Malaria Journal the Relationship of Plasmodium Falciparum Humeral Immunity with Hiv-1 Immunosuppression and Treatment Efficacy in Zambia

Background: HIV-1 infection affects malaria humeral immunity during pregnancy, but data for non-pregnant adults are lacking. This study reports the impact of HIV-1 infection and other variables on the level of malaria humeral immunity in adults with clinical malaria and whether humeral immune suppression was a risk factor for treatment failure.


Background
Humeral responses are of critical importance to blood stage immunity to Plasmodium falciparum [1]. Malaria-spe-cific antibodies mediate important anti-parasitic effector functions, including inhibition of cyto-adherence, inhibition of erythrocyte invasion, opsonization for phagocytic clearance, antibody-dependent cyto-toxicity and cellular inhibition [2]. Well-known merozoite antigens are the apical membrane antigen 1 (AMA-1) and merozoite surface proteins (MSPs) [3]. These antigens are involved in erythrocyte invasion [4,5] and are important vaccine candidates [6]. Variant surface antigens (VSAs) are important targets of protective immunity [7], but are also responsible for parasite evasion of the immune system by means of clonal antigenic variation [8][9][10].
Co-infection with HIV-1 and malaria is common in Africa [11]. HIV-1 infected people with low CD4 count have a higher prevalence of P. falciparum malaria infection, disease and treatment failure [12][13][14][15]. However, little is known regarding the impact of HIV-1 infection on humeral immunity to P. falciparum. Differences in antimalarial antibody levels have been shown in HIV-1 infected pregnant adults [16][17][18] and adults hospitalized with AIDS [19], but data for non-pregnant HIV-1 infected individuals are lacking. The impairment of the humeral response to malaria by a HIV-1 infection might partly explain the predisposition of HIV-1 infected adults to malaria disease. Understanding malaria immunity in HIV-1 infected individuals may also have implications for the deployment of future malaria vaccines.
This study assessed the anti-malarial humeral immunity in HIV-1 infected individuals and its association with anti-malarial treatment failure

Patients
This study was conducted in Ndola, Zambia, an area of meso-to hyperendemic malaria [20], between October 2004 and June 2005 within a randomized clinical trial (RCT) comparing the safety and efficacy of artemetherlumefantrine (AL) and sulphadoxine-pyrimethamine (SP) in adults with uncomplicated P. falciparum malaria.
The study and the results have been reported elsewhere [20]. Briefly, all individuals aged 15-50 years, attending four peri-urban health centers and with fever (body temperature ≥ 37.5°C), and/or history of fever in the previous 48 hours without any other obvious disease were screened for P. falciparum malaria infection and pregnancy (if applicable) and were included if they had a parasite density of at least 1,000 parasites/μL. Additional exclusion criteria were: severe malaria; documented intake of SP or AL two weeks prior recruitment; other cause of fever; evidence of underlying chronic diseases (cardiac, renal, hepatic, malnutrition); pregnancy; history of allergy to study drug or other sulfa drugs; non-resident in the study area.
Clinical history, body temperature and physical findings were recorded. Venous blood (5 ml) was used to prepare blood films, impregnated filter papers (Schleicher & Schuell) for molecular analysis, measurement of hemoglobin (HemoCue ® ) and test for HIV-1 infection, CD4 count and viral load (if HIV-1 infected). Residual plasma was separated, stored and transported at -70°C to be assayed by ELISA and FACS for malarial antibody quantification. Patients were followed up until 45 day post-treatment when CD4 count was reassessed, as a proxy of underlying immune suppression. The study was approved by the ethical and scientific committees of the Institute of Tropical Medicine, Antwerp, Belgium, The Antwerp University, the Tropical Disease Research Centre, Ndola, Zambia and Melbourne Health Research Directorate, Australia.

Laboratory methods
All laboratory technicians were blinded to clinical data. Thin blood films were fixed with methanol and thin and thick blood films were stained with 10% Giemsa. Parasite densities were determined by microscopy as the number of asexual P. falciparum parasites per 200 white blood cells (WBC). Parasitaemia/μl was computed using the actual WBC counts. Internal quality control was organized as recommended by WHO [21]. HIV-1 testing consisted of a screening EIA (Abbott Determine, Abbott laboratories, US) and confirmation of reactive samples by a second EIA (Genie II, Sanofi, Canada). Samples with discordant results were retested with Capillus (Cambridge, Diagnostics, Ireland) whose result was considered as final. CD4 count were performed on all individuals with a direct volumetric absolute CD4 counting instrument (Cyflow ® Counter, Partec, Germany) [22]. A FACSCount ® instrument (Becton Dickinson, US) was used to validate the Cyflow data and served as a quality control. Based on previous research, a CD4 count of 300/μl at study entry and 450/μL at 45 days follow up was used as a threshold between low and high counts [13]. In order to distinguish recrudescence from reinfection, blood samples, collected on filter paper, were assessed with a nested PCR technique as described previously [20]. HIV-1 RNA was assayed in plasma by the Roche Amplicor HIV-1 Monitor Test, version 1.5 (Roche Diagnostics, Branchburg, NJ, USA).
Several parasite lines (E8B, A4 and HCD6) were used for assessing malarial humeral immunity status. Parasite line E8B, expressing a mix of var genes, adheres to CD36 and ICAM-1. Of these var genes, A4var (which binds to ICAM-1 [23]) is a minor transcript (M Duffy, unpublished). Var gene expression of parasite line A4 was maintained by positive selection using monoclonal antibody BC6 [24] and was provided courtesy of Prof C. Newbold. Parasite line HCD6 was derived from a laboratory adapted patient isolate by repeated panning on CD36. HCD6 also expresses a mix of var genes and adheres to CD36 but not ICAM-1. Infected erythrocytes (IE) were cultured as described [25]. For flow cytometry, IE with trophozoitestage parasites were harvested at 7-12% parasitaemia and washed three times in phosphate buffered saline/1% newborn calf serum (PBS+; Commonwealth Serum Laboratories, Melbourne, Australia). IE were resuspended in PBS+ at 10 7 /mL with test serum (1 in 20 dilution, final volume 100 μL) in microtitre plates and incubated at room temperature for 30 min, washed as before, and incubated for 30 min with rabbit anti-human IgG and (after further washing as before) with Alexafluor ® 488-conjugated donkey anti-rabbit IgG (Invitrogen, Eugene, Oregon USA) and ethidium bromide (final concentration 10 mg/L, PRO-GEN, Brisbane, Australia). Washed cells were resuspended in 200 μL PBS+ and analyzed on a Becton Dickinson FAC-SCalibur flow cytometer with Cell Quest software. IE were gated according to ethidium bromide fluorescence, and 1,000 cells positive for ethidium bromide were collected. For each serum sample, the geometric mean Alexafluor 488 fluorescence intensity (MFI) generated by the gated population of IE was recorded. Control serum samples from malaria naïve adults were included in each assay. A positive control pool of hyper-immune serum against VSAs of E8B, A4 and HCD6 was made from the serum of 11 Malawian adults and run in duplicate in each assay. Samples with readings below the mean of the unexposed controls were assigned half the lowest value of that particular VSA variable in order to permit log-transformation; samples given a positive reading were assigned relative values by use of the formula (sample reading minus negative-control reading divided by positive control reading minus negative-control reading) × 100. Samples giving a reading above positive control were further diluted and values were assigned following the same formula and recalculated to the original dilution.
Antibody levels to merozoite antigens were measured by ELISA. Recombinant 3D7 or FC27 MSP2 or AMA-1 proteins (2 μg/ml in PBS, kindly provided by Prof R Anders) were used to coat microtitre plates overnight at 4°C. Plates were blocked for 1 h with PBS/5% skim milk powder (Blotto) and washed five times with phosphate-buffered saline containing 0.05% Tween (PBS/Tween). Samples diluted 1 in 1,000 in Blotto were added to plates (50 μL, in duplicate) and incubated for 2 h. After washing, horseradish-peroxidase-conjugated sheep antibody to human IgG (1 in 2,000; Silenus) was added and the plates were incubated for 2 h then washed three times in PBS/ Tween and twice in deionized water. Peroxidase substrate was added and color was developed, plates were read at 415 nm on a Biorad plate reader version 5.2, and OD results were expressed relative to positive and negative controls as for VSA antibodies. Results were also classified as positive (optical density greater than the mean plus two SD of non-exposed sera) or negative. To estimate the "breadth" of immunity a binary variable "low responders" was created. Low responders were defined as having antibody levels below the geometric mean on all three antigens.
Treatment outcomes were defined according to the most recent WHO classification and are described in detailed elsewhere [13,21]. For this report, it was considered that the adequate parasitological and clinical response was the absence of recurrent parasitaemia. Recurrent parasitaemia distinguished new infections from recrudescence by PCR genotyping.

Statistical analysis
Clinical data were double entered and organized in Epiinfo (version 6.04b; Centers for Disease Control and Prevention, Atlanta, GA). All data were exported to STATA version 10.0 (Stata Corporation, College Station, Texas, USA) for analysis. Normally distributed variables were compared by Student's t test, non-normally distributed variables by Mann-Whitney's rank sum test (two groups).
Differences in proportions were assessed by χ 2 analysis.
Linear regression modeling was used to assess associations between humeral immunity and other factors. For the linear regression modeling, all non-normally distributed variables were log transformed and factors with a Pvalue < 0.10 were retained, as well as factors modifying the regression coefficient of the main determinant by more than 10%. All reported P-values are two-sided. Logistic regression modeling was used to assess if humeral immunity was a risk factor for treatment failure. P-values < 0.05 were considered significant.

Antibody levels to variant surface antigens
Antibody levels to VSA of E8B and A4 were inversely related to CD4 count at day 45 (both P = 0.02) though there was an interaction between initial parasitaemia and CD4 count at day 45 (P = 0.05. In HIV-1 infected with a CD4 count at day 45 <450 cells/μL, no association  between parasite load and antibody levels to VSA E8B or A4 was found. In HIV-1 infected with a CD4 count ≥ 450 cells/μL on day 45, antibody levels to VSA of E8B and A4 were inversely associated with parasite density (both P = 0.03).

Malaria humeral immunity and malaria treatment failure
Of the evaluable subjects, 82.8% (222/268) patients had an adequate parasitological and clinical response at day 45. PCR genotyping identified 16 patients with new infections (6.0%) and 30 patients with recrudescence (11.2%).
No difference in antibody levels to merozoite antigens or VSA was found between patients successfully treated for malaria and those with recurrent parasitaemia. However, after PCR correction, high antibody levels to the VSAs of E8B, A4, and HCD6 protected for recrudescence P = 0.02; P = 0.02 and P = 0.04 respectively) (  [12][13][14]. Given the central importance of humeral immunity  in protecting against malaria, antibody levels to key merozoite antigens and VSA were assessed in adult Zambians with HIV-1 infection and related immune suppression and their association with anti-malarial treatment outcome [13]. Since merozoite antigens and VSAs differ both in their timing of expression and in their conservation or variation between different isolates, they are discussed separately.

Merozoite antigens: AMA-1, MSP2 3D7 and MSP2 FC27
HIV-1 infection was associated with low antibody levels to AMA-1 and, among HIV-1 infected adults, low AMA-1 antibody levels were associated with low CD4 count. And HIV-1 infected adults were twice as likely as HIV-1 negative adults to have low antibody levels to all three merozoite antigens combined.
Reduced concentrations of antibody levels to AMA-1 have also been demonstrated in HIV-1 infected pregnant Malawian women [18]. In that particular study, antibody levels to AMA1 were not associated with CD4 count, but AMA-1 antibody levels were higher in HIV-1 infected women with malaria infection than those without malaria infection (S Rogerson, unpublished observations).
Acute P. falciparum infection induces a short-lived depression in circulating T cell numbers [26,27]. As HIV-1 infection and malaria both influence CD4 count, difficulties arise when assessing associations between those infections and cellular immunity. The positive relationship between the concentration of antibodies to AMA-1 and the CD4 count on enrolment may indicate that low CD4 count directly influences antibody production, as required T cell help is limited. AMA-1 antibody levels at day 0 were not associated with CD4 count at day 45, suggesting that the association between AMA-1 antibody and   CD4 count at day 0 may be a function of the degree of T cell reallocation, rather than a direct effect of HIV-1 on antibody levels. Unfortunately, antibody levels were not measured at follow up, when CD4 count was restored, and malaria infection had usually been eliminated: such measurements, and measurement of IgG subclass responses, could provide useful information on the dynamics of immune responses following symptomatic malaria in adults [28]. Limited studies have examined the effect of HIV-1 on antibody immunity to malaria in adults. One such study suggested that HIV-1 infected adults only become vulnerable to malaria when they develop AIDS [19]. Because T and B cell functions are affected early in HIV-1 infection [29], malaria specific humeral immunity might also be affected in the early HIV-1 stages. Antibodies to different targets probably act in an additive or synergistic manner [3] and, under natural exposure, protective immunity to malaria results from high titer antibody levels to multiple antigenic targets [30][31][32]. To begin to examine the impact of HIV-1 on antibody response to multiple antigenic targets, antibody results for the three merozoite antigens tested were combined [32].
In this study, HIV-1 infected adults were over twice as likely to be "low responders" to this combination of targets, and low responders tended to have a higher parasite load. HIV-1 might decrease antibody to many targets by small amounts; in combination, such defects could predispose to disease or (as these data suggest) to uncontrolled parasite replication.
Somewhat unexpectedly, within the HIV-1 infected population, low responders were less anemic. The recruited patients came from a community where malaria transmission is relatively homogeneous, so differences in exposure and concomitant development of malarial anemia seem unlikely. Second, the major contributor to the hemolytic anemia is the accelerated destruction of uninfected RBC, probably linked to immune mechanisms [33]. Therefore, lower antibody levels might be an independent protective factor for erythrocyte destruction. However, as low responders have higher parasite loads, the overall impact might be limited. Additional research with a longitudinal follow up and a larger panel of antigenic targets is required to determine whether antibody to blood stage parasites influence anemia risk in this already immunecompromised population.
In the whole study population, antibody levels to both MSP2 types were negatively associated with parasite density indicating their direct involvement in parasite control whereas AMA-1 antibody levels were not. The results found for MSP2 IgG confirm studies that have shown associations between antibody levels to blood stage antigens and decreased prospective risk of clinical malaria [6,31,32,[34][35][36].

Variant surface antigens of the parasite lines E8B, A4, and HCD6
Adult study participants should already have immunity to severe malaria and their antibody repertoire to VSAs may be extensive [3]. It may, therefore, not be surprising that no differences were found in antibody levels to VSA of the different parasite lines between HIV-1 infected and HIV-1 negative adults. Since natural immunity may include the acquisition of a large repertoire of cross-reactive VSA specific antibodies, it may take considerable time until the impact of HIV-1 on humeral responses is apparent. In previous studies, asymptomatic HIV-1 infected individuals maintained antibody levels [37], in contrast to patients with advanced clinical AIDS [19]. Indeed, only increased immune suppression diminishes B cell stimulation, resulting in decreased production of malaria specific antibodies [38]. Nevertheless, reduced antibody production to blood stage antigens and functional abnormalities of VSA specific IgG have been found in HIV-1 pregnant women without clinical AIDS [17,18]. Malaria in pregnancy is characterized by development of immunity to unique VSA expressed by IE capable of sequestering in the placenta [39]. HIV-1 is associated with decreased IgG antibody levels to these VSA, and decreased opsonizing antibody levels that cause phagocytic clearance of such IE [16,18]. Because immunity to pregnancy-associated malaria is only acquired during pregnancy, it may be more susceptible to the effects of concomitant HIV-1, compared to immunity built up by the subjects in this study over a lifetime, much of it preceding HIV-1 infection. The same reasoning might be applicable for children living in malaria endemic areas. Malaria in children is characterized by a development of immunity to VSAs. Low antibody levels to VSAs might be associated with increased clinical malaria incidence and treatment failure and HIV-1 infection might be associated with decreased IgG antibody levels to these VSA. Further research will be needed to assess this hypothesis.
Although VSA antibody levels were not directly associated with HIV-1 infection, they appear to have important roles in controlling malaria parasitaemia in this cohort. Among HIV-1 infected adults with a WBC count ≥ 4,900/μL, antibody levels to VSA were inversely related to parasitaemia. Among all patients, for those with a CD4 count >450/μL on day 45 there was a negative association between parasite load and antibody levels to VSAs of parasite lines E8B and A4. Antibody to VSA operates by preventing sequestration of IE in the vasculature (to avoid splenic clearance), or by opsonization of IE by cytophilic antibodies [40]. Further research should include IgG isotype determination and functional assays of these properties to assess and confirm this finding.
Antibody levels to VSA were similar in patients successfully treated for malaria and the patients who experienced recurrent infection, but high levels of antibody levels to VSAs were associated with decreased risk of recrudescence, suggesting that these antibodies may complement the therapeutic response to the anti-malarial drug [41]. Indeed, an adequate host immunological response is needed in order to maximize the pharmacodynamic properties of an anti-malarial drug [12,41]. As PCR has some technical limitations in distinguishing recrudescences from new infections further research will be needed to conclusively interpret this result [42].

Conclusion
This study provides evidence that HIV-1 affects humeral responses to AMA-1. Although levels of antibody to the other merozoite antigens and VSA were not or little affected by HIV-1 infection, they appeared to play an important role in controlling parasite density, and the inability to control malaria parasite density is one of the features of HIV-1 immune suppression. Furthermore, recrudescence was associated with low VSA antibody titers to all three parasite lines tested. Specific research in HIV-1 and malaria co-infected adults, with pre-established malaria-immunity, might offer additional insights into malaria immunity.