Superoxide anion production by human neutrophils activated by Trichomonas vaginalis.

Neutrophils are the predominant inflammatory cells found in vaginal discharges of patients infected with Trichomonas vaginalis. In this study, we examined superoxide anion (O2 (.-)) production by neutrophils activated by T. vaginalis. Human neutrophils produced superoxide anions when stimulated with either a lysate of T. vaginalis, its membrane component (MC), or excretory-secretory product (ESP). To assess the role of trichomonad protease in production of superoxide anions by neutrophils, T. vaginalis lysate, ESP, and MC were each pretreated with a protease inhibitor cocktail before incubation with neutrophils. Superoxide anion production was significantly decreased by this treatment. Trichomonad growth was inhibited by preincubation with supernatants of neutrophils incubated for 3 hr with T. vaginalis lysate. Furthermore, myeloperoxidase (MPO) production by neutrophils was stimulated by live trichomonads. These results indicate that the production of superoxide anions and MPO by neutrophils stimulated with T. vaginalis may be a part of defense mechanisms of neutrophils in trichomoniasis.

Trichomonas vaginalis is a sexually-transmitted flagellate with a worldwide distribution [1,2]. In the Republic of Korea (=Korea), the prevalence of T. vaginalis in women in Kangwon-do (from 1988 to 1993) and Gyeonggi-do (from 1996 to 1997) were reported to be 7.6% and 10.4%, respectively [3,4]. In men, T. vaginalis infection can cause urethritis and prostatitis, and T. vaginalis has been detected by PCR in specimens of Korean patients with chronic urethritis or prostatitis [5,6].

Numerous neutrophils have been detected in the vaginal discharge of trichomonal vaginitis patients, and attachment of trichomonads to neutrophils has also been observed [1]. Superoxide anions (O2.-) are known to play an important role in the protective mechanisms of neutrophils, but it is unclear whether they generate superoxide anions against T. vaginalis. When superoxide dismutase and catalase (which can scavenge superoxide anions and hydrogen peroxide, respectively) were added to cocultures of trichomonads and neutrophils, fewer trichomonads were killed than in the absence of these enzymes [7]. These findings demonstrated the importance of reactive oxygen species (ROS) such as superoxide anions and hydrogen peroxide in killing T. vaginalis by neutrophils. Various oxidants generated by myeloperoxidase, a heme enzyme released from intracellular granules of neutrophils, are known to play an important role in immune responses to invading pathogens [8]. In this study, we evaluated the production of superoxide anion and myeloperoxidase by neutrophils stimulated with trichomonads.

The human trichomonad, T. vaginalis (KT4 isolate), was obtained from the vaginal discharge of a Korean woman with vaginitis [9]. It was subcultured every 24 hr in screw-capped glass test tubes containing 15 ml of Diamond's trypticase-yeast extract-maltose (TYM) medium [10]. Lysates, membrane components (MC), and excretory-secretory products (ESP) were prepared as described previously with minor modifications. Briefly, T. vaginalis were harvested in log phase and washed by centrifugation. They were lysed by 3 bursts at 15 sec intervals from a sonicator (Heat System-Ultrasonics, Farmingdale, New York, USA), then centrifuged at 10,000 g for 30 min. The resulting supernatants were used as T. vaginalis lysates after filtration through 0.22 µm filters [11]. To prepare the membrane component of T. vaginalis, trichomonads were homogenized in Tris-lysis buffer (1 mM EDTA, 1 mM EGTA, 1 mM PMSF) (Sigma; St.Louis, Missouri, USA) with 20 strokes of a homogenizer, and centrifuged at 1,000 g for 10 min. The supernatants were then centrifuged at 50,000 g for 30 min, and the pellets were resuspended in a lysis buffer (1.5% n-octylglucoside) (Sigma), and sonicated 3 times at 15 sec intervals. After centrifugation at 100,000 g for 30 min, the supernatants were dialyzed (against PBS), filtered and used as MC [12]. T. vaginalis ESP was prepared by incubating 1×107/ml trichomonads in a 12-well plate at 37℃ for 90 min then centrifuging them at 10,000 g for 30 min. The supernatants were filtered and used as ESP [11].

Neutrophils were isolated from healthy donors by dextran sedimentation and Histopaque 1,077 density gradient fractionation, as previously described with minor modifications. Ten volumes of venous blood containing 5 U/ml heparin were well mixed with 2 volumes of 4.5% dextran T500 (Pharmacia, Uppsala, Sweden). After 30 min sedimentation at 37℃, the supernatant was overlayed on Ficoll-Histopaque 1077 and centrifuged at 385 g, at 4℃ for 30 min. After lysis of any erythrocytes in the sediment with sterile ice-cold distilled water, the isolated neutrophils were diluted in culture medium and kept on ice until use. Cell viability (>99%) was determined by the trypan blue exclusion method. To rule out monocyte contamination, cells were counted with a flow cytometer (BD Bioscience, San Jose, California, USA) after staining with fluorescein isothiocyanate (FITC)-conjugated anti-CD14 antibody (BD Bioscience), and neutrophils were found to make up more than 99.8% of the cells. Superoxide anion was measured on the basis of cytochrome c (Sigma) reduction [13]. A 100-µl of T. vaginalis lysate, ESP, or MC was added to each well of a 96-well plate followed by 100 µl of a solution containing cytochrome c (12 mg/ml) and neutrophils (4×104) in Hanks balanced salt solution (HBSS). After incubation at 37℃ in a 5% CO2 incubator for 30-180 min, the absorbance of each well was measured at 550 nm with a microplate autoreader (Thermomax; Molecular Devices, California, USA).

Superoxide anion generation was calculated using the extinction coefficient (38.16×103 M-1cm-1) of reduced cytochrome c at 550 nm, and is shown as nmoles of reduced cytochrome c per 1×105 neutrophils. To determine the role of trichomonad protease in superoxide anion generation, each trichomonad product (300 µl/ml of lysate, 200 µg/ml of MC, or 100 µl of ESP) was treated with protease inhibitor cocktail (PIC; Boehringer Mannheim/Roche, Mannheim, Germany) for 30 min at 37℃ before incubation with neutrophils. However, the effect of the generated superoxide anion on growth of T. vaginalis was investigated using neutrophil supernatants as follows: neutrophils (5×104) were incubated for 3 hr with T. vaginalis lysate (300 µg/ml) and the supernatant was collected. Trichomonads (5×105) were incubated with this supernatant for 3 hr, then transferred to TYM medium and incubated for 14 hr after which their numbers were counted by light microscopy, and compared with those of trichomonads incubated with control neutrophil supernatants.

For measurement of myeloperoxidase (MPO) release by neutrophils, neutrophil suspensions (1×107) were put into 6-well plates, then live T. vaginalis (1×106) was added at a ratio of 10:1 (=N:T). The final volumes were adjusted to 3 ml. Culture supernatant was collected after 1-24 hr incubation at 37℃ in a 5% CO2 incubator, and released MPO was determined using an ELISA kit (R&D systems, Minneapolis, Minnesota, USA).

For statistical analysis, results are expressed as the mean±SD of at least 3 independent experiments. The Student's t-test was used to determine the statistical significance. Significance was accepted at a P value of<0.05. The statistics program used was SPSS 12.0K (SPSS Inc., Chicago, Illinois, USA).

Superoxide anion generation by neutrophils was measured after incubation with the 3 trichomonad products for 3 hr. Superoxide anions were generated in response to T. vaginalis products in a dose- and time-dependent manner (Fig. 1). A marked increase of superoxide anion was observed after incubation with 300 µg/ml of T. vaginalis lysate or 200 µg/ml of MC (Fig. 1A, B). With ESP (100 µl), superoxide anion generation increased after 30 min incubation (6.0±0.24 nmole), and reached 7.8±0.56 nmole after 3 hr (Fig. 1C).

Fig. 1

Superoxide anion production by neutrophils activated by T. vaginalis. Superoxide anion was measured on the basis of cytochrome c reduction after T. vaginalis lysate (A), membrane component (B), or excretory-secretory product (C) pretreatment. Data are mean±SD values.

The role of the protease of T. vaginalis in generating superoxide anion production by neutrophils was determined by adding protease inhibitor (Fig. 2). Pretreatment with protease inhibitor cocktail (PIC) reduced superoxide anion generation in response to T. vaginalis lysate in a concentration-dependent manner, and similar results were obtained in the case of ESP and MC (Fig. 2). Although constituents of the 3 trichomonad products were expected to be different, superoxide anion generation by neutrophils after each trichomonad product treatment showed similar results (Figs. 1, 2). As shown in Fig. 3, growth of T. vaginalis was inhibited by preincubation with supernatants of neutrophils incubated for 3 hr with T. vaginalis lysate (see Methods part); pretreatment with supernatant reduced the number of trichomonads by 19.8% (P<0.05) at 14 hr of cultivation.

Fig. 2

Effects of protease inhibitor cocktail (PIC) on superoxide anion production by neutrophils activated with T. vaginalis lysate, T. vaginalis MC, and ESP for 3 hr. Data are mean±SD values. aP<0.05.

Fig. 3

Effects of superoxide anion on growth of T. vaginalis. Live T. vaginalis was incubated in neutrophil-trichomonads-coculture supernatant containing superoxide anion for 3 hr, then transferred to TYM medium and incubated for 14 hr. The number of trichomonads was counted with a hemocytometer. aP<0.05.

Myeloperoxidase release by neutrophils was determined by ELISA after stimulation with live T. vaginalis (Fig. 4). In this experiment, live T. vaginalis increased MPO after 1 hr of incubation (624±64 ng/ml), and secretion of MPO increased up to 9 hr (2,049±196 ng/ml).

Fig. 4

Myeloperoxidase production by neutrophils activated by T. vaginalis. Myeloperoxidase was determined by ELISA after coincubation of neutrophils and live T. vaginalis (N:T=10:1). Data are mean±SD values. aP<0.05.

Neutrophils are regarded as one of the key components of the innate immune response, and are involved in the first line of defense against invading pathogens, along with macrophages, eosinophils, and platelets. The microbicidal activities of neutrophils and macrophages are usually classified according to their oxygen dependence. The production of ROS and of reactive nitrogen species (RNS) are regarded as key processes in the oxygen-dependent microbicidal pathway. Reactive oxygen species are involved in various cellular activities, including stimulation of cell proliferation or cell death [14,15]. Examples of ROS include the superoxide anion (O2.-), hydroxyl radical (OH), hydrogen peroxide (H2O2) and hypochlorite anion (ClO-). Superoxide anion generation of neutrophils with some parasite infection, such as cysticercus cellulosae (=the metacestode of Taenia solium) and Plasmodium vivax, was previously reported [16,17]. Likewise, reactive nitrogen species, such as nitric oxide (NO), nitrogen dioxide (NO2), and nitrous acid (HNO2), play important roles in various physiological processes [18]. However, ROS and RNS also contribute to the oxygen-dependent antimicrobial activities of phagocytic cells. During phagocytosis, oxygen uptake into phagocytes, called the respiratory burst, is increased. After activation of NADPH oxidase in phagosomal membranes, O2 is reduced to the relatively stable intermediate, superoxide anion which can be bactericidal. Superoxide anion is the precursor of other powerful oxidants such as hydroxyl radicals [19]. The superoxide anion is related to RNS generation. For example, peroxynitrite (ONOO-), one of the RNS, is formed by a reaction between superoxide anion and nitric oxide [20]. Myeloperoxidase is released from intracellular granules of neutrophils and contributes to their microbicidal activity. The generation of various oxidants including hypochlorous acid (HOCl) and hypobromous acid (HOBr) by myeloperoxidase in the presence of superoxide anion is believed to contribute to the antimicrobial activities of neutrophils [21,22].

In a previous report, neutrophils were shown to kill T. vaginalis in aerobic conditions, and the addition of catalase or superoxide dismutase prevented this death [7]. This suggested that superoxide anion and hydrogen peroxide were important in killing of trichomonads by neutrophils. Moreover, the observation of reduced nitroblue tetrazolium (NBT) precipitates during co-incubation of neutrophils and trichomonads indirectly confirmed that superoxide anion was generated. In our present experiments, we directly measured superoxide anion generation by neutrophils stimulated by various products of trichomonads (Fig. 1). Our results were in good accord with previous reports done with other parasites [16,17]; however, further work is required to understand detailed stimulation mechanism of each trichomonad product and the role of superoxide anion in killing of trichomonads.

Chemorepulsion has been reported when trichomonads and an oxygen metabolite, such as hydrogen peroxide or hypochlorite, are placed on either side of polycarbonate membrane filters [23]. Migration of T. vaginalis into the filter was observed when neutrophils were placed alone on the opposite side of a filter. However, the addition of cell-free hydrogen peroxide or hypochlorite inhibited the movement of trichomonads across the filter due to chemorepulsion. Moreover, chemotaxis of neutrophils to trichomonad ESP has been reported [24]. These observations throw an interesting light on the relationship between host and parasite.

T. vaginalis protease has been shown by electrophoresis to be a typical cysteine protease [25]. The trichomonad protease is required for adhesion to epithelial cells, and for escape from the host immune system by degradation of human immunoglobulins [11,26]. We showed previously that T. vaginalis protease was involved in IL-8 production by neutrophils [27]. In the present work, the decreased superoxide anion production by neutrophils incubated with PIC-pretreated T. vaginalis indicates that the trichomonad protease is also involved in superoxide anion production (Fig. 2). In addition to PIC, iodoacetic acid (IAA), a cysteine protease inhibitor, and EDTA, a metalloprotease inhibitor, also decreased the production of superoxide anion (data not shown). Further research is needed to define the exact mechanism of action of the protease.

Myeloperoxidase is a heme enzyme found in the intracellular granules of neutrophils and primary lysosomes of monocytes. During the oxidative burst, MPO in activated neutrophils oxidizes chloride ions (Cl) with hydrogen peroxide (H2O2) as oxygen donor, and produces hypochlorous acid (HOCl), which phagocytic cells use to kill microbes [22,28]. Interestingly, genetically-modified MPO-deficient mice, whose neutrophils lack MPO activity have increased susceptibility to Candida albicans infection [29]. MPO-treated Entamoeba histolytica showed morphological alterations, leading to death [30]. It has been suggested that killing of Staphylococcus aureus by neutrophils is caused by myeloperoxidase-dependent production of superoxide anion [31]. Substantially more frequent severe infection has been noted in MPO-deficient human individuals [32]. In the present study, 3 different trichomonad preparations triggered the release of superoxide anion and MPO in neutrophils and these products are likely to be directly involved in killing of T. vaginalis.

In conclusion, the release of superoxide anion and MPO by neutrophils activated by trichomonads appears to be involved in defense mechanisms of human neutrophils against T. vaginalis.