages of the parasites. At least one previous study has suggested that Coquillettidia crassipes is a natural vector of P. gallinaceum and another unidentified Plasmodium sp. in Ceylon 17.

Recently, several new species and lineages of malaria parasites of the subgenus Novyella have been described from African birds, Cyanomitra olivaceae and Andropadus latirostris from the same study sites where Coquillettidia spp. were collected 437. Interestingly, lineages of these parasites were not found in Coquillettidia spp. It is thus probable that these lineages may not be transmitted by Coquillettidia spp., but that Coquillettidia spp. may be important vectors of eight other Plasmodium spp. lineages described in the present study. Species identities of these lineages remain unknown. It is not unprecedented for a malaria parasite lineage to be restricted to infecting limited species within just one mosquito genus (but see Valkiūnas 2 for avian malaria). For instance, five species of anopheline mosquitoes serve as the major vectors for P. falciparum in continental sub-Saharan Africa, and all five species belong to the subgenus Cellia 6465666768. Such strict vector specificity may however, not hold true for avian malaria since these bird parasites are very diverse. In avian malarial systems, the vectors of Plasmodium forresteri, P. elongatum, P. juxtanucleare, P. gallinaceum, and Plasmodium kempi do not belong to same genus 165169. If avian Plasmodium spp. lineages seem to a large extend to be host-generalists 559707172, one would expect expansion of parasites to occur freely if the appropriate vectors are present.

At least eight Plasmodium spp. lineages were found in this study, with two of the lineages, PV11 and PV12 being the most common, occurring in over 88% of the positive pools screened. The reason for the existence of multiple distinct Plasmodium lineages found in mosquitoes of the genus Coquillettidia (seven of which are found in C. aurites alone) is not known, but may provide a plausible explanation for the co-occurrence of two or more parasite lineages in the same vertebrate host 36 and clarify the contrasting views of Oaks et al 64 and Gager et al 73. The former purported that multiple parasite species that share a vertebrate host could be transmitted by the same mosquitoes genera or species, while the latter's explanation for co-occurrence of congeneric malarial parasites in an avian host to transmission by mosquitoes of different genera. Further work with multiple independent markers from different parts of the Plasmodium spp. genome should be carried out to clarify species limits.

The genetic distance between recorded lineages ranged between 0.2% and 17.4%. Because genetic differences between lineages PV11, PlasCoq2 and PasCoq5 are small (Figure 6), it is possible that these three lineages represent genetic variations of the same species, as has been shown to be the case with numerous lineages of avian P. relictum and several avian Haemoproteus spp. 437. Lineages with genetic distances of <5% in cytochrome b gene has been shown to be a measure representing intraspecific variation in avian Plasmodium spp, although there are exceptions to this rule 4. Thus, the molecular criterion of > 5% sequence divergence in cytochrome b gene for identification of haemosporidian species should be applied only through the careful linkage of molecular and microscopical data. Some of the genetic distances observed in this study are within this range, and higher than the average pairwise distances between Plasmodium cytochrome b sequences from many other avian malaria studies 74, as well as the average cytochrome b distance among three most closely related human malarial parasites that are known to be different species, i.e. Plasmodium vivax, Plasmodium malariae and Plasmodium ovale 58.