key: cord-0002058-zvnqiy9p authors: ZHANG, NAICHUN; DENG, JIANNING; WU, FENGYAO; LU, XIANGCHAN; HUANG, LEI; ZHAO, MIN title: Expression of arginase I and inducible nitric oxide synthase in the peripheral blood and lymph nodes of HIV-positive patients date: 2015-11-23 journal: Mol Med Rep DOI: 10.3892/mmr.2015.4601 sha: 4e0773d0ae56a69211b358144a99bbecbad56bac doc_id: 2058 cord_uid: zvnqiy9p Arginase I (Arg I) and inducible nitric oxide synthase (iNOS) are important in regulating immune functions through their metabolites. Previous studies have revealed that the expression of Arg I is increased and the expression of iNOS is reduced in the serum and peripheral blood mononuclear cells of human immunodeficiency virus (HIV)-infected patients. As one of the most important immune organs and HIV replication sites, whether similar changes are present in the lymph nodes following HIV infection remains to be elucidated. To investigate this, the present study collected lymph node and blood specimens from 52 HIV-infected patients to measure the expression levels of Arg I and iNOS by immunohistochemistry and fluoresence-based flow cytometry. Compared with control subjects without HIV infection, the patients with HIV had significantly higher expression levels of Arg I in the lymph nodes and higher frequencies of Arg I(+) CD4(+) T cells and CD8(+) T cells in the blood and lymph nodes, and these results were contrary the those of iNOS in the corresponding compartments. The expression levels of Arg I in the lymph nodes and blood were negatively associated with peripheral CD4(+) T cell count and positively associated with viral load. However, the expression levels of iNOS in the lymph nodes and blood were positively associated with peripheral CD4(+) T cell count and negatively associated with viral load. These results showed that alterations in the expression levels of Arg I and iNOS in the peripheral T cells and peripheral nodes of HIV infected patients are associated with disease progression in these patients. These results indicate a potential to therapeutic strategy for delaying disease progression through regulating and manipulating the expression levels of Arg I and iNOS in patients infected with HIV. At present, the trends in human immunodeficiency virus (HIV) infection remain at a high level worldwide (1) . The treatment of HIV/acquired immune deficiency syndrome (AIDS) has been challenging, although highly active antiretroviral therapy (HAART) has significantly reduced the number of new cases of HIV infection and improved the prognosis of patients with HIV/AIDS (2) . During previous decades, there have been significant advances in understanding the pathogenesis of HIV/AIDS, however certain aspects remain to be elucidated, including the functional changes in immune organs, for example the lymph nodes, following HIV infection. The damage caused by HIV infection is gradual and multi-staged, and ends in AIDS (3) . Chronic HIV infection may progressively compromise immune functions. The loss of peripheral CD4 + T lymphocytes due to continuous and severe injury has been a marker of AIDS progression and a major cause of immune dysfunction in HIV/AIDS (4) . However, HIV infection-induced chronic inflammation and the reduction in the number of CD4 + T lymphocytes does not fully explain the immune dysfunction, which occurs in the progression of HIV/AIDS. Previous studies have shown that the metabolism of L-arginine is one of the important mechanisms underlying the regulation of immune responses (5, 6) . L-arginine is a substrate of arginase (Arg), including Arg I and II, and nitric oxide synthase (NOS), including NOS1, 2 and 3). Arg I and II hydrolyzes L-arginine into L-ornithine and urea, and L-ornithine is further metabolized into polyamines, which are involved in the proliferation and differentiation of cells (7) . NOS catalyzes the conversion of L-arginine into citrulline and nitric oxide (NO), and NO is an important effector and regulator of the immune system (8, 9) . Arg I is released from immune cells, including polymorphonuclear neutrophils, during inflammation, and is also involved in the inflammatory response (10) . NOS2, or inducible NOS (iNOS) is expressed in a variety of immune cells (11) . Studies have reported that Arg I regulates the bioavailability of L-arginine, which is involved in certain immune-associated pathological processes, including inflammation-triggered immune dysfunction, immune evasion of cancer cells, fibrosis, immunosuppression and immune responses to infectious agents (5, 11, 12) . As a competitor to Arg I, iNOS hydrolyzes L-arginine into NO, which is important in destroying parasites, bacteria, viruses and cancer cells, as well as in vascular dilation (13) (14) (15) . Previous studies have revealed that the expression of Arg I is increased (16, 17) and the expression of iNOS is reduced (18) in the serum and peripheral blood mononuclear cells (PBMCs) of patients with HIV. However, the expression levels of Arg I and iNOS in the peripheral lymph nodes (LNs) of HIV-infected patients remains to be fully elucidated. In the present study, the expression levels of Arg I and iNOS in peripheral LNs and peripheral T cells were investigated, with the aim of elucidating the roles of Arg I and iNOS in the progression of HIV/AIDS. Informed consent was obtained prior to surgical resection of the LNs, and the study was approved by the Ethics Committees of the 302 Hospital of PLA (Beijing, China) and the 4th People's Hospital of Nanning (Nanning, China). LNs were routinely collected during surgery from the neck (n=27), armpit (n=20) and groin (n=5), and were processed for further examination. At the same time, 10 ml peripheral blood was collected from the patient and control groups. HIV/AIDS was diagnosed according to the Guidelines for the Use of Antiretroviral Agents in HIV-1-infected Adults and Adolescents (USDHHS 2013) (19), and these patients were divided into an asymptomatic group (n=19) and an AIDS group (n=33). In addition, peripheral superficial biopsies of the LNs were collected from the neck and armpit of 13 subjects without HIV infection, recruited from the 302 Hospital of PLA, and were processed for pathological examination by two experienced pathologists. Exclusion criteria included the presence of cancer, infection and autoimmune diseases, and the presence of reactive hyperplasia was confirmed in those subjects who then served as controls. In addition, peripheral blood was collected from 20 healthy control subjects. Absolute CD4 + T cell count. The peripheral blood CD4 + T-cell counts were determined using the Multitest Imk Lymphocyte kit (cat. no. 340503; BD Biosciences, San Jose, CA, USA) and Trucount tubes (cat. no. 340504; BD Biosciences). 50 µl whole blood was collected and incubated with 10 µl antibodies for 20 min at room temperature. 1X BD Multitest IMK kit lysis solution was subsequently added to the tubes and after 15 min of incubation at room temperature, CD4 + T cells were counted using flow cytometry (FACSCanto II; BD Biosciences). Detection of viral load. Blood was processed within 2-4 h post-collection by centrifugation for 10 min at 1,100 x g for plasma separation, followed by HIV RNA extraction by using a Roche Cobas AmpliPrep/Cobas TaqMan automatic analysis system (Roche Diagnostics; Basel, Switzerland, USA). The viral load was quantitatively measured using a Roche Cobas AmpliPrep/Cobas TaqMan HIV-1 test kit (version 2.0; Roche Diagnostics) according to the manufacturer's instruction. Separation of mononuclear cells from LNs. The LNs were minced and filtered through a 100 mesh filter (pore size, 150 µm; xbs-100; Shanghai 3bio, Shanghai, China), and the filtrate was retained and layered onto Ficoll-Paque™ PLUS (cat. no. 17-1440-02; GE Healthcare, Little Chalfont, UK) and centrifuged at 800 x g for 15 min at 20˚C to obtain mononuclear cells, which included lymphocytes (20, 21) . Detection of the expression levels of Arg I and iNOS using streptomycin avidin-biotin-peroxidase complex immunohistochemical analysis. The LNs were collected, fixed in 4% paraformaldehyde (Beijing Chemical Works, Beijing, China), embedded in paraffin (Leica Biosystems, Nussloch, Germany) and sectioned (4 µm). Briefly, the slides were washed in xylene (ZSGB-BIO, Beijing, China) to remove the paraffin, rehydrated through serial dilutions of alcohol (Beijing Chemical Works), followed by washing with phosphate-buffered saline (PBS; pH 7.2; ZLI-9062, ZSGB-BIO). Treated slides were then placed in a 0.01-mol/l citrate buffer (pH 6.0; ZSGB-BIO) and heated in a microwave oven for 15 min for retrieval of antigens, treated with 1.5% H 2 O 2 (Beijing Chemical Works) in methanol (Beijing Chemical Works) to inactivate endogenous peroxidase and treated with fetal bovine serum (Invitrogen; Thermo Fisher Scientific, Waltham, MA, USA) to block non-specific binding. The sections were then incubated overnight at 4˚C with anti-hArginase1 antibody [cat. no. IC8026P; monoclonal mouse immunoglobulin (Ig) G2B; clone 658922; 1:350 dilution; R&D Systems, Minneapolis, MN, USA], anti-iNOS antibody (cat. no. ab15323; rabbit polyclonal; 1:80 dilution; Abcam, Cambridge, UK) and washed three times with PBS, followed by incubation with horseradish peroxidase (HRP)-conjugated secondary antibody (cat no. D39-110; Polink-2 Plus HRP Rabbit for DAB Bulk kit; or cat no. D37-110; Polink-2 Plus HRP DAB Mouse Bulk kit; Golden Bridge International, Bothell, WA, USA) for 15 min at 37˚C. The sections were then incubated with 3,3-diaminobenzidine (ZSGB-BIO) to visualize the expression of Arg I and iNOS. Positive cells contained brown granules. As a negative control for the LNs from HIV-infected patients, phosphate-buffered saline was used in place of the primary antibody. LN sections from subjects without HIV were treated with primary antibody also served as a control. Determination and image capture. The specimens were evaluated semi-quantitatively by two pathologists in a blinded-manner (22) . The frequencies of positive cells to total cells at x200 magnification were scored as follows: 1, ≤25%; 2, 26-50%; 3, >51%. The staining intensity above the background level was scored as follows: 0, no staining; 1, light yellow; 2, yellow-brown; 3, brown. These scores served as measures of target protein expression. The final score was the product of the above two scores: 0, negative (-); 1-2, weakly positive (+); 3-4, positive (++); 6-9, strongly positive (+++). Slides were mounted with gum for examination and captured using an Olympus BX51 microscope (Olympus Corp., Tokyo, Japan) and a Nikon Digital Camera System (80i; Nikon Corp., Tokyo, Japan) for study comparison. For this evaluation, five fields were randomly selected per section (magnification, x200). Detection of the expression levels of Arg I and iNOS using flow cytometry. The mononuclear cells from the peripheral blood or LNs were added to three tubes (2-5x10 5 cells/tube), and were incubated with anti-CD3-fluorescein isothiocyanate (cat. no. 349201; monoclonal mouse IgG1; clone SK7; BD Biosciences) and anti-CD8-peridinin chlorophyll protein (cat. no. 347314; monoclonal mouse IgG1; clone SK1; BD Biosciences) and permeabilized using a Cytofix/Cytoperm Fixation/Permeabilization kit (BD Biosciences). Subsequently, the three tubes (Arg, iNOS and isotype control) were divided into three groups and either anti-hArginase1-phycoerythrin (cat. no. IC8026P; monoclonal mouse IgG2B; clone 658922; R&D Systems), anti-iNOS antibody (cat. no. ab15323; rabbit polyclonal; Abcam) or isotype control antibody (cat. no. IC0041P; monoclonal mouse IgG2B; clone 133303; R&D Systems) was added to one tube containing peripheral blood mononuclear cells and one tube containing LN mononuclear cells. 1XBD Perm/Wash™ Buffer from the kit was used for washing. The cells in the iNOS group were incubated with goat anti-rabbit IgG-allophycocyanin (cat. no. ab130805; polyclonal; Abcam) for 15 min at 20˚C and fixed in 1% paraformaldehyde for 24 h. Flow cytometry was performed within 24 h using a FACSCanto II flow cytometer (BD Biosciences). FlowJo software (version 7.6.1; FlowJo LLC, Ashland, OR, Canada) was used to analyze the data. The lymphocytes were gated based on forward scatter/side scatter, which were further separated into CD8 + T cells (CD3 + /CD8 + ) and CD4 + T cells (CD3 + /CD8 -), and the expression levels of Arg I and iNOS were analyzed. Statistical analysis. Statistical analysis was performed using SPSS version 17.0 (SPSS, Inc., Chicago, IL, USA). Continuous variables were compared using analysis of variance (ANOVA) and one-way ANOVA was used to evaluate the differences among groups. Non-continuous variables were compared using a Mann-Whitney U test between two groups and Kruskal-Wallis H non-parametric test among groups. Correlation was evaluated using Pearson's or Spearman's correlation analysis. P<0.05 was considered to indicate a statistically significant difference. In order to determine changes in the expression levels of Arg I and iNOS in LNs following HIV infection, the present study firstly evaluated the expression levels of Arg I and iNOS in peripheral LNs in situ using immunohistochemistry. The results showed that Arg I was predominantly expressed in the cytoplasm, and the levels of expression varied among the groups, between negative to strongly positive. In the control group (Fig. 1A) , the expression of Arg I was most weakly positive or positive, whereas the expression levels of Arg I in the patient groups ( Fig. 1B and 1C) , were almost positive or strongly positive. By contrast, the expression of iNOS exhibited the opposite trend to the changes in the expression of Arg I, with the expression of iNOS being positive in the control group (Fig. 1D) , and positive, weakly positive or negative in the patient groups ( Fig. 1E and F) . Taken together, the results of the immunohistochemical analyses showed that, in the patient groups, the expression levels of Arg I were significantly higher, compared with the control group (P<0.01; Fig. 1G ), whereas the expression levels of iNOS were significantly lower, compared with the control group (P<0.05; Fig. 1H ). No significant differences were observed between the asymptomatic and AIDS groups (P>0.05). Expression levels of Arg I and iNOS in the peripheral T cells of patients with HIV/AIDS. Subsequently, the present study detected the frequencies of Arg I + and iNOS + CD4 + T cells and CD8 + T cells, which were isolated from the peripheral blood samples or LN tissues of the asymptomatic patients, symptomatic patients with AIDS and controls. Flow cytometry was performed to further assess the changes in the expression levels of Arg I and iNOS in the T lymphocyte subsets. In the asymptomatic and symptomatic AIDS groups, the frequencies of CD4 + T cells positive for Arg I in the peripheral blood were significantly higher, compared with the control (P<0.05), and the frequencies of CD4 + T cells positive for iNOS in the peripheral blood were significantly lower, compared with the control (P<0.05) (Fig. 2 ). In addition, the frequencies of CD8 + T cells positive for Arg I in the peripheral blood were significantly higher, compared with the control (P<0.05), and those positive for iNOS in the peripheral blood were significantly lower, compared with the control (P<0.05) (Fig. 3) . However, the frequencies were similar between these patient groups (P>0.05). Analogous results were obtained from peripheral LNs. In the two patient groups, the frequencies of CD4 + T cells positive for Arg I in the peripheral LNs were significantly higher (P<0.05), and those positive for iNOS were significantly lower (P<0.05), compared with the controls (Fig. 4) . The frequencies of CD8 + T positive for Arg I in the peripheral LNs cells were significantly higher (P<0.05), and those positive for iNOS were significantly lower (P<0.05), compared with the control (Fig. 5) . The frequencies did not differ significantly among the patient groups (P>0.05). Correlation between the expression levels of Arg I and iNOS, and CD4 + T cell counts. The CD4 + T cell count is an important clinical indicator of the progression of AIDS (23) . To investigate the effects of Arg I and iNOS on the progression of AIDS, the associations between the peripheral blood CD4 + T cell count and the frequencies of CD4 + T cells and CD8 + T cells positive for Arg I and iNOS were examined in the peripheral blood and peripheral LNs. The protein expression levels of Arg I and iNOS in the peripheral LNs were also evaluated. As shown in Fig. 6 , the peripheral CD4 + T cell count was negatively associated with the frequencies of CD4 + T cells and CD8 + T cells positive for Arg I in the peripheral blood (r=-0.393; P<0.01 and r=-0.527; P<0.01; respectively) and peripheral LNs (r=-0.326; P<0.01; and r=-0.292; P=0.036, respectively). However, the peripheral CD4 + T cell count was positively associated with the frequencies of iNOS + CD4 + T cells and CD8 + T cells in the peripheral blood (r=0.690; P<0.01 and r=0.604; P<0.01; respectively) and peripheral LNs (r=0.596; P<0.01 and r=0.611; P<0.01, respectively; Fig. 6 ). Correlation between the expression levels of Arg I and iNOS, and viral load. Viral load is another important indicator used to evaluate the severity of AIDS. Therefore, the present study also evaluated the association between the viral load and the frequencies of CD4 + T cells and CD8 + T cells positive for Arg I or iNOS in the peripheral blood and LNs. The association with the protein expression levels of Arg I and iNOS in the peripheral LNs were also examined. As shown in Fig. 7 , viral load was positively associated with the frequencies of Arg I positive CD4 + T cells and CD8 + T cells in the peripheral blood (r=0.495; P<0.01 and r=0.307; P=0.027, respectively), peripheral LNs (r=0.546; P<0.01 and r=0.458; P<0.01, respectively). However, the viral load was negatively associated with the frequencies of iNOS positive CD4 + T cells and CD8 + T cells in the peripheral blood (r=-0.735; P<0.01 and r=-0.757; P<0.01, respectively), peripheral LNs (r=-0.778; P<0.01 and r=-0.670; P<0.01, respectively). In terms of protein expression levels, the peripheral CD4 + T cell count was negatively associated with the protein expression of Arg I (r=-0.563; P<0.01; Fig. 8A ) and the viral load was positively associated with the protein expression of Arg I in the LNs (r=0.736; P<0.01; Fig. 8B ). Furthermore, the peripheral CD4 + T cell count was positively associated with the expression of iNOS (r=0.394; P<0.01; Fig. 8C ) in the LNs. The viral load as negatively associated with the protein expression of iNOS in the LNs (r=-0.529; P<0.01; Fig. 8D ). As one of the most important amino acids, L-arginine can exert a variety of biological effects. It is involved in the synthesis of proteins, urea, creatine and NO (24) , and is metabolized in the human body via the 'Arg pathway' and 'iNOS pathway,' which differ in their effects on immune function. As mentioned above, the expression of Arg I is increased (16, 17) and the expression of iNOS is reduced (18) in the serum and PBMCs of HIV-infected patients. LNs are important sites for the proliferation, differentiation and development of lymphocytes, and are crucial in the maintenance of normal immune function (25) . Changes in the metabolism of LNs by L-arginine remains to be fully elucidated in patients with HIV infection. Therefore, in the present study, immunohistochemistry and flow cytometry were used to detect the expression levels of Arg I and iNOS in peripheral T cells and LNs. The results showed that, compared with controls, asymptomatic and symptomatic HIV infected patients exhibited increased frequencies of Arg I positive CD4 + T cells and CD8 + T cells in the peripheral blood and LNs, and increased protein expression levels of Arg I in the LNs. In addition, the frequencies of Arg I positive CD4 + T cells and CD8 + T cells in the peripheral blood and LNs, and the protein expression levels of Arg I in the LNs were negatively associated with peripheral CD4 + T cell count and positively correlated with HIV load. By contrast, the frequencies of iNOS positive CD4 + T cells and CD8 + T cells in the peripheral blood and LNs, and the protein expression levels of iNOS were decreased in the LNs of HIV-infected patients, compared with controls. Furthermore, the frequencies of iNOS positive CD4 + T cells and CD8 + T cells in the peripheral blood and LNs, and the protein expression levels of iNOS in the LNs were positively associated with peripheral CD4 + T cell count and negatively associated with HIV load. In arginine-mediated metabolism, L-arginine is hydrolyzed into urea and ornithine, and ornithine is a precursor of polyamines, which are indispensable for the proliferation of cells and parasites (5, (26) (27) (28) . At least two subtypes of arginase have been identified in mammals: Cytoplasmic Arg I and mitochondrial Arg II (29) . These are involved in the same reaction (30) , although Arg I is more important in the urea cycle of the liver. In addition to its role in L-arginine metabolism, Arg is important for immune system function (31,32) as it can inhibit NO synthesis, induce fibrosis and tissue regeneration (33, 34) . Arg is also involved in multiple inflammatory diseases, and is essential for normal T cell function (6, 35, 36) . In myeloid cells, Arg I downregulates CD3ζ-chain expression, and inhibits the expression of cell cycle regulatory protein D3 and cell cycle regulatory protein-dependent kinase 4, leading to the inhibition of T cell activation and subsequent suppression of the immune function of T cells (37, 38) . This mechanism is important in the immunosuppression of certain inflammation-associated conditions. Helicobacter pylori and Toxoplasma gondii, may use arginine to induce inflammation-associated immune suppression, leading to immune evasion (12, 31, 32, 39) . In the NOS pathway, L-arginine is metabolized by iNOS into citrulline and NO, and NO is important in the destruction of cancer cells, viruses, bacteria and parasites and in regulation of a variety of immune cells (40) . NOS has three isoforms, which include two constitutive isoforms, neural NOS and endothelial NOS, and one inducible isoform (iNOS) (41) . Constitutive NOS is predominantly involved in the physiological synthesis of NO and the regulation of different physiological functions, and its activity is Ca2 + -dependent (42) . However, iNOS is predominantly involved in the immune regulation and pro-inflammatory response (43, 44) . L-arginine is a substrate of Arg and iNOS, therefore, high expression levels of Arg may deplete L-arginine and increase levels of ornithine and polyamines, which are required for the proliferation of cells and parasites. A reduction in L-arginine causes a decrease in NO through the iNOS pathway (11) . The competition between Arg and iNOS is pivotal in the immune response to infection and determines the course of infection. For example, the peritoneal macrophages in rats differ from those in mice by being resistant to Toxoplasma gondi infection in nature. This resistance has been ascribed to the increased expression and activity of iNOS and, reduced activity of Arg I in rat peritoneal macrophages, compared with mouse peritoneal macrophages (12) . HIV infection significantly reduces the number of CD4 + T cells, particularly in the AIDS phase, and as polyamine, which is the metabolic product of L-arginine by Arg, is an essential substrate for cell proliferation, increased Arg I in the peripheral blood and LNs can increase the number of CD4 + T cells following HIV infection (11) . The results of the present study indicated the negative correlation between the expression of Arg I in peripheral T cells and LNs and peripheral CD4 + T cell count, suggesting that the expression of Arg I increased to compensate for the reduction in CD4 + T cells. However, L-arginine regulates the transcription of iNOS in a concentration-dependent manner (39) and Arg significantly reduces the levels of L-arginine, leading to reduction in iNOS synthesis. Thus, the increase in the expression levels This Arg-induced reduction in iNOS synthesis leads to a reduction in the production of NO, and this release of NO by macrophages is important role in innate immunity (11) . The reduced synthesis of NO may directly impair innate (6, 45, 46) . All these factors contribute to the significant increase in HIV replication and compromise anti-infection ability in the AIDS phase, resulting in the development of opportunistic infections. The reduction in NO due to the competition between Arg and iNOS is also important in the pathogenesis of a variety of diseases, including atherosclerosis and hypertension, myocardial ischemia/reperfusion injury, diabetes, allergic asthma and inflammatory diseases (47) (48) (49) (50) . Thus, as an important metabolic enzyme, which affects NO synthesis, mechanisms to inhibit the progression of disease by inhibiting Arg activity and functional interference remains an area of increased interest. Certain synthetic and natural compounds that inhibit Arg have been investigated as disease therapies, with certain small molecule inhibitors of Arg showing potential in the treatment of diabetes, allergic inflammation and Schistosoma mansoni parasitic infection (47, 51, 52) . At the same time, evidence in rats shows that Arg I may serve as a biomarker for the diagnosis of type 2 diabetes (53) . The results of the present study also showed that HIV load and peripheral CD4 + T cells were independently associated with the expression levels of Arg I and iNOS. Thus, although HAART may exert therapeutic effects by reducing the expression of Arg I and increasing the expression of iNOS, Arg inhibitors may be used as an adjuvant therapy to treat HIV infection, particularly in those with AIDS, and to improve immune function, prevent opportunistic infections and inhibit viral replication. In addition, this correlation suggests that the expression levels of Arg I and iNOS in peripheral T cells may be used diagnostically to predict the progression of HIV infections. In conclusion, the present study suggested that abnormalities in the expression levels of Arg I and iNOS in peripheral blood and LN T cells may be a contributor to compromised immunity in patients with HIV, which are responsible for the significant elevations in viral load during the AIDS phase and the appearance of opportunistic infections. In addition, the expression levels of Arg I and iNOS in the T cells of peripheral blood and LNs may be as a potential parameter to predict disease progression, as the expression levels of Arg I and iNOS in peripheral blood and LN T cells were found to be correlated with HIV load and CD4 + T cell count. 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