India contributes 1.5–2 million annual confirmed cases of malaria. Since both parasites and vectors are evolving rapidly, updated information on parasite prevalence in mosquitoes is important for vector management and disease control. Possible new vector-parasite interactions in Goa, India were tested.
Methods
A total of 1036 CDC traps were placed at four malaria endemic foci in Goa, India from May 2013 to April 2015. These captured 23,782 mosquitoes, of which there were 1375 female anopheline specimens with ten species identified using morphological keys. Mosquito DNA was analysed for human and bovine blood as well as for Plasmodium falciparum and Plasmodium vivax infection.
Results
Human host feeding was confirmed in Anopheles stephensi (30 %), Anopheles subpictus (27 %), Anopheles jamesii (22 %), Anopheles annularis (26 %), and Anopheles nigerrimus (16 %). In contrast, Anopheles vagus, Anopheles barbirostris, Anopheles tessellates, Anopheles umbrosus and Anopheles karwari specimens were negative for human blood. Importantly, An. subpictus, which was considered a non-vector in Goa and Western India, was found to be a dominant vector in terms of both total number of mosquitoes collected as well as Plasmodium carriage. Plasmodium infections were detected in 14 An. subpictus (2.8 %), while the traditional vector, An. stephensi, showed seven total infections, two of which were in the salivary glands. Of the 14 An. subpictus infections, nested PCR demonstrated three Plasmodium infections in the salivary glands: one P. vivax and two mixed infections of P. falciparum and P. vivax. In addition, ten gut infections (one P. vivax, six P. falciparum and three mixed infections) were seen in An. subpictus. Longitudinal mosquito collections pointed to a bimodal annual appearance of An. subpictus to maintain a perennial malaria transmission cycle of both P. vivax and P. falciparum in Goa.
Abkürzungen
CDC
Centres for Disease Control and Prevention
CSP
circumsporozoite protein
DDT
dichlorodiphenyl trichloroethane
DNA
deoxynucleic acid
ELISA
enzyme linked immune sorbent assay
HBI
human blood index
ICEMR
International Centre of Excellence for Malaria Research
MESA
Malaria Evolution in South Asia
NIAID
National Institute of Allergy and Infectious Diseases
NVBDCP
National Vector Borne Diseases Control Programme
PCR
polymerase chain reaction
RNA
ribose nucleic acid
USA
United States of America
UV
ultraviolet
WHO
World Health Organization
Background
India contributes significantly to the total malaria burden in the world with about 1.5–2 million confirmed malaria cases and annual death estimates ranging from 15,000 to 95,000 [1, 2]. The epidemiology of malaria in India is complex due to the geo-ecological diversity of the country, multi-ethnicity of human hosts, wide distribution of different anopheline species, and extensive human mobility within the country and from outside [1]. Historically, the 1950s malaria eradication programme in India, led by World Health Organization (WHO) and focused on vector control using indoor residual insecticide DDT, was considered a success. Malaria incidence in humans decreased from about 75 million in 1947 to less than 100,000 in 1964 [1]. Malaria was then thought to be on the verge of eradication in India, but it re-emerged in 1976 [3].
Areas with unstable malaria present an important opportunity to re-examine human-parasite-vector interactions that contribute to the transmission of malaria. Traditionally, there are six recognized primary vectors of malaria in India, viz., Anopheles culicifacies, Anopheles stephensi, Anopheles dirus (Anopheles baimaii), Anopheles fluviatilis, Anopheles minimus and Anopheles sundaicus. Vectors of secondary importance are Anopheles annularis, Anopheles varuna, Anopheles jeyporiensis and Anopheles philippinensis [4]. Anopheles stephensi has been incriminated repeatedly and strongly in different parts of India. The species is capable of transmitting malaria at very low densities and is an important urban malaria vector in the country [4].
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In the coastal belt of Goa, following a 1986 malaria outbreak in urban Panaji, An. stephensi was extensively studied for its role as the primary vector in malaria transmission in terms of both its resting and biting behaviour and its breeding habits [5‐8]. A recent study carried out in Goa showed that one out of 54 An. stephensi was positive for P. falciparum malaria infection with CSP ELISA [9]. The prevailing view has been that other anopheline species do not contribute significantly to malaria transmission along the Western Coast, including Goa. In addition to An. stephensi in urban areas, Goa also has at least two other recognized rural malaria vectors, An. culicifacies and An. fluviatilis [8, 10]. Anopheles culicifacies is found in low densities in the sub-coastal belt of Goa where it breeds in irrigation channels, ponds and rice paddies and An. fluviatilis is abundant in the eastern hilly regions of the state where it breeds in stagnant waters in streams and paddy fields [8, 10]. There have been reports of An. dirus in forested hinterlands of Goa, but it has not been extensively studied for its role in malaria transmission [11].
The present study involved a broad and unbiased re-assessment of vectorial capacity of all significant Anopheles mosquitoes in urban Goa. This was motivated, in part, by the MESA-ICEMR hypothesis that parasites and mosquitoes may change their relationships as each comes under increasing pressure from malaria control programs [13, 14]. Other basic science studies show that parasite populations have powerful strategies to select for beneficial changes in their haploid genome without collateral damage [12, 14, 15]. While this has previously been of interest with respect to acquisition of resistance to anti-malarials, it is possible that interactions between parasites and vectors may also be fluid. Unproductive interactions between human malaria parasites and non-vector anophelines may evolve so that human malaria parasites develop successfully in Anopheles mosquitoes not suspected to be productive hosts [16]. Continual broad investigation into the role of local anopheline species in malaria transmission areas was, thus, considered important.
Here, nested PCR was employed and both Plasmodium falciparum and P. vivax were detected in the salivary glands and guts of wild anopheline mosquitoes collected from Goa. The results show that anophelines other than An. stephensi may participate in the propagation of human malaria in urban Goa and that parasites may exploit multiple vectors to maintain perennial transmission in Goa. The findings and this particular open-ended approach may have important implications for vector control strategies in urban India, particularly in Goa.
Methods
Study area and time
Goa, a state covering a geographical area of 3702 km2, is situated on the West Coast of India. It has a population of 1.5 million residing in two districts (North and South Goa) [8]. Construction sites located in Panjim, Candolim, Porvorim (North Goa) and Margao (South Goa) were identified as focal points for the malaria transmission study based on data received from Goa Directorate of Health Services, local Urban and Primary Health Centres, and malaria patient data from MESA-ICEMR operations at Goa Medical College and Hospital. Such targeted deployment of CDC traps maximised the possibility of capturing malaria vectors within active transmission zones. This paper analyses the human and bovine blood meal and the presence of human Plasmodia in the mosquitoes collected from May 2013–April 2015 in Goa.
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Mosquito collection
CDC traps (John W. Hock, USA) with UV lights and 6 V batteries were used for trapping mosquitoes. Verbal informed consent was obtained from construction-site engineers and from house owners prior to trap deployment. People residing around the collection sites were informed of the study and they helped protect the traps from disturbance. Traps were hung inside labourer’s shelters at 6 pm and collected at 9 am the following morning, avoiding shelters where firewood was used for cooking. The shelters where collections took place were not sprayed with any insecticides.
Identification and preservation of mosquitoes
Following deployment and recovery of traps, the mouth of each collection bag was secured to prevent escape of mosquitoes. The bags were separated from trap machines and transported to the NIMR-Goa laboratory with care to avoid damage to the mosquitoes.
Back at the NIMR-Goa lab, the freshly collected mosquitoes were anesthetized with diethyl ether and identified using standard morpho-taxonomic keys [17, 18]. Morphological features used for identification were head, proboscis, thorax, legs, wings and palpi. The mosquitoes were individually placed in 1.5 mL microfuge tubes. The tubes were labelled with specific codes, sealed and placed in separate boxes designated to capture information on origin of the mosquito (including the time, place, and exact trap they came in). The samples were preserved at −80 °C for further analysis.
DNA extraction
Mosquitoes collected from May to July 2013 were not separated prior to DNA extraction. The rest of the mosquitoes were dissected into two parts, head/thorax (H) and abdomen (A) by making a sharp cut between the thorax and abdomen. The legs and wings were detached from the main body and stored separately at −80 °C. Genomic DNA from whole mosquitoes or individual parts (H and A) of each anopheline mosquito was extracted using QIAamp DNA Mini Kits (Qiagen, Germany). Isolated DNA, eluted in 100 µL nuclease free water (Ambion) was then stored at −80 °C for further use. DNA extracted from individual head and abdomen parts was used as the template for the PCR reaction, except for mosquitoes collected from May to July 2013. In these cases, DNA extracted from the whole mosquito was used as a template.
Blood meal analysis
To determine the potential anthropophagic nature of the mosquitoes, abdomens were screened for the presence of human and bovine blood by PCR using specific primers derived from ribosomal RNA intergenic spacer sequence of Homo sapiens and mitochondrial DNA (mtDNA) of Bos taurus respectively (Table 1). The PCR conditions were: initial denaturation at 95 °C for 4 min followed by 35 cycles of denaturation at 95 °C for 30 s, annealing at 50 °C for 30 s, extension at 72 °C for 1 min and final extension at 72 °C for 8 min [19]. Anopheles stephensi and An. subpictus were also screened for bovine blood using specific primers by PCR as described by Corona et al. [20]. The PCR conditions were: initial denaturation at 95 °C for 2 min; 10 cycles of denaturation at 94 °C for 1 min, annealing at 58 °C for 1 min, extension at 72 °C for 1 min 30 s; 20 cycles of denaturation at 90 °C for 1 min, annealing at 58 °C for 1 min, extension at 72 °C for 1 min 30 s; and final extension at 72 °C for 10 min.
Table 1
Primers for detection of human blood, bovine blood and malaria parasites
The sibling species identification of An. subpictus using allele-specific PCR was carried out using the gene specific ITS2 region and confirmed by sequence analysis. The PCR conditions were: initial denaturation at 95 °C for 4 min, followed by 35 cycles of denaturation at 95 °C for 30 s, annealing at 50 °C for 30 s, extension at 72 °C for 1 min, and final extension at 72 °C for 8 min.
Mosquito infection status
The mosquito samples were screened for Plasmodium by PCR, initially using genus specific universal primers (28S rDNA specific universal primer set) (Table 1) [21, 22]. The following mixture was subjected to Plasmodium universal PCR: 1.5 µL 10X PCR buffer (500 mM KCl, 200 mM Tris-HCl), 1.0 µL of 50 mM MgCl2, 2.5 µL of 2.5 mM dNTPs each (GeNei, Bangalore), 0.5 µL oligonucleotide primers (Eurofins Genomics India Pvt Ltd) 20 pM/µL each, 0.5 µL (5 units/µL) of Taq polymerase (Invitrogen), 3.5 µL of nuclease free water (Ambion) and 15 µL of template DNA in a final volume of 25 µL. The PCR conditions were set as follows: initial denaturation at 94 °C for 5 min followed by 40 cycles of denaturation at 94 °C for 30 s, annealing at 55 °C for 1 min, extension at 72 °C for 2 min, and final extension at 72 °C for 5 min.
Species-specific nested PCR
In order to identify the species of Plasmodium in the infected mosquitoes, the initial amplified PCR product was generated using genus specific primers. This was then purified using Qiagen PCR purification kits and subjected to nested PCR using species specific primers [19, 21, 22]. Nested PCR was performed using the following mixture: 2.0 µL 10X PCR buffer (500 mM KCl, 200 mM Tris-HCl), 1.0 µL (50 mM MgCl2), 2.0 µL (2.5 mM of each dNTPs), 0.5 µL of each primer (20 pM/µL), 0.5 µL (5 units/µL) of Taq polymerase, 8.5 µL of nuclease free water and 10 µL of PCR product in a total volume of 25 µL. The PCR conditions were: initial denaturation at 94 °C for 5 min followed by 40 cycles of denaturation at 94 °C for 1 min, annealing at 55 °C for 2 min, extension at 72 °C for 2 min, and final extension at 72 °C for 5 min.
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Data and sample management
REDCap electronic data management tools were utilized to record all information related to trap placement, collection and mosquito identification [23]. A FreezerPro database was used to manage mosquito and mosquito derivative storage. Data recorded in both systems were available to MESA-ICEMR partner labs in both India and the USA in real-time.
Results
Anophelines collected with CDC traps
A broad and unbiased approach was taken to determine which anopheline species in Goa may currently be transmitting human malaria. In all 23,782 mosquitoes belonging to 27 species were collected including 16,201 females and 7586 males. A total of 1375 anopheline mosquito specimens were caught in 1036 traps deployed during the study period. This collection included ten Anopheles species. One of the two dominant anopheline species was the well-studied urban and semi-urban vector An. stephensi (334, 24.3 %). Another abundant vector in the traps was An. subpictus (501, 36.4 %), actually out numbering An. stephensi. Together, the two species constituted 60.7 % of the total anophelines trapped. There were eight other less abundant anopheline mosquito species in the traps, including 363 An. jamesii (26.4 %), 66 An. vagus (4.8 %), 57 An. annularis (4.1 %), 36 An. nigerrimus (2.6 %), 9 An. barbirostris (0.6 %), 7 An. tessellates (0.5 %), and 1 each of An. umbrosus and An. karwari.
Seasonality of the dominant anophelines
Not only were the absolute numbers of captured An. subpictus higher than those of An. stephensi, but An. subpictus showed a wider annual prevalence. As shown in Fig. 1a (red line), An. subpictus mosquitoes were captured in high numbers from May to July (117/501, 23.3 %), but prevalence continued later including a prominent peak between December and April (334/501, 66.7 %). For reference, the rainier months in Goa are from May to October and the dry period is from November to April (Fig. 1b, green bars). As expected and as shown in Fig. 1a (blue line), the conventional vector An. stephensi collections were most abundant during the monsoon months of May to October (226/334, 67.6 %), but the numbers of An. stephensi decreased during the drier months with the 6 months of November to April yielding 108 An. stephensi (32.4 %).
Fig. 1
Relationship between vector buildup, infected mosquitoes, rainfall in Goa, and numbers of malaria patient cases in Goa. aAnopheles stephensi and Anopheles subpictus prevalence from May 2013 to April 2015 (blue and red lines, respectively) and times of mosquito Plasmodium infections from May 2013 to April 2015 (squares and trianglesabove the lines). Each spot depicts one Plasmodium infection/mosquito in different months. The colour key is as follows: Blue square: An. stephensi (Pv + Pf), Green square: An. stephensi (Pv), Red square: An. stephensi (Pf), Blue triangle: An. subpictus (Pv + Pf), Green triangle: An. subpictus (Pv), Red triangle: An. subpictus (Pf). b Seasonal variation in traps placed (purple line with triangles), rainfall (green bars), humidity (plain purple line). The scale on the left applies to all three measurements (number of traps, rainfall in cm, and humidity in % value). c Annual distribution of malaria cases at clinics and hospitals in Goa
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Blood meal analysis of the anophelines
It was important to test whether An. subpictus, as expected for An. stephensi, was biting human hosts. Indeed, when tested for human blood with PCR (Fig. 2), the two most prevalent Anopheles species were positive for human blood at comparable frequencies.
Fig. 2
Demonstration of human blood in representative mosquitoes. PCR amplification of ribosomal RNA intergenic spacer sequence (rDNA) of H. sapiens: Lane 1 100 bp DNA ladder; Lane 2 and Lane 3An. stephensi (519 bp; sample ID, ST65 and ST66); Lane 4An. subpictus (519 bp; sample ID, SP28); Lane 5 Negative control (nuclease free water)
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Out of 334 An. stephensi, 100 were positive for human blood (29.9 %), but none for bovine blood. Of these, 15.4 % An. stephensi assayed were positive for human blood during the monsoon phase (May–October) and 14.5 % were positive during the dry period (November–April), showing no seasonal variation. Out of 501 An. subpictus, 135 were positive for human blood (26.9 %) and only six were positive for bovine blood (1.2 %). In contrast with An. stephensi, 2.4 % An. subpictus assayed were positive for human blood during the monsoon phase and 24.1 % were positive during the dry period, showing significant seasonality.
Three additional anopheline species were positive for human blood: 80 An. jamesii (21.9 %), 15 An. annularis (25.9 %), and 6 An. nigerrimus (17.1 %). None of the remaining five Anopheles species tested positive for human blood.
Plasmodium infections
To determine which anophelines in the collection harboured human malaria parasites, diagnostic PCR was conducted on each of the anopheline mosquitoes. In the case of An. subpictus, Plasmodium infection was seen in 2.8 % (14/501) of specimens as revealed by PCR amplification of a 1100 bp DNA fragment using Plasmodium specific universal primers (Fig. 3). In addition, nested PCR was used to identify the species of Plasmodium causing infection (Fig. 4). Out of these 14 An. subpictus positive for the Plasmodium genus, two (0.6 %) showed P. vivax mono-infection, six (1.2 %) showed P. falciparum mono-infection, and another six (1.2 %) harboured a mixture of P. vivax and P. falciparum confirmed by nested PCR (Table 2). The infectivity rate based on salivary gland positivity in An. subpictus (0.6 %) was comparable to that of An. stephensi.
Fig. 3
Demonstration of successful PCR amplification of Plasmodium DNA using universal primers to detect an infection. Lane 1 & 3 (Negative controls); Lane 5 negative control (Nuclease free water); Lane 2 positive (1100 bp; Sample ID, SP328); Lane 4 (500 bp DNA ladder)
Fig. 4
Demonstration of representative nested PCR amplification to detect P. vivax (a) and P. falciparum (b): aLane 1,2,3,4An stephensi (Mosquito sample ID, ST24, ST31, ST32, ST54) positive for P. vivax; Lane 5An. subpictus positive for P. vivax (SP12); Lane 6 100 bp DNA ladder bLane 1 100 bp DNA ladder, Lane 2,3,4,6,8,9,11,12 (Negative, Sample ID, SP315, SP322, SP325, SP369, SP386, SP389, SP392, SP 399). Lane 5, 7 are positive for An. subpictus (SP328, SP371) and Lane 10 is positive for P. falciparum in An. stephensi (ST298)
Table 2
Detection of Plasmodium species in Anopheles subpictus and in Anopheles stephensi
Vector species
No. Plasmodium +ve/assayed
Parts of mosquito tested
Number tested
Only Pv
Only Pf
Pv + Pf
Total positive
Infection/infectivity rate (%)
An. subpictus
14/501
Whole
25
0
0
1
1
2.8b
Abdomen
476
1
6
5 (2a)
12 (2a)
Head
476
1
0
2a
3 (2a)
0.6c
An. stephensi
7/334
Whole
56
3
0
1
4
2.1b
Abdomen
278
0
2 (1a)
1a
3 (2a)
Head
278
0
1a
1a
2a
0.6c
PvP. vivax; PfP. falciparum
aIndicates same mosquito tested positive for both head and abdomen hence counted once
bIndicates infection rate
cIndicates infectivity rate
×
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For comparison, Plasmodium infection was seen in 2.1 % (7/334) of the traditional vector An. stephensi as revealed by PCR amplification of an 1100 bp DNA fragment using Plasmodium specific universal primers (Fig. 3). In addition, three out of the seven infected An. stephensi were positive for P. vivax alone (120 bp amplicon), two (0.6 %) had P. falciparum alone (205 bp band size) and another two (0.6 %) contained both P. vivax and P. falciparum (Table 2; Fig. 4). Finally, anthropophily of the two vectors that were positive for human malaria parasites were cross-checked. Seven of the 14 Plasmodium positive An. subpictus also showed a positive reaction for human blood as did five of the seven An. stephensi positive for Plasmodium.
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A preliminary study using allele-specific PCR suggests that both sibling species A and B of An. subpictus occur in equal proportions. Three An. subpictus sibling species ‘B’ were Plasmodium positive in the salivary glands, suggesting a role in malaria transmission in Goa. The role of other An. subpictus sibling species in malaria transmission needs to be further investigated.
Temporal distribution of vector infections in urban Goa
The time frames for Anopheles species with P. falciparum and P. vivax infections allowed first glimpses of when each mosquito species was most active at transmitting malaria. The conventional vector, An. stephensi, was most active as a vector from May to July. Unlike An. stephensi, An. subpictus were found positive for malaria parasites from December to April as well as May to July (Table 3; Fig. 1a). This may help explain ongoing malaria cases being reported during these months at local clinics and hospitals (Fig. 1c).
Table 3
Transmission periods assessed by times of positive specimens in the CDC trap collections
Vector
P. vivax
P. falciparum
P. vivax + P. falciparum
An. subpictus
May 1
January 1
January 2
June 1
February 4
March 2
March 1
April 1
June 1
An. stephensi
June 3
June 1
March 1
August 1
July 1
The seasonal analysis of anthropophagic index of these two vector species and their specimens positive for human Plasmodium showed good correlation in the case of An. subpictus. While 3/501 (0.6 %) An. subpictus were positive for human Plasmodium species during the pre-rainy season, its anthropophagic index was found to be 2.8 %. In contrast, 121/501 (24.1 %) An. subpictus were positive for human Plasmodium species during the dry period while its infection rate was 2.2 %. In contrast, during the rainy season 6/334 (1.8 %) An. stephensi tested Plasmodium positive while its anthropophagic index was 14.4 %. In the dry period, in spite of a 15.6 % human blood index, the Plasmodium infection rate was only 0.3 %.
Geographic distribution of vector infections in urban Goa
The presence of An. subpictus and its infectivity was not restricted to one specific part of urban Goa. In the present study, 343, 218, 124 and 150 CDC traps were placed in Panaji, Candolim, Porvorim and Margao, respectively, for a total of 1036 traps (Table 4). There was an even distribution of infected versus uninfected mosquitoes in traps between the different towns. The Plasmodium infection in An. subpictus and An. stephensi, were 8 (2.3 %), 4 (1.8 %), 4 (3.2 %), and 5 (3.3 %), respectively, in these four locations. On average, 2.0 % of the CDC traps captured infected mosquitoes.
Table 4
Anophelessubpictus and Anopheles stephensi collections and their infection status at multiple sites in Goa
Locality in Goa
No. of traps
No. of Anopheles
Mean Anopheles vectors/trap
No. AnophelesPlasmodium+ve (IR %)
% Trap with infected vectors
stephensi
subpictus
Total
Panaji +
328
142
201
343
1.04
8 (2.3)
2.4
Candolim
245
85
133
218
0.88
4 (1.8)
1.6
Porvorim
176
47
77
124
0.70
4 (3.2)
2.3
Margao
287
60
90
150
0.52
5 (3.3)
1.7
Total
1036
334
501
835
0.8
21 (2.5)
2.0
Panaji+ Panaji and surroundings, IR combined infection rate in vectors
Discussion
Traditional views of major urban malaria vectors in western India do not include An. subpictus. While An. subpictus infected with P. falciparum and P. vivax is new in Western India, and in Goa in particular, An. subpictus has been reported as a malaria vector in Sri Lanka, Eastern and Central India, Maldives and several other parts of South and South East Asia [24‐31].
In the present open-ended study, CDC traps were continuously deployed in four malaria endemic towns of Goa over a period of two years. An. subpictus was found to harbour Plasmodium alongside An. stephensi in Goa. Salivary gland positivity further suggested that An. subpictus was capable of propagating both P. vivax and P. falciparum in humans in Goa. The present collection showed one of the highest reported figures for An. subpictus testing positive for human blood in an urban area [28]. Furthermore, An. subpictus showed an infection rate of nearly 2.8 % and an infectivity rate of 0.6 % (Table 2), which is comparable to earlier findings [27]. Other known malaria vectors in non-urban and forested areas of Goa, An. culicifacies and An. fluviatilis, were not caught in CDC traps, confirming earlier findings [6, 8, 9].
It was surprising and important to note that not only was An. subpictus the predominant anopheline mosquito, but that it also had two prevalence peaks during the year. Anopheles subpictus showed a wider window of transmission from December to April and then again from May to July, overlapping with the An. stephensi peak transmission. It appears that the two vectors work in tandem to sustain continual malaria transmission throughout the year. Without An. subpictus, An. stephensi may not be able to sustain transmission through the drier months itself.
An interesting question is how An. subpictus is better able to propagate than An. stephensi during the dry season of December to April. While An. stephensi breeds mainly in manmade habitats in Goa such as curing waters, masonry tanks, terraces, lintels, overhead tanks and wells, An. subpictus additionally breeds in a variety of natural puddles, pools, ponds, pit wells, rice paddies and backwaters [5, 6]. This wider choice of breeding habitat may give An. subpictus one advantage over An. stephensi. Detailed work on the south coast of Java showed the salt water sibling species ‘B’ of An. subpictus complex positive for sporozoite infection in salivary glands [32, 33]. The fact that An. subpictus can breed in fresh water as well as salt water systems, where it can tolerate a very high degree of salinity, may have important implications for its ability to breed year round [4].
One important outcome of this study is that continual, open-ended surveys of all potential vectors of human malaria transmission can be an effective monitoring tool to guide control strategies, particularly in urban areas, and may help identify conventionally overlooked vectors.
Conclusions
The present study shows the presence of P. vivax and P. falciparum in both salivary glands and mid-guts of An. subpictus in Goa, India. The study highlights that An. subpictus is more prevalent than the recognized primary urban vector, An. stephensi in the coastal region of Goa. There is high probability that An. subpictus contributes to the propagation of malaria in urban Goa especially during the post-monsoon period when An. stephensi numbers decline. Given that An. subpictus is present throughout India and Asia and can breed year-round in coastal areas, monitoring and further study of An. subpictus should be an integral part of national urban vector control measures in Asia.
Authors’ contributions
AM, MN, TS, SJ, RH, AS, and SK performed the experiments and analyzed the results. TS, AM, AK, LC, and PR wrote and edited the manuscript. AK, NV, LC and PR designed and administered the study. All authors read and approved the final manuscript.
Acknowledgements
This work was supported by the US NIAID MESA-ICEMR Program Project U19AI08688 (NIH) to the University of Washington, Seattle, WA, USA, and by the Government of India (Indian Council of Medical Research and the National Institute of Malaria Research). The authors thank Jennifer Maki and Suresh Kumar M. of the University of Washington, and Siddhatray Tari, Shamu Angalkurthi, Prathmesh Ghavanalkar and Chetan Dabhale, Sushma Bhinge, Pallavi Borkar, Priyanka Raikar, Hemanth Kumar, and additional support staff of NIMR. This manuscript was approved by the publication committee of NIMR and bears approval No.058/2015.
Competing interests
The authors declare that they have no competing interests.
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