Background
In Brazil, the largest number of malaria cases (98%) occurs within the Legal Amazon region. Between 2005 and 2009, the number of cases decreases from 607,801 to 306,908. A similar reduction was found for mortality (52.5%) and malaria incidence (25.6 to 12.1 cases per thousand inhabitants). In 2011, only 263,323 cases were reported [
1]. In other Brazilian regions, the transmission risk is low or nonexistent [
2]. In Mato Grosso, the disease is predominantly focal. It is endemic only in the northern region of the State [
3] with 2,161 cases reported in 2010 [
4].
The infection caused by
Plasmodium vivax has long been considered a benign disease, especially when compared to infections caused by
Plasmodium falciparum[
5]. Recently, literature report has shown that vivax malaria caused more severe forms of the disease than previously described, and the most common symptoms of these complications are severe anaemia, respiratory distress and acute lung injury, coma, among other manifestations [
6,
7]. The increasing drug resistance and the complications of this parasitic disease require joint efforts for a better understanding and resolution.
Evidence suggests that during infection, malaria causes activation and dysfunction of T cells and lymphopaenia [
8]. The CD8+ T cells and the cytokines IFN-γ and TNF confer protection against parasites pre-erythrocytic
Plasmodium within hepatocytes [
9], whereas CD4+ T cells restricted growth of parasites erythrocytes of
Plasmodium through secretion of cytokines, activation of macrophages and direction of humoral immunity [
10]. Recently, the involvement of regulatory T cells in infection caused by
P. vivax was demonstrated [
11], suggesting that the balance between pro-and anti-inflammatory cytokines is needed to track changes related to malaria [
12].
Besides cytokines, other factors can modulate the differentiation of T helper lymphocytes, for example, the affinity of the antigen by a T cell receptor (TCR). With low affinity antigen generally induce a Th2 response, whereas high affinity induces differentiation into a Th1 response [
13,
14]. Annexin-A1 (ANXA1) is an endogenous protein with anti-inflammatory functions, endowed with potent anti-migratory activity of neutrophils, ensuring the transitory nature of the inflammatory response [
15,
16]. This protein is identified in several types of leukocytes [
17,
18] and positively modulates TCR signaling, making it an important molecular target in the differentiation and proliferation of lymphocytes. In the lymphocytes, ANXA1 has been characterized as an antiproliferative protein [
17], but new studies have indicated other mechanisms, like regulates the T cell production of IFN-γ, IL-17, TNF and IL-6 [
19] and the suppressive activity of apoptotic cells on the immune response [
20].
Therefore, the aim of this study was to investigate the expression of ANXA1 in CD4+, CD8+ T cells, regulatory T cells (Treg) and quantification of the cytokine IL-10 in plasma from patients with malaria caused by P. vivax. The relationship between the presence of lymphocyte sub-populations and release of immunoregulatory molecules may contribute to the understanding of the dynamics of the immune response in vivax malaria.
Methods
Malaria patients and healthy controls
Sixty-nine malaria patients from the Julio Müller University Hospital of the Federal University of Mato Grosso State, Cuiabá – MT, were included in this study. The age, number of previous episodes of malaria, and other infectious diseases history of each participant were recorded using a standard questionnaire. Patients who have already been treated with some type of anti-malarial drug were excluded from the study. Thirty-seven healthy volunteers living in Cuiabá, a non-endemic malaria area, were recruited as the control group. These volunteers had no history of malaria infection. Written informed consent was obtained from all patients or their legal representatives before enrollment in the study. The study protocol was approved by the Ethics Committee from Julio Müller University Hospital (633/CEP-HUJM/09). The study subjects were matched by sex and age. The average age of patients with malaria was 33.7 ± 1.9 years. And it was 37.6 ± 2.2 years in the control group.
Blood collection
Blood samples were taken from each patient. A finger-tip smear was taken for the parasitological diagnosis, and then approximately 5 mL of venous blood was collected for the analysis of cytokines and ANXA1 expression. The blood was drawn aseptically into Vacutainer® tubes (Becton Dickson and company, Franklin Lakes, NJ, USA) with EDTA. The haemoglobin, platelets and whole blood cells (WBC) were quantified with the Blood Cell Count (Pentra, Horiba Diagnostics, Kyoto, Japan). After, the blood was centrifuged at 1,200 g for 10 min at room temperature. The serum was separated out and the samples were aliquoted and stored at −20°C until assayed.
Parasitological diagnosis
Thick blood smears were stained with 5% Giemsa solution and examined for
Plasmodium species by two microscopists. Parasitaemia was assessed by counting the number of parasites per 200 leukocytes. If nine or fewer parasites were found, 300 additional leukocytes were counted. Parasitaemia were expressed as parasites/μL of blood from each individual. Patients were grouped by level of parasitaemia (low parasitaemia up to 750 parasites/μL and high parasitaemia above 752.5 parasites/μL) as recommended by clinical procedures [
21] and number of previous episodes of malaria (Ø episode - no previous episodes of malaria or primoinfected and > 1 episode - more than one previous episode of malaria).
Cytokine assay
The plasma levels of the cytokine IL-10 was assessed by enzyme-linked immunonosorbent assay (ELISA), using pairs of cytokine-specific monoclonal antibodies provided by commercially available assay (BD Biosciences - Pharmingen, San Diego, CA, USA). All tests were performed according to the manufacturer’s instructions. Each plate included a standard curve of recombinant human cytokine in parallel with the samples, the final enzyme activity was measured by a microplate reader automatic, V-max (Molecular Devices, Sunnyvale, USA) at 405 nm. All samples were measured in duplicate, and the average of the two values of optical density was used for all analyses.
Immunofluorescence
Blood smears of patients infected with
P. vivax and healthy controls were incubated with 5% albumin bovine in PBS (PBSA) to block nonspecific binding and permeabilized with Teen 20 at 0.4% in PBS, as described before [
22]. A cocktail of primary antibodies were used to identify ANXA1 expression and lymphocyte subpopulation. Thus a polyclonal rabbit anti-ANXA1 antibody (1/200 in 1% PBSA) (Invitrogen, USA) and a specific lymphocyte marker: mouse anti-CD8, anti-CD4, anti-CD25 and anti-FOXP3 (Invitrogen, USA) (1/200 in 1% PBSA) were added into the slides and incubated overnight at 4°C. After repeated washings in 1% PBSA, a goat anti-rabbit (Fc fragment-specific) antibody conjugated to fluorochrome ALEXAFLUOR 488® and goat anti-mouse, conjugated to fluorochrome ALEXAFLUOR 546® (1/50 in 1% PBSA) and the marker DAPI nuclei (4′,6-diamidino-2-phenylindole) were added. Analysis was conducted with a microscope AxioScopeA1 (Carl Zeiss, GR) equipped with a DXM1200 digital camera, using the Software AXIOVISION, version 4.8. For cell number quantification: CD4+, CD8+ and Treg cells (CD4+/CD25+/FOXP3+) and ANXA1 expression 100 separate fields of each individual smears were evaluated. The protein ANXA1 expression was quantified by mean optical density (MOD) measured by the Software Axiovision. Data was obtained from the light spectrum, with values that range from 0 to 255 (arbitrary units – A.U.).
Statistical analysis
Data were expressed as mean ± standard error of the mean (SEM). To compare the haematological and parasitological data of individuals, the Mann-Whitney’s U and student’s t test was used. To compare cytokine IL-10 levels and ANXA1expression, data were tested using a one-way analysis of variance (one-way ANOVA) with a Bonferroni pos-test. For all statistical analysis, the Software GraphPad PRISM (La Jolla, CA, USA) was used. The p value < 0.05 was considered significantly different.
Discussion
Studies evaluating the mechanisms involved in
Plasmodium infection showed that the immune system develops a potent response against the parasite causing changes in several haematological components and mediators of immune system [
23,
24]. Moreover, more than 80% of diagnosed cases in Brazil are caused by
P. vivax[
25].
Several studies have reported haematological changes in patients with malaria. In this study, a reduction in haematocrit, haemoglobin, leukocytes and platelets was observed during the acute phase of the disease induced by
P. vivax[
26‐
28]. In the literature, there are two mechanisms that can explain the lymphocytes depletion in patients with
P. falciparum and
P. vivax in the acute phase of the disease: sequestration of cells to lymph nodes or other body parts and abnormal cell death through apoptosis [
29].
Furthermore, Braga
et al. [
30] demonstrated that malaria-specific proliferative T cell responses to various malaria antigens are commonly observed to be higher in non-immune or semi-immune rather than in the immune subjects, i.e., continuous exposure to malaria in areas of low endemicity may lead to a specific decrease of the T cell function. As described in the literature [
28,
31‐
33], the number of CD4+ and CD8+ T cells were significantly lower during acute malaria.
There is a well-recognized but unmet need for improved diagnostics based on biological markers to characterize disease status, parasitaemia and clinical outcome. Therefore, the evaluation of IL-10 and ANXA1 in the individuals with malaria was performed. Plasma levels of IL-10 were elevated in patients with high parasitaemia and who have had more than one episode of malaria. This result shows that re-exposure to
P. vivax may induce IL-10 production. High levels of IL-10 were also detected in African and Indian children with anaemia and high levels of parasitaemia [
33,
34]. Other studies also showed a positive relationship between the levels of IL-10 and parasite density in individuals infected with
P. vivax[
35]. IL-10 plays an important role in immunoregulation, inhibiting Th1 function and promoting the activity of NK cells [
35‐
40]. Other studies indicate that IL-10 were associated with Th2 response during malaria [
41]. The results obtained in this work together with previous literature findings, emphasize that IL-10 may regulate the proinflammatory response, participates in parasite elimination and contributes to the pathogenesis of the disease.
The expression of ANXA1 in subpopulations of T lymphocytes CD4+, CD8+ and Treg were assessed. ANXA1 is known to be constitutively expressed on leukocytes and epithelial cells [
17,
18,
42,
43]. Depending on the cell stimulus, ANXA1 expression may be increased endogenously in order to regulate the inflammatory processes [
18,
44]. In this work, lymphocytes sub-populations were observed to expressed ANXA1. This data is in agreement with findings in the literature, which indicates a pleiotropic mechanism of action of this protein in the innate and adaptive immune system [
18,
19,
45,
46].
Some studies suggest that ANXA1 demonstrated an antiproliferative activity in lymphocytes [
17,
19,
44,
47]. It was demonstrated a reduction in ANXA1 expression in CD4+ and CD8+ T cells. It was also observed a positive relation between ANXA1 expression and the number of previous episodes of malaria in CD4+ T cells. These data might indicate that ANXA1 could regulate the number of this cell population. This is the first time a paper analyses the expression of ANXA1 in infection by this parasite.
With respect to Treg lymphocytes, the number of these cells and the ANXA1 expression were increased in patients with low parasitaemia. There are no data on the literature about the ANXA1 functionality in Treg cells. These results are interesting and may indicate that this protein can function differently in each lymphocytes subpopulation.
Also, it is important to highlight that high ANXA1 expression in some lymphocytes and other leukocytes might had influence on the levels of IL-10 in malaria patients. Some studies described that ANXA1 can induce the IL-10 production [
20,
47,
48] through activation of ERK cascade [
49]. This cytokine can be produced by several cell types, such as lymphocytes Treg [
44], CD8+ lymphocytes and monocytes [
50].
Acknowledgements
This work was supported by the Conselho Nacional de Pesquisa - Brazil (CNPq grant number 555652/2009-2) and Fundação de Amparo à Pesquisa do Estado de Mato Grosso - Brazil (FAPEMAT), PRONEX-Rede Malária, Mato Grosso, Brazil. QIB is funded by Coordenação de Aperfeiçoamento de Pessoal de Nível Superior - Brazil (CAPES) (master studentship). A.S.D. is funded by Conselho Nacional de Desenvolvimento Científico e Tecnológico (CNPq, 303997/2011-7).
Competing interests
The authors declare that they have no competing interests.
Authors’ contributions
QIB and ASD were responsible for cytokines detection and immunofluorescence and wrote the manuscript. CJFF was responsible for selection of the patients and collection of the samples and final correction of the manuscript. All authors read and approved the final manuscript.