Background
Undernutrition results from insufficient dietary intake, poor absorption and/or inadequate use of the nutrients consumed. It is a major health concern, mainly throughout the developing world and children are especially affected. An estimated 826 million people in the world are undernourished, of those 95.9% are in the developing world [
1]; 178 million children under the age of 5 are stunted and 55 million are wasted [
2]. In 2011, 6.9 million children under 5 years died, one third of these deaths were related to increased susceptibility to infections due to undernutrition [
2]. Protein energy malnutrition (PEM) is thought to be one of the major causes of immunodeficiency. PEM and infection have always been closely associated, as PEM is a common cause of susceptibility to infections. Undernutrition in children negatively impacts on thymic development, therefore compromising immune responses [
3]. In malnourished patients, both innate and acquired immunity are affected [
4,
5] and common immune defects are an imbalance in the ratio of CD4/CD8
+ T cells [
6], low expression levels of CD69 on lymphocytes [
7], biased T helper cell responses [
8], reduced antibody responses [
6]; impaired phagocytosis by macrophages [
9,
10], lower nitrite/nitrate concentrations in wound fluid [
11] and decreased NF-kappaB activation by macrophages [
12] have also been shown in experimental models of PEM.
Arginase, an enzyme that catalyses the conversion of L-arginine, can be upregulated in murine macrophages, dendritic cells and neutrophils [
13], however, human neutrophils constitutively express arginase (reviewed in [
13]). There are two isoforms of arginase in mammals, arginase I and arginase II [
14,
15]. The catabolism of L-arginine by arginase can regulate the availability of L-arginine and therefore the efficiency of T cell responses: increased catabolism of L-arginine by arginase results in the depletion of L-arginine from the microenvironment; since L-arginine is essential for efficient T cell activation, this decrease in L-arginine results in impaired T cell responses [
13,
16‐
18]. In addition, the catabolism of L-arginine by arginase results in the production of ornithine, which is further catabolised into polyamines that are crucial for cell division; and into proline, which is the building block for collagen synthesis. L-arginine is also the substrate for nitric oxide synthase (NOS), that catabolises L-arginine into nitric oxide (NO), a molecule critical for the regulation of vascular homeostasis, neurotransmission and the killing of many pathogens [
19]. Therefore, by competing for the shared substrate L-arginine, increased arginase activity also modulates the production of NO. Consequently, deficiencies in L-arginine metabolism can disrupt many cellular and organ functions.
Increased arginase activity is common to several pathological and physiological conditions: it has been prominently described in cancer [
16,
18], but also in asthma, myocardial infarction, pregnancy and infectious and autoimmune diseases (summarised in [
13]). We have recently shown that increased arginase activity is a marker of disease severity in HIV seropositive (HIV+) patients [
20], in patients with visceral leishmaniasis and HIV co-infection [
21] and in patients with visceral [
22] and cutaneous [
23] leishmaniasis. Malnutrition is a major contributor to both progression and severity of visceral leishmaniasis (VL) and several studies in the mouse have shown that PEM and micronutrient deficient diet exacerbates VL [
24].
Nutrition has been shown to impact on the phenotype of macrophages: in obesity, adipose tissue is characterized by infiltration of inflammatory macrophages, in contrast to lean adipose tissue, where a majority of anti-inflammatory macrophages are present [
25]. In the present study, we tested the hypothesis that malnutrition impacts on macrophage effector functions and results in increased arginase activity, therefore contributing to increased susceptibility to disease.
Methods
Mice
Specific pathogen free female BALB/c mice (18 g) were purchased from Charles River (UK) and were kept in individually vented cages. The animal colonies were screened regularly for mouse pathogens and consistently tested negative.
Ethics statement
Animal experiments were performed in accordance with home office and institutional guidelines. The project licence (PPL 70/6712) was approved by the Imperial College Central Animal Welfare & review Body (AWERB) committee.
Mice were fed on the different diets following a 3-day period of acclimatisation. Control mice were fed a diet consisting of 14.4% protein, 61.7% carbohydrates and 2.7% fat (RM1, Harlem Laboratories Inc, Madison, Additional file
1). The group of mice that was malnourished (MN group) was fed a diet consisting of 0.7% protein, 87.0% carbohydrates and 4.1% fat (Modification of TestDiet AIN-93 M w/No protein, TestDiet, Additional file
2). Both diets had similar amounts of calories: control group =3.5 kcal/g and MN group: 3.85 kcal/g and both groups of mice had
ad libitum access to food and water.
Sample collection
Bone marrow cells were obtained by flushing the femurs of BALB/c mice and precursor cells were used immediately for flow cytometry or were frozen in PBS containing 1% protease inhibitor cocktail (Sigma) for the determination of arginase activity. To obtain bone marrow derived macrophages (BMMΦ), fresh precursor cells were cultured for 8 days in a humid atmosphere at 37°C and 10% CO
2 in hydrophobic Teflon bags in DMEM (Sigma) containing 10% heat-inactivated FCS (Gibco), 5% horse serum (Gibco), the supernatant of L929 fibroblasts at a final concentration of 15% (v/v) as a source of colony stimulating factor (CSF), 50 IU/ml penicillin, 50 μg/ml streptomycin, and 292 μg/ml L-glutamine (Sigma) as described in [
26]. To obtain bone marrow-derived neutrophils, fresh precursor cells were cultured for 7 days as described in [
27].
Peripheral blood mononuclear cells (PBMCs): blood was collected in EDTA tubes by cardiac puncture and PBMCs were isolated by density gradient centrifugation on Histopaque-1077 (Sigma). Before harvesting the interphase, the plasma was collected and frozen for further analysis. Cells were washed in phosphate buffered saline (PBS) and were used immediately for flow cytometry or were frozen in PBS containing 1% protease inhibitor cocktail (Sigma) for the determination of arginase activity.
Spleen cells: spleens from BALB/c mice were homogenised in PBS and red cells were lysed with red cell lysis buffer as described in [
27] and were frozen in PBS containing 1% protease inhibitor cocktail (Sigma) for the determination of arginase activity.
Macrophage activation
Mature BMMΦ and mature BM-derived neutrophils were harvested and 5 × 105 BMMΦ/ml were plated in DMEM (Sigma) containing 5% heat-inactivated FCS (Gibco), 50 IU/ml penicillin, 50 μg/ml streptomycin, and 292 μg/ml L-glutamine (Sigma) and 5 × 10-5 M 2-mercaptoethanol (Sigma). BMMΦ were stimulated with 20U/ml IL-4 or with 100U/ml IFN-γ and 500U/ml TNF-α (Peprotech) or with 1 μg LPS (Sigma) for 72 hours, unstimulated macrophages were used as control. Mature BM-derived neutrophils were stimulated with 20U/ml IL-4 (Peprotech) and unstimulated mature BM-derived neutrophils were used as control.
Phagocytosis assay
Mature BMMΦ (1 × 105 BMMΦ) were incubated for 1 hour with pHrodo™ Bioparticles® fluorescent particles according to the manufacturer’s protocol (Molecular Probes). Analysis of the mean fluorescence intensities (MFI) was performed on a LSRII (BD Bioscience) and results were analyzed using Summit v4.3 software.
Flow cytometry
Antibodies used were as follows: anti-Ly-6C (clone HK1.4, eBioscience), anti-Ly-6G (clone RB6-8C5, eBioscience), anti-F4/80 (clone BM8, BD Biosciences), anti-arginase I (Polyclonal sheep IgG, R&D). Cells were washed with PBS, the fixation step was performed with 2% formaldehyde in PBS and the permeabilisation step with 0.5% saponin in PBS. Analysis was performed on a LSRII (BD Bioscience) and results were analyzed using Summit v4.3 software.
The percentages of positive cells with the isotype controls were <1%.
Determination of nitrite and arginase activity
NO
2- accumulated in the supernatant was used as an indicator of NO production and measured using the Griess reagent as described in [
28]. Culture supernatants were collected after 48 h, and equal volumes of macrophage culture supernatants and Griess reagent (1% sulphanilamide/0.1% N-(1-naphthyl)ethylenediamine dihydrochloride/2.5% H
3PO
4) were mixed and incubated for 10 min at room temperature. Absorbance was measured at 540 nm. Nitrite concentration was determined using NaNO
2 as standard.
The enzymatic activity of arginase was measured as previously described [
29]. Briefly, the cell lysate was activated by heating for 10 min at 56°C. L-arginine hydrolysis was conducted by incubating the activated lysate with 0.5 M L-arginine (pH 9.7) at 37°C for 15 to 120 minutes. The reaction was stopped with H
2SO
4(96%)/H
3PO
4(85%)/H
2O (1:3:7, v/v/v, VWR). α-isonitrosopropiophenone (ISPF, dissolved in 100% ethanol, Sigma) was added and incubated for 45 min at 100°C, followed by 30 min at 4°C. A standard curve was obtained by treating serially diluted urea with ISPF and incubated in the final step. The optical density (OD) was measured at 550 nm.
Protein concentration of samples was measured using the BCA Protein Assay kit (Pierce) as previously described [
29]. One unit of enzyme activity is defined as the amount of enzyme that catalyzes the formation of 1 μmol of urea per min.
Determination of L-arginine and L-ornithine concentrations
The concentration of L-arginine and L-ornithine in plasma were measured by ion exchange chromatography and quantified by post-column ninhydrin derivatisation using an amino acid analyser (AminoTac JLC- 500/V) as described previously [
30].
Infection of mice and macrophages with Leishmania infantum
Mice
Leishmania (L) infantum amastigotes (MHOM/MA/67/ITMPA263 (MON-1) were derived from infected RAG1.B6 mice. BALB/c mice were infected 7 days after start of the experiment with 3 × 106 amastigotes in the lateral tail vein and were culled 9 days later. Spleen cells were isolated as described above and 5 × 106 cells were resuspended in 1 ml M199 containing 50 IU/ml penicillin, 50 μg/ml streptomycin, and 292 μg/ml L-glutamine (Sigma), 2% hepes and 4 μM sodium bicarbonate (Sigma) and 10% fetal bovine serum (Gibco) and incubated in a humid atmosphere at 26°C and 5% CO2. Eight days later, the wells were resuspended carefully and the transformed promastigotes were fixed with PBS containing 2% formaldehyde and counted using a haemocytometer.
Macrophages
5 × 10
5 BMMΦ/ml cells were plated and stimulated with 20U/ml IL-4 or with 100U/ml IFN-γ and 500U/ml TNF-α (Peprotech). Unstimulated macrophages were used as control. Four hours later, the cultures were infected with 25 × 10
5/ml
L. infantum promastigotes. After 96 h, the macrophages were washed and lysed with HEPES-buffered medium containing 0.008% SDS [
31] and 1 ml of complete M199 was added to each well, incubated and the transformed promastigotes were counted as described above.
Statistical analyses
Data were evaluated for statistical differences using a two-tailed Mann–Whitney test (GraphPad Prism 5) and differences were considered statistically significant at p <0.05. Results are expressed as mean with 95% CI.
Discussion
PEM is one of the major causes of immunosuppression, modifying both innate and adaptive immunity. It is highly prevalent in low-income countries, particularly in children [
4]. In the developed world, PEM is also a serious health concern, mainly seen in the elderly, with up to 10% of older people undernourished in nursing homes and up to 50% of older people undernourished when discharged from hospital [
34]. Malnutrition is associated with a plethora of problems, such as fatigue, anaemia, cognitive abnormalities, immune dysfunctions and increased susceptibility to infections [
34]. Monocytes and macrophages play a major role in the elimination of pathogens. Here we show that the frequency of monocytes is increased in the bone marrow and PBMCs of MN mice, suggesting a dysregulation in the haematopoiesis in these mice. This is in agreement with a study by Borelli et al. [
35] that showed a 2.5-fold increase in the number of peripheral blood monocytes. Whereas macrophages and monocytes can be instructed to kill intracellular pathogens, they can also act as “safe target”. Indeed, in
Leishmania major infected nonhealing mice, macrophage-granulocytes precursor cells were shown to be dramatically increased during infection, thereby offering a large number of host cells for the parasites to infect [
36,
37]. Since these cells have not yet developed their full microbicidal potential [
37], the parasites cannot be killed efficiently and the myeloid cells represent therefore a more permissive environment for the parasites to survive. We also showed an increase in the frequency of F4/80 + Ly6C + inflammatory macrophages in the blood of MN mice; these macrophages have been shown to be rapidly recruited to sites of inflammation. Since malnutrition has been associated with chronic inflammation [
38], this might explain the increased frequency of these macrophages during PEM.
Whereas we detected arginase activity in the BM cells, we were not able to able to identify the phenotype of arginase-expressing cells. Since other cells than macrophages have been shown to express arginase, it is possible that cells such as dendritic cells, neutrophils [
27,
28] or innate lymphoid cells [
39] might contribute.
Here, we showed that PEM did not impact on the capacity of BMMΦ to produce NO in response to activation with IFN-γ and TNF-α or LPS; nor on the capacity of BMMΦ capacity to kill intracellular
Leishmania parasites. We also showed that
in vitro, bone marrow cells from malnourished mice did proliferate and differentiate similarly to those from control mice as both the number of cells after 8 days of differentiation were similar. Furthermore, phagocytosis of bioparticles was not impaired in BMMΦ derived from malnourished mice. In contrast, it has been previously shown that some macrophage functions are altered during PEM: the phagocytic capacity and production of superoxide anions, indicative of their microbicidal competence, were shown to be impaired [
10,
40,
41], suggesting that increased susceptibility to disease might be due to an impaired capacity of phagocytic cells to kill pathogens. The discrepancies between these studies and ours could be due to the different macrophages used: BMMΦ in our study versus elicited peritoneal exudate macrophages in the other studies [
10,
40,
41]. Macrophages derived from different compartments such as bone marrow, spleen or peritoneum have different capacities to phagocytose dextran beads [
42]. It is also possible that the different diets used, characterised by differences in calories, fat, micronutrient and protein contents, also impact on macrophage effector functions.
We have previously shown that bone marrow derived macrophages from younger mice express significantly higher levels of arginase 1 than aged mice and promote parasite growth more efficiently [
43]. Furthermore,
L. major-infected younger mice develop exacerbated lesion pathology and higher parasite burdens than aged mice [
43]. A previous study from 1984 showed that arginase was decreased in the saliva of children with different grades of PEM [
44]. We have previously compared the levels of arginase activity in the saliva of severely malnourished patients with visceral leishmaniasis and severely malnourished patients with visceral leishmaniasis and HIV co-infection and did not find significant differences or correlation between the levels of malnutrition and the levels of arginase activity [
21]; nor did we find differences when compared to healthy controls (P. Kropf, unpublished data).
Our results show that BMMΦ derived from malnourished mice express significantly more arginase in response to IL-4 or LPS, and we also measured considerably more arginase activity in the bone marrow cells and PBMCs of malnourished mice directly
ex vivo. We and others have shown that increased arginase activity is associated with the severity of a variety of infectious diseases [
20,
21,
23,
45,
46]. At least two distinct arginase-mediated mechanisms can impact on the severity of disease:
i) Increased catabolism of L-arginine by arginase results in the depletion of L-arginine from the microenvironment; since L-arginine is essential for efficient T cell activation, this decrease in L-arginine results in impaired T cell responses [
17,
18,
47,
48]. In an experimental model of leishmaniasis, we have recently shown that increased arginase activity causes local depletion of L-arginine, which impairs the capacity of T cells in the lesion to proliferate and to produce interferon-γ [
30]. Healing, induced by chemotherapy, resulted in control of arginase activity and reversal of local immunosuppression; competitive inhibition of arginase as well as supplementation with L-arginine restored T cell effector functions and reduced pathology and parasite growth at the site of lesions [
30]. Indeed, our results also show that the levels of L-arginine are lower in MN mice. L-arginine is derived from 1) turnover of cellular protein; 2) from endogenous synthesis: by
de novo synthesis from citrulline; and 3) the diet via protein, which contained from 3-15% of L-arginine [
14,
15]. It is therefore likely that insufficient level of protein in the diet result in reduced levels of L-arginine in plasma [
49‐
51]. Consequently, both PEM and increased levels of arginase might contribute to the lower level of L-arginine.
PEM malnutrition not only results in lower levels of L-arginine, it also results in severe alteration of the levels of different amino acid [
49‐
51]. It is likely that these changes impact on macrophage effector functions; for example, glutamine deprivation impacts on antigen presentation, HLA-DR expression and cytotoxic effect of TNF-α of macrophages [
52]. Furthermore, increased intracellular levels of arginase-induced L-arginine catabolites such as ornithine, putrescine, spermine and spermidine can downregulate macrophage [
53‐
55]. Of note, we have previously shown that
in vitro, L-arginine deprivation did not impact on arginase activity and NO production [
56].
ii) Increased arginase activity has also been shown to promote the growth of
Leishmania parasites directly via the polyamine synthesis in macrophages [
26]: arginase hydrolyses L-arginine to urea and ornithine; the latter is the main intracellular source for the synthesis of polyamines, which are necessary for parasite growth. Inhibition of arginase in activated BMMΦ clearly reduced parasite replication [
26]. Indeed, our results show that BMMΦ derived from MN mice express significantly more arginase and provide a more permissive environment for
Leishmania replication. Furthermore, the increased parasite burden in the spleen of MN BALB/c mice infected with
L. infantum coincides with increased arginase activity.
To the best of our knowledge, this is the first study that shows that PEM results in increased arginase activity in monocytes and macrophages, however the mechanisms responsible for this upregulation of arginase have not been identified yet. Upregulation of arginase has been extensively described in murine macrophages: cytokines such as IL-4 and IL-13, which can synergize with IL-10 and IL-21, as well as IL-6, induce the expression of arginase; in addition, lipospolysaccharide and lipoprotein, as well as inflammatory stimuli such as thioglycollate, carrageenan and casein can also induce arginase [
13]. Therefore, it is tempting to speculate that upregulation of arginase is induced as a result of PEM-induced inflammation. Whereas arginase upregulation in macrophages during PEM is STAT6- or TLRs- dependent remains to be established [
57].
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Competing interests
The authors declare that they have no competing interests.
Authors’ contributions
KC, VY, CM, HE and SS performed experiments and analyzed data. SH, PB, MMo, MMu and IM analysed data. PK designed the research, performed experiments, analyzed data and wrote the manuscript. All authors read and approved the final manuscript.