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A method for multiple sequential analyses of macrophage functions using a small single cell sample

Abstract

Microbial pathogens such as bacillus Calmette-Guérin (BCG) induce the activation of macrophages. Activated macrophages can be characterized by the increased production of reactive oxygen and nitrogen metabolites, generated via NADPH oxidase and inducible nitric oxide synthase, respectively, and by the increased expression of major histocompatibility complex class II molecules (MHC II). Multiple microassays have been developed to measure these parameters. Usually each assay requires 2-5 x 10(5) cells per well. In some experimental conditions the number of cells is the limiting factor for the phenotypic characterization of macrophages. Here we describe a method whereby this limitation can be circumvented. Using a single 96-well microassay and a very small number of peritoneal cells obtained from C3H/HePas mice, containing as little as <=2 x 10(5) macrophages per well, we determined sequentially the oxidative burst (H2O2), nitric oxide production and MHC II (IAk) expression of BCG-activated macrophages. More specifically, with 100 µl of cell suspension it was possible to quantify H2O2 release and nitric oxide production after 1 and 48 h, respectively, and IAk expression after 48 h of cell culture. In addition, this microassay is easy to perform, highly reproducible and more economical.

Macrophages; Nitric oxide; Hydrogen peroxide; MHC II; Method


Braz J Med Biol Res, September 2003, Volume 36(9) 1221-1226

A method for multiple sequential analyses of macrophage functions using a small single cell sample

F.R.F. Nascimento*, D. Rodríguez*, E. Gomes, E.C. Fernvik and M. Russo

Departamento de Imunologia, Instituto de Ciências Biomédicas, Universidade de São Paulo, São Paulo, SP, Brasil

References

Correspondence and Footnotes Correspondence and Footnotes Correspondence and Footnotes

Abstract

Microbial pathogens such as bacillus Calmette-Guérin (BCG) induce the activation of macrophages. Activated macrophages can be characterized by the increased production of reactive oxygen and nitrogen metabolites, generated via NADPH oxidase and inducible nitric oxide synthase, respectively, and by the increased expression of major histocompatibility complex class II molecules (MHC II). Multiple microassays have been developed to measure these parameters. Usually each assay requires 2-5 x 105 cells per well. In some experimental conditions the number of cells is the limiting factor for the phenotypic characterization of macrophages. Here we describe a method whereby this limitation can be circumvented. Using a single 96-well microassay and a very small number of peritoneal cells obtained from C3H/HePas mice, containing as little as £2 x 105 macrophages per well, we determined sequentially the oxidative burst (H2O2), nitric oxide production and MHC II (IAk) expression of BCG-activated macrophages. More specifically, with 100 µl of cell suspension it was possible to quantify H2O2 release and nitric oxide production after 1 and 48 h, respectively, and IAk expression after 48 h of cell culture. In addition, this microassay is easy to perform, highly reproducible and more economical.

Key words: Macrophages, Nitric oxide, Hydrogen peroxide, MHC II, Method

Introduction

Activated macrophages play an essential role in innate and T cell-mediated immunity. In the process of activation, macrophages undergo profound functional changes that result in enhanced antimicrobial and anti-tumor activities and an increased capacity to present antigens to T cells. The microbicidal and tumoricidal activities are associated with the generation of highly toxic molecules derived from reduction of oxygen or oxidation of nitrogen, referred to as reactive oxygen intermediates and reactive nitrogen intermediates (1,2). The increased capacity to present antigens is associated with an increased expression of major histocompatibility complex (MHC) molecules (3).

Microassays measuring reactive oxygen and nitrogen intermediate production and MHC class II expression have been developed to evaluate macrophage functions. Since the limiting factor usually is the number of cells available the drawback of these methods is the amount of cells required for measuring these three macrophage functions, i.e., roughly one million cells. However, in some experimental conditions the number of available cells is less than one million. Keeping this in mind, we developed a 96-well microassay in which multiple macrophage functional parameters could be determined sequentially with a small number of cells (2 x 105 macrophages per well). The results were compared to those obtained with multiple samples. The parameters analyzed were macrophage hydrogen peroxide (H2O2) release, nitric oxide (NO) production and the expression of MHC class II antigens (IAk).

We show that the results obtained with a single macrophage sample (2 x 105 cells) are similar to those obtained with multiple samples of the same macrophage population. Moreover, the microassay permits the measurement of more than three macrophage functions with only 2 x 105 cells and it is easy to perform, highly reproducible and economical.

Material and Methods

Mice

C3H/HePas mice were originally obtained as breeding units from Institut Pasteur (Paris, France) and have been maintained for many generations in our own Animal Breeding Unit (Biotério de Camundongos Isogênicos, ICB, USP, São Paulo, SP, Brazil) under standard pathogen-free conditions. Animals were age and sex matched, fed sterilized food and acidified water and treated according to ICB-USP Animal Welfare guidelines.

Bacillus Calmette-Guérin treatment

C3H/HePas mice received two intraperitoneal (ip) injections of 2 mg bacillus Calmette-Guérin (BCG, ONCO oral BCG, 500 mg; Instituto Butantan, São Paulo, SP, Brazil) on day 0 and day 14. Control animals received two ip injections with phosphate-buffered saline (PBS). The peritoneal cells were harvested four days after the last injection.

Peritoneal cell harvesting

Mice were killed by CO2 asphyxia and the peritoneal cells were aseptically collected by washing the peritoneal cavity with 5 ml sterile ice-cold PBS devoid of calcium and magnesium ions. Total cell counts were performed using a bright-line hemacytometer (Sigma, St. Louis, MO, USA).

Single analysis of macrophage functions using multiple macrophage samples

Two million peritoneal cells from individual mice were centrifuged at 160 g for 10 min at 4ºC and suspended in 1 ml phenol red solution, or complete RPMI 1640 medium or PBS with 5% fetal calf serum (FCS) for determination of H2O2 release, NO production and IAk expression as described elsewhere (4-7). In all microassays 100 µl of the cell suspensions was plated onto each well of a 96-well flat-bottomed tissue culture plate (Corning, New York, NY, USA).

Hydrogen peroxide assay

H2O2 release was measured using the horseradish peroxidase-dependent phenol red oxidation microassay (6). The phenol red solution was freshly prepared and consisted of ice-cold Dulbecco's PBS containing 5.5 mM dextrose, 0.56 mM phenol red (Sigma) and 8.5 U/ml horseradish peroxidase type II (Sigma). Peritoneal cells suspended in fresh phenol red solution were incubated for 1 h at 37ºC in a humid atmosphere containing 5% CO2-95% air. The reaction was stopped with 10 µl 1 N NaOH. Absorbance at 620 nm was measured with a microplate reader (MR 5000, Dynatech Laboratories Inc., Gainesville, VA, USA). Conversion of absorbance to µM H2O2 was deduced from a standard curve obtained with known concentrations of H2O2 (5 to 40 µM) as described by Pick and Keisari (4).

Nitric oxide assay

For NO determinations, peritoneal cells were suspended in RPMI 1640 medium supplemented with 10 mM HEPES, 11 mM sodium bicarbonate, 100 U/ml penicillin, 100 µg/ml streptomycin, 2 mM L-glutamine, 23 mM L-asparagine, 1 mM folic acid, 0.1 mM pyruvic acid, and 5% FCS. After plating, the cells were incubated for 48 h at 37ºC in a humid atmosphere containing 5% CO2-95% air. The accumulation of nitrite (a stable end product of NO) in supernatants was determined with the standard Griess reagent (5). Briefly, 50 µl of the supernatants was incubated with an equal volume of Griess reagent (1% sulfanilamide/0.1% naphthalene diamine dihydrochloride/2.5% H3PO4) at room temperature for 10 min and absorbance at 550 nm was determined. Conversion of absorbance to µM NO was deduced from a standard curve using known concentration (5-60 µM) of sodium nitrite diluted in RPMI medium.

IA k expression

IAk expression by the peritoneal macrophages was determined by cell-ELISA using a mouse H-39.487.7 (IgG2a) anti-IAk biotinylated monoclonal antibody as described previously (7-9). Briefly, 100 µl of peritoneal cells was suspended in PBS-10% FCS and incubated for 1 h at 37ºC in a humid atmosphere containing 5% CO2-95% air. The nonadherent cells were removed by gentle washing of the wells with PBS-5% FCS three times. The remaining adherent cells were fixed with 1% paraformaldehyde dissolved in PBS for 15 min, washed twice with PBS-0.05% Tween 20 (PBS-T20), and incubated for 30 min with 1 µg/ml of the anti-IAk biotinylated monoclonal antibody. The plates were washed five times with PBS-T20 and 25 µl of ExtrAvidin peroxidase conjugate (Sigma) diluted 1:10,000 in PBS was added to each well. After incubation for 15 min at room temperature, the wells were rinsed five times with PBS-T20. Five milligrams ortho-phenylenediamine (Sigma) was diluted in 10 ml sodium citrate buffer (0.1 M sodium citrate plus 0.1 M citric acid, pH 5.0) containing 5 µl H2O2 (30%). Ortho-phenylenediamine was added to each well (100 µl) and the plate was incubated at room temperature in the dark for 15 min. The reaction was stopped with 50 µl 4 N sulfuric acid per well and absorbance at 492 nm was determined.

Sequential analyses of macrophage functions using a single sample of macrophages

In a single macrophage sample we sequentially determined H2O2 release, NO production and IAk expression using the same standardized microassays as described above.

Macrophages were harvested and two million peritoneal cells were suspended in 1 ml freshly prepared phenol red solution. One hundred microliters of the cell suspension (60-80% macrophages) was plated onto each well and incubated for 1 h at 37ºC in a humid atmosphere containing 5% CO2-95% air. The plates were centrifuged once at 150 g for 3 min and the supernatants were collected for H2O2 determination as described above. Next, the wells were washed three times with PBS and the remaining adherent cells were cultured in complete RPMI 1640 medium (100 µl/well) for 48 h. The supernatants were collected and NO production was quantified as described above. Finally, the plates were washed again with PBS and fixed with 25 µl 1% paraformaldehyde for 15 min. After washing three times with PBS the plates were incubated for 15 min in the presence of PBS containing 0.045% H2O2 (100 µl/well) to quench peroxidase activity. After this step, the cell-ELISA assay for MHC class II expression was performed as described above.

Statistical analysis

Statistical significance was determined by ANOVA, with the level of significance set at P < 0.05. All analyses were carried out using the Instant Program (Graph PAD Software, Inc., San Diego, CA, USA). All determinations were performed in quadruplicate and the results are reported as means ± SEM.

Results and Discussion

Comparison between the multiple analysis and single analysis methods

We first determined the macrophage functions by standard methods that use single analysis and multiple samples. We observed that BCG-activated macrophages release and produce large amounts of H2O2 and NO and express high levels of IAk molecules as compared to nonactivated control macrophages (Figure 1A,C and E). These results demonstrate that our protocol of BCG administration is highly effective in inducing macrophage activation. Next, we determined macrophage functions by the multiple analysis method using a single cell sample. For this procedure we sequentially determined H2O2 release, NO production and IAk expression. The results obtained were statistically equivalent to those obtained by the standard methods employing single analysis of macrophage functions using multiple cell samples (Figure 1B,D and F). Although not statistically significant, the results of IAk expression obtained were always lower for the multiple analysis method compared to the single analysis method. The lower IAk expression might be due to the time of macrophage culture. Using single analysis, IAk expression is measured immediately after cell harvesting, while in multiple analyses it is measured after 48 h. Nevertheless, our results clearly show that when using a single macrophage sample it is possible to determine at least three macrophage functions as accurately as when using standard microassays with multiple macrophage samples. Actually, with the multiple analysis method it is possible to measure more than three functions. For instance, it is possible to analyze macrophage spreading after performing the H2O2 analysis. For this, the number of spread macrophages can be quantified under an inverted phase contrast microscope as described by Rabinovitch et al. (10). Moreover, it is possible to measure different macrophage products such as TNF, GM-CSF, etc., by collecting the supernatants (50 µl) from the wells at different time intervals (data not shown).

However, when using the multiple function analysis method, it is fundamental to determine that the measurement of one macrophage function does not interfere with the macrophage response subsequently analyzed. For instance, phorbol myristate acetate (PMA) is often used to trigger the oxidative burst (11). Since PMA activates protein kinase C (12) and this enzyme is known to influence NO production (13), PMA should be avoided or a second macrophage sample without PMA run in parallel should be included. In our experiments we did not include PMA because, as shown previously, freshly explanted BCG-activated macrophages release spontaneously large amounts of H2O2 (14). In contrast, concanavalin A-stimulated macrophages only release significant amounts of H2O2 when PMA is present (15). Therefore, we suggest that for sequential determination of reactive oxygen and nitrogen intermediate production, at least two macrophage samples (with and without PMA) should be included in the experiment. Another relevant point regarding H2O2 determination in the peritoneal cell population is the number of polymorphonuclear cells present in the peritoneal exudates. In the BCG model, at the time of cell harvesting the number of polymorphonuclear cells was minimal and did not interfere with the assay (data not shown). However, if the percentage of polymorphonuclear cells exceeds 5%, an adhesion step for selecting macrophages is required. Thus, peritoneal cells suspended in Ca2+- and Mg2+-free PBS should be allowed to adhere to a 96-well plate for 30 min and, after one PBS washing, the nonadherent cells (including polymorphonuclear cells) are easily removed.

Finally, we wish to emphasize that the major advantage of the multiple function analysis method is that it requires as few as 200,000 cells. Moreover, the method is easy to perform, reproducible and more economical.

Figure 1.
Comparison of H2O2 release, NO production and MHC class II (IAk) expression by bacillus Calmette-Guérin (BCG)-activated peritoneal macrophages. C3H/HePas mice were injected ip with 2 mg BCG or 0.2 ml PBS at days 0 and 14 and the macrophage functions determined 4 days later. H2O2 release, NO production and MHC II expression were determined using multiple cell samples (left) or a single cell sample (right). H2O2 release (A and B) was quantified 1 h after cell culture. NO production (C and D) was determined 48 h after cell culture. IAk expression was evaluated after 1 h using multiple cell samples (E) or 48 h after cell culture using a single cell sample (F). One representative experiment of three is shown. Results are reported as means ± SEM (N = 5). *P < 0.05 for BCG compared to control (ANOVA). There was no statistical difference between single and multiple analyses (ANOVA). MHC, major histocompatibility complex; NO, nitric oxide.

Acknowledgments

We thank Nancy Starobinas, Instituto Butantan, São Paulo, SP, Brazil, for helpful suggestions.

Address for correspondence: M. Russo, Departamento de Imunologia, ICB IV, USP, Av. Prof. Lineu Prestes, 1730, 05508-900 São Paulo, SP, Brasil. Fax: +55-11-3091-7377. E-mail: momrusso@icb.usp.br

Research supported by FAPESP and CNPq. *Both authors contributed equally to the work. Received November 13, 2002. Accepted May 23, 2003.

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  • Correspondence and Footnotes

  • Publication Dates

    • Publication in this collection
      19 Aug 2003
    • Date of issue
      Sept 2003

    History

    • Accepted
      23 May 2003
    • Received
      13 Nov 2002
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