Background
Plasmodium vivax poses a serious threat to half of the world’s population, including the whole of South Asia [
1]. In 2015, an estimated 13.8 million cases were caused by
P. vivax [
2]. India, Pakistan and Ethiopia are estimated to contribute greater than 80% of
P. vivax cases in the world [
2]. Hypnozoites, the dormant liver forms that are unique to
P. vivax and
Plasmodium ovale, can spontaneously re-activate and lead to periodic clinical relapses [
3]. Many of the asymptomatic
P. vivax infections in endemic areas are caused by hypnozoites [
4] and these sub-clinical infections are difficult to detect, and thus complicate control measures.
Until now, in the absence of a culture system for continuous development of
P. vivax, most of the knowledge on
P. vivax is based on experimental and natural human infections [
4‐
7]. For example, unlike
Plasmodium falciparum, which invades all stages of erythrocytes,
P. vivax selectively invades reticulocytes [
6,
8‐
10].
P. vivax sexual development takes place in vectors when they ingest mature, infective gametocytes circulating in the peripheral blood [
6,
11]. Compared to
P. falciparum, gametocytes are more commonly observed in
P. vivax infections [
12], and they appear in blood smears much earlier in an infection [
13]. Although clinical studies have shown that blood from asymptomatic, sub-microscopic gametocyte infections can infect mosquitoes, the correlation between
P. vivax gametocytaemia and mosquito infections have been variable, with studies showing positive [
14,
15], weak [
5,
16,
17] and poor correlation [
18‐
20]. Studying gametocytes in human blood is further complicated by the fact that the conventional microscopic techniques used for counting gametocytaemia are not always accurate and could contribute to the over- or underestimation of parasites in patient blood smears [
21‐
24]. Furthermore, in controlled mosquito infections, the correlation between midgut oocyst numbers and salivary gland sporozoite load in
P. vivax infections is not well understood. Successful mosquito infection of
Plasmodium could be influenced by a number of parasite, vector and human factors including the state of gametocyte maturation, proportion of male and female gametocytes, variation in parasite genetics and transmission-blocking antibodies [
11,
25‐
30]. Additionally, mosquito factors such as age, genetic diversity and microbiota could potentially affect the
P. vivax infection rate and oocyst load [
26,
31‐
33]. Many of the above uncertainties in studying the complex life cycle of
P. vivax may be overcome with controlled feeding experiments.
The standard membrane feeding assay (SMFA) and direct skin feeding are the two most commonly used techniques for controlled mosquito infections studies [
34]. Although direct skin feeding is more sensitive [
34], ethical considerations and practical constraints favour the use of SMFA at many endemic sites.
As a part of the US NIH International Centers of Excellence for Malaria Research (ICEMR) [
35‐
37], the Malaria Evolution in South Asia (MESA) programme has set up a controlled mosquito-feeding laboratory at the MESA-National Institute of Malaria Research (NIMR) joint study site in Panaji, Goa, India. For mosquito-feeding experiments,
P. vivax-infected blood was obtained from patients recruited at the nearby Goa Medical College and Hospital (GMC), the other MESA study site in Goa [
38]. To better understand the dynamics of parasite development in mosquitoes in southwestern India, 30 laboratory-feeding experiments were conducted with wild
An. stephensi [
39,
40] and
P. vivax-infected patient blood. This paper describes the importance of patient blood parasitaemia and gametocytaemia on successful mosquito infection, as measured by oocyst numbers and sporozoite load. The potential role of Indian mosquito immunity in controlling
P. vivax sporozoite load is also described.
Methods
Wild An. stephensi larvae collection and maintenance
Wild An. stephensi larvae and pupae were collected from breeding habitats, the curing waters in construction sites, around Ponda city in the state of Goa, India. The mosquito larvae and pupae were collected using the dipping technique and were transferred, along with breeding water, to plastic containers. The containers were then brought to the MESA insectary at the NIMR Goa field station. In the insectary, third and fourth instar larvae were separated from the first and second instar larvae and were reared separately. Pupae collected from the field were kept in 500-ml plastic bowls containing 200 ml of tap water, and inside a closed cage for controlled emergence. The larvae were reared in plastic trays containing tap water under laboratory conditions at 27 ± 2 °C, 70 ± 5% relative humidity and 12 h light/12 h dark photoperiod cycling. A pinch of Cerelac® powder (Nestle) and fish food (1:1) mixture was given to the larvae once a day until pupal stage development was visible. Once formed, pupae were collected in fresh plastic bowls containing tap water, and then kept inside a closed cage for emergence of adults. The adult mosquitoes that emerged from these pupae were given 10% glucose soaked in a cotton pad. The species of emerged adult mosquitoes were identified using standard morphological keys.
Ethics and approvals
The human subjects protocol governing collection of malaria parasites at GMC was approved by the Institutional Ethics Committee of Goa Medical College and Hospital, the University of Washington Institutional Review Board and by the US NIH/NIAID Division of Microbiology and Infectious Disease (DMID). The MESA-ICEMR programme project was additionally approved by the Health Ministry Screening Committee (HMSC) of the Government of India and by the Government of Goa Public Health Department.
Blood collection from P. vivax patients
Plasmodium vivax patients confirmed by microscopy at GMC were briefed about the study by the project staff, and volunteers were recruited for the study. Prior to blood collection, informed consent was obtained from each patient. Approximately 6 ml of blood was drawn into an acid citrate dextrose vacutainer by venipuncture. Immediately after collection, the vacutainer was placed in a thermos flask maintained at 37 °C and was transported to the mosquito infection laboratory at NIMR-Goa.
Mosquito-feeding experiments
Six to seven days old, adult, female mosquitoes were used for all the experiments. Female mosquitoes were caught using an aspirator and were transferred to plastic cups covered with mesh netting secured by a rubber band and a cup lid. Approximately 125 mosquitoes were placed in each cup. These mosquitoes were starved for 16–18 h prior to blood feeding. The close proximity of the malaria patient pool at GMC helped in receiving the patient blood at NIMR-Goa within one-and-a-half hours from the time of blood draw. Within minutes of arrival at NIMR-Goa, 2 ml of infected blood was added to a 5-cm wide water-jacketed membrane feeder fitted to a circulating water bath maintained at 37 °C. The feeder was positioned in the centre of the plastic container holding the mosquitoes. The blood was maintained at 37 °C during the entire 90-min feeding time to avoid premature exflagellation. After feeding, unfed mosquitoes were separated from fully engorged ones using an aspirator. The plastic cup containing the fully fed mosquitoes were kept in Percival incubators at 27 °C ±2 and 80% ±2 relative humidity. A cotton pad soaked in 10% glucose solution feed was provided until the mosquitoes were dissected at various time points (see below).
Mosquito dissections and microscopy
For oocyst dissection on days 7/8 post blood feeding, five mosquitoes at a time were caught using a glass aspirator and were transferred to a test tube, which was then plugged with cotton. The test tube was placed in a −20 °C freezer for 2–3 min to immobilize the mosquitoes. Once the mosquitoes were knocked down, the test tube was placed on ice. Proboscis, wings and legs were first dissected to prevent accidental escape of infected mosquitoes. The dissected midgut was placed in a drop of 2% mercurochrome in PBS on a microscope slide with a coverslip, and examined for oocysts. The oocysts were counted using a phase contrast microscope at 5× and 10× (Carl Zeiss Axio Lab. A1). Salivary glands were dissected on different days post-infection, and were imaged at 40× magnification with a phase contrast microscope (Carl Zeiss Axio Lab. A1). Oocysts and sporozoites were counted independently by two project staff. The sporozoite load was calculated based on earlier studies [
19,
41], and the gland index was recorded as: 1+ for (1–10 sporozoites), 2+ for (10–100 sporozoites), 3+ for (101–1000 sporozoites), 4+ for (>1000 sporozoites). In the present study, oocyst infection rate indicates the percentage of mosquitoes that contain one or more oocysts in a feeding experiment. Average oocyst load indicates the average number of oocysts in a population of mosquitoes in a feeding experiment. Sporozoite infection rate indicates the percentage of mosquitoes that contain one or more sporozoites in a feeding experiment.
Patient blood parasite counts
Thin and thick smears were prepared with the donor patient blood and were stained with a 10% Giemsa solution. Patient blood parasitaemia and gametocytaemia in thin smears were counted by two trained technicians. Counting was done by the Miller reticule technique [
42], and for every smear, 100 fields were counted. The ratio of large reticule to small reticule was calculated by ImageJ software, and was 4:1. The reticule factor was 25.
Statistics
Statistical analysis was performed using the GraphPad Prism software. Pearson correlation was used to determine the significance of correlation between the counts of two independent slide readers. Linear regression was used to study the correlation between donor blood gametocytaemia and parasitaemia, and successful mosquito infections. The correlation between average oocyst load and sporozoite load was also evaluated using linear regression.
Discussion
Controlled laboratory-feeding experiments can help in understanding the development kinetics of
Plasmodium in its vector [
5,
6,
43]. Mosquito-feeding experiments were carried out using wild
An. stephensi mosquitoes that emerged from field-caught larvae. In contrast, to date, most of the
P. vivax infection experiments published earlier were done with colonized
Anopheles mosquitoes [
11,
14,
19,
41,
44‐
48]. When field mosquitoes are colonized, they generally undergo genetic drift, lose rare alleles, and show a decrease in heterozygosity and an increase in inbreeding that may not fully represent the biological interactions with parasite that happen in the wild [
43,
49‐
51]. A recent report suggested that, by the 21st generation, colonized
Anopheles darlingi underwent low to moderate differentiation from the original wild mosquito population [
50]. Although collecting wild larvae requires additional human resources, is tedious, and collections are limited by seasonal availability, infection experiments with wild mosquitoes provide a solid baseline simulation of
Plasmodium-
Anopheles interactions in the wild. In the future, experiments with high passage colonized
An. stephensi maintained in the MESA NIMR Goa insectary will be compared with the wild population for their susceptibility to
P. vivax infections.
In many places, it is not common to have patient blood with
P. vivax and vector laboratories in close proximity. The MESA-ICEMR mosquito infection laboratory at NIMR is located within 5 km of GMC, the study site where
P. vivax patients are recruited and enrolled [
38]. The close proximity of the two study sites facilitates easy transport of blood and enables feeding of mosquitoes to within one-and-a-half hours from the time of blood collection. The short duration between blood collection and mosquito feeding minimizes the loss in infectivity of the blood sample due to environmental factors, such as drop in temperature and change in blood pH [
26,
52]. A recent study found that blood samples fed to mosquitoes at 8 h were significantly less infective than samples fed at 4 h post blood collection [
26]. Furthermore, from the point of collection through mosquito feeding, the blood was always maintained at 37 °C to prevent premature exflagellation and any accompanying loss in mosquito infectivity.
Studying the correlation between the parasite load in the patient blood sample and the corresponding mosquito infections may help better understand the dynamics of parasite development in its vector in specific geographic locations. Correlations made between gametocyte density and mosquito infection based on thick smears are not always reliable, as up to 80% of gametocytes may be lost during the staining procedure [
21], and the density of white blood cells (WBCs), to which gametocyte counts are related, is difficult to ascertain [
22,
23]. In this study, two expert microscopists counted the parasites in 100 fields each by the Miller counting technique, and their counts were significantly similar, thereby giving greater confidence in the correlation analysis. Positive correlation was observed between gametocytaemia and parasitaemia in
P. vivax patient smears. The correlation between gametocyte density and mosquito infection is often considered weak [
7‐
10]. In the studies presented here, there was weak correlation between gametocytaemia/parasitaemia to oocyst numbers and no correlation to oocyst infection rate. Also, the ratio of female to male gametocytes did not affect mosquito infections. It appears that the number of mature/infective gametocytes in the blood sample is more important in determining the oocyst load than the absolute number of gametocytes. Furthermore, since the study was conducted in a malaria-endemic area, the transmission blocking immunity in the host serum [
28‐
30] may also help determine the oocyst numbers. In experiments where the average mosquito oocyst load was greater than 20, the proportion of male gametocytes in patient blood was closer to 50%. This indicates that for good infectivity in this transmission setting, equal proportion of male and female gametocytes are required. In natural infections of
P. falciparum [
53‐
55] and in
P. vivax [
14], ratios of three or four female gametocytes to a male gametocyte is common, although there are variations depending on clones [
56], treatment [
57,
58] and the course of infection [
59,
60]. The high proportion of male gametocytes in this geographical location may be an adaptation of the parasite to counter host’s transmission blocking immune mechanisms that may affect the production of male gametes [
61]. Also, in
P. falciparum, it has been suggested that gametocyte density may affect gametocyte sex ratios, with low density favouring greater proportion of male gametocytes and increased transmission [
62].
Sub-microscopic gametocyte infections are less common with
P. vivax than with
P. falciparum [
12] and, as reported earlier [
6], gametocytes were seen in all of the patient samples. In agreement with earlier studies [
19,
63], at one level, development of parasites from oocytes to sporozoites appeared very efficient in mosquitoes. There was a strong positive correlation between the percentage of mosquitoes positive for oocysts and per cent sporozoite positivity. However, the correlation between oocyst numbers in individual mosquitoes and sporozoite load was not linear. When the average oocyst load ranged between 0 and 66, a positive correlation with the sporozoite load was observed, as indicated by the increase in mosquitoes with gland indices of 3+ and 4+. While
P. vivax studies of this type in
An. stephensi are not known, an earlier study reported a linear correlation between oocyst and sporozoite load in
Anopheles dirus and
Anopheles minimus infected with
P. vivax [
47]. In the present study, however, when the average oocyst load was greater than 79, there was a decrease in the number of mosquitoes with a gland index of 4+. On day 12, some salivary glands were dissected in parallel with the midguts of the same mosquitoes and examined for oocyst health and load. In several cases, mosquitoes with numerous melanized and unhealthy oocysts failed to have a heavy sporozoite load (4+). This suggests that when the oocyst load is sufficiently high, enhanced melanization is activated in the mosquito, providing protection from tissue damage that would be caused by rupturing oocysts and continuously invading sporozoites. In contrast, an earlier study based on
P. vivax infections in colonized
An. dirus and
An. minimus suggests that once oocysts are formed, the mosquito does not impose a ‘carrying capacity’ on the developing oocysts [
47]. Here, in wild
An. stephensi, the presence of melanized and unhealthy oocysts in the midgut strongly suggest a potential role of the mosquito’s immune system in controlling infection.
As seen in earlier studies [
19,
41], in most feeding experiments, there was high variability in the oocyst load within individual mosquitoes of the same batch: Some were completely protected (zero oocysts) and some allowed large oocyst loads (>200). The genetic diversity of the wild mosquito population could be a critical factor that determines
P. vivax infection load.
Anopheles gambiae, the African malaria vector has been shown to exist in M and S forms based on its larval habitat and this adaptive divergence may influence the vector capacity and concomitant malaria epidemiology [
64]. Future research on understanding the underlying traits that confer protection to
Plasmodium infections in the wild would be of value.
Authors’ contributions
PBN, AKM, NV, AK, and PKR designed the study. LC, SKM, AK, NV, and PKR administered the study. PBN, AKM, SB, SV, SBH, MD, JW, and AM carried out the experiments. PBN, AKM, AK, and PKR analyzed the data. PBN, AKM, LC, NV, AK, and PKR wrote and edited the manuscript. All authors read and approved the final manuscript.