Enhanced Egress of Intracellular Eimeria tenella Sporozoites by Splenic Lymphocytes from Coccidian-Infected Chickens

Animals.Outbred, specific-pathogen-free White Leghorn chickens from a local hatchery (Beijing Meiliyaweitong Experimental Animal Technology Co., Ltd., Beijing, China) and broiler chickens from Longenecker's Hatchery (Ross/Ross, Elizabethtown, PA) were used. All animals were housed under Eimeria-free conditions, with food and water provided ad libitum. All experiments were performed following Institutional Animal Care and Use Committee guidelines.

Parasites.Oocysts of E. tenella strains BJ and Beltsville WLR-1 were propagated, isolated, and sporulated as described previously (24). Sporozoites were purified using DE-52 anion-exchange chromatography (32).

Preparation of chicken cells for E. tenella infection.Primary chicken kidney (PCK) cells were prepared as previously described (27), with modifications. Kidneys were aseptically removed from 7- to 14-day-old chickens, placed in Ca²⁺- and Mg²⁺-free Hanks' balanced salt solution (CMF-HBSS) containing 100 U/ml penicillin and 100 μg/ml streptomycin, and cut into small pieces. Kidney pieces were incubated with 0.25% trypsin (Sigma, St. Louis, MO) for 5 min at 37°C, trypsin was inactivated by addition of Iscove's modified Dulbecco's medium (IMDM; Invitrogen, Carlsbad, CA) containing 20% fetal calf serum (FCS; HyClone, Thermo Scientific, Logan, UT), and the cells in the supernatant were collected by centrifugation. This process was repeated 3 times, and the PCK cells were pooled and resuspended in IMDM containing 10% FCS. Chicken peripheral blood mononuclear cells (PBMCs) were prepared as previously described (18). Whole blood was collected aseptically by venipuncture of the wing vein and was diluted 1:1 with CMF-HBSS at 4°C. PBMCs were isolated by density gradient centrifugation using Polymorphprep (Fresenius Kabi, Oslo, Norway). After being washed with CMF-HBSS, the cells were resuspended in IMDM containing 10% fetal bovine serum (FBS), 1× nonessential amino acids, 100 U/ml penicillin, and 100 μg/ml streptomycin. Cell viability, determined by trypan blue exclusion, was consistently >90%.

Preparation of chicken spleen lymphocytes.Three-week-old chickens were randomly divided into two groups. Chickens in group I were orally inoculated with 200 μl of phosphate-buffered saline (PBS) as uninfected controls. Chickens in group II were kept in a separate room and were orally inoculated with 200 μl of PBS containing 1.0 × 10⁴ E. tenella sporulated oocysts. One week after primary infection, chickens in group I were still given PBS and chickens in group II were given a secondary oral infection with 1.0 × 10⁵ E. tenella sporulated oocysts in PBS. Splenic lymphocytes from uninfected and infected animals were isolated as previously described (7), with modifications. Spleens were obtained aseptically at 7 days post-secondary infection, and single-cell suspensions were prepared by passage through a wire mesh in IMDM containing 5% FBS, 10 mM HEPES, 100 U/ml penicillin, and 100 μg/ml streptomycin. The cells were passed through a nylon wool column to remove clumps and debris, and splenic lymphocytes were enriched by density gradient centrifugation through Polymorphprep as described above. Purified lymphocytes were resuspended in IMDM containing 10% FBS, 1× nonessential amino acids, 100 U/ml penicillin, and 100 μg/ml streptomycin. Cell viability, determined by trypan blue exclusion, was consistently >90%.

Egress assay.PCK cells and PBMCs were seeded in 24-well plates containing glass slides (2.0 × 10⁷ cells/well) and cultured overnight at 41°C, and nonadherent cells were removed by washing with CMF-HBSS. Two to 3 days later, the cells were incubated overnight at 41°C with E. tenella strain BJ (for PCK cells) or strain WLR-1 (for PBMCs) sporozoites at a multiplicity of infection of 1.0 (parasite/cell ratio of 1:1). Free parasites were removed by washing with CMF-HBSS at 41°C. Following sporozoite infection, the cells were left untreated or were cocultured with splenic lymphocytes from uninfected or E. tenella-infected animals for 1, 3, or 5 h at 41°C, using splenocyte:PCK cell or splenocyte:PBMC ratios of 25:1, 50:1, and 100:1. In some experiments, sporozoite-infected PBMCs were cocultured with spleen cells in Transwell membrane inserts (8-μm pore size; Corning, Lowell, MA) to assess the role of cell-cell contact in parasite egression. Following coculture incubation, the splenocytes were removed by washing with CMF-HBSS, and the infected cells were fixed with methanol for 10 min at 4°C and permeabilized with 0.05% Triton X-100 in PBS for 10 min at 4°C. The cells were incubated with mouse anti-Eimeria antibodies for 30 min at 4°C, washed, and incubated with Alexa Fluor 488-conjugated goat anti-mouse IgG secondary antibody (Invitrogen) in 0.1 μg/ml of Evan's blue for 30 min at 4°C. Intracellular parasites were counted in 30 randomly selected fields by use of a fluorescence microscope (Carl Zeiss, Thornwood, NY, or Olympus). The percentage of parasite egress was calculated using the following formula: % egress = [(N₁ − N₂)/N₁] × 100, where N₁ is the number of intracellular parasites in cells cocultured with splenocytes from primed or naive chickens and N₂ is the number of intracellular parasites in cells cocultured with IMDM. Each experiment was repeated 3 times.

Determination of sporozoite viability and infectivity.E. tenella sporozoite-infected PCK cells were cocultured with splenocytes in Transwell membrane inserts. After 5 h of incubation, cell culture medium which contained egressed E. tenella sporozoites was collected, and the viability of egressed sporozoites was determined using trypan blue dye exclusion. To evaluate the infectivity of egressed sporozoites, they were added to the monolayer of PCK cells overnight. The freshly prepared E. tenella sporozoites were used as a control. Free parasites were removed by washing with CMF-HBSS at 41°C, and the intracellular parasites were quantified by counting a minimum of 10 fields per well (×40 objective; Olympus IX71 microscope). Infection rates were calculated by dividing the number of intracellular parasites by the total number of inoculated parasites.

Host cell viability evaluation.After overnight incubation of the PCK cells with sporozoites, PCK cells were washed and cocultured with E. tenella-primed or naive splenocytes at a lymphocyte-to-PCK-cell ratio of 100:1 for 3 h at 41°C in a 5% CO₂ incubator. At each time point, PCK cells were washed and viability was assessed using an annexin V-fluorescein isothiocyanate (annexin V-FITC) apoptosis detection kit (Nanjing Keygen Biotechnology Co. Ltd., China). Briefly, the adherent PCK cells were washed in cold PBS, gently trypsinized, and washed again twice in PBS, and single cells were resuspended in 500 μl binding buffer. Next, 2 μl of annexin V-FITC and 5 μl of propidium iodide (PI) were added and incubated at room temperature for 15 min in the dark. The dead cells were visualized by fluorescence microscopy (Olympus IX71) with appropriate filters. Viability of host cells after parasite egression was calculated according to the following formula: % viability = (% egress − % death)/% egress, where % death means the total number of dead host cells divided by the total number of host cells.

Magnetic bead cell subpopulation depletion.Spleen lymphocyte subpopulations were depleted using a commercial cell separation system (BD IMag cell separation system; BD Biosciences, San Jose, CA). Splenocytes were incubated with mouse monoclonal antibodies detecting chicken B cells or CD4⁺ or CD8⁺ T cells (21) in CMF-HBSS containing 3% heat-inactivated FCS and 0.01% sodium azide (staining buffer) for 30 min at 4°C. The cells were washed with staining buffer and incubated with biotinylated goat anti-mouse IgG antibody for 30 min at 4°C. The cells were washed, resuspended in BD IMag buffer containing a pretitrated volume of streptavidin-labeled magnetic particles, and exposed to a magnetic field to remove the labeled cells, and the cells remaining in the supernatant were cocultured with sporozoite-infected cells for the egress assay. The efficiency of each depleted cell population was verified by flow cytometry. The cell depletion efficiency was routinely >95%, with >90% cell viability.

Effects of Eimeria antibody or chicken cytokines on parasite egress.Sporozoite-infected PBMCs were preincubated with recombinant chicken cytokines (interleukin-2 [IL-2], IL-15, and gamma interferon [IFN-γ]) or with recombinant swine IL-13 or chicken anti-Eimeria IgY antibody or nonimmune IgY as a negative control for 5 h at 41°C, the cells were washed, and egress was calculated as described above. Cytokines were produced in COS-7 cells as previously described (22, 34). Anti-Eimeria IgY and nonimmune IgY antibodies were prepared from egg yolks of specific-pathogen-free hens hyperimmunized and not immunized, respectively, with live oocysts of E. tenella, E. acervulina, and E. maxima as described previously (16, 17). Antibody concentrations were determined using the Bradford reagent (Sigma), with bovine serum albumin as the standard.

Effect of PLC inhibition or parasite motility on egress.U-73122 (phospholipase C [PLC] inhibitor; Sigma) and cytochalasin D (motility inhibitor; Sigma) were used to investigate the roles of PLC and actin-dependent parasite motility on sporozoite egress. Stock solutions of 1.0 mM U-73122 and cytochalasin D were prepared in dimethyl sulfoxide (DMSO; Sigma). E. tenella sporozoite-infected host cells were pretreated for 1 h at 41°C with DMSO vehicle alone or with 2.0 or 10 μM drug in IMDM. The cells were washed with IMDM and cocultured with splenocyte suspensions (100:1) or incubated with IgY antibody (200 μg/ml) for 3 h at 41°C, and egress was calculated as described above.

Statistical analysis.Each sample was analyzed in triplicate. Statistical analyses were performed using GraphPad Prism 4 or SPSS software (SPSS 15.0 for Windows; SPSS, Chicago, IL), and all data are expressed as means with standard errors of the means (SEM). Comparisons of the mean values were performed by Student's t test, and differences between means were considered statistically significant for P values of <0.05.