Exogenous Interleukin-12 Protects against Lethal Infection with Coxsackievirus B4

Viral replication in the pancreatic tissues of untreated and IL-12-treated mice. Pancreata harvested from CVB4-V-infected, IL-12-treated mice (○) and from infected, untreated mice (•) were assayed for viral infectivity by plaque assay. Organs from four mice were analyzed at each time point. Mean values and standard deviations are shown.

Histopathology of pancreatic tissues from CVB4-V-infected mice treated with either IL-12 or IFN-γ. Pancreata were harvested at 14 days postinfection, processed for routine histology, and stained with hematoxylin and eosin. (A) Uninfected; (B) CVB4-V-infected; (C) CVB4-V-infected and treated with 500 ng of IL-12; (D) CVB4-V-infected and treated with 100 ng of IFN-γ on multiple days (0.5, 1, and 2) after infection. Labeling: A, acini; I, islet of Langerhans; L, lymphocytic infiltrate; AN, acinar cell necrosis. Magnifications: ×234 for panels A, B, and C; ×117 for panel D.

IFN-γ production in CVB4-V-infected mice treated with IL-12. Organs and sera were collected from groups (n = 3) of IL-12-treated (○) or untreated (•) mice at various times after infection and assayed for IFN-γ by ELISA. Uninfected mice (▪) were included as controls. (A) Serum; (B) spleen; (C) pancreas; (D) heart. Each datum point represents the result for one mouse. The mean value for each group is shown. Statistically significant differences (P < 0.05) between IL-12-treated and untreated mice are denoted by asterisks.

Administration of IL-12 increases IFN-γ production by NK and NKT cells. Intracellular IFN-γ staining of splenocytes from IL-12-treated and CVB4-V-infected, CVB4-V-infected, and uninfected mice. (A) Representative histograms of IFN-γ staining (thick lines) NK cells and background staining (thin lines). Each panel represents data from one mouse. (B) Summary of IFN-γ staining NK cells, NKT cells, and T cells from CVB4-V-infected, IL-12-treated mice, CVB4-V-infected mice, and uninfected mice (n = 6 for each group). Theresults are expressed as the percentage of each cell population staining for IFN-γ minus the background staining. Mean values and standard deviations are shown. Statistically significant differences (P < 0.01) between IL-12-treated and untreated mice are denoted by asterisks.

Cytokine treatment of CVB4-V-infected mice. (A) Administration of IL-12 to CVB4-V-infected GKO mice was not protective. Each group contained seven mice. Curves: dashed line, 500 ng of IL-12; solid line, vehicle alone. (B) Administration of IFN-γ to CVB4-V-infected, BALB/c mice was protective. Each group contained four to six mice. IFN-γ treatment significantly (P < 0.05) increased survival of CVB4-V-infected mice. Curves: dotted line, 50 ng of IFN-γ; dashed line, 100 ng of IFN-γ; solid line, vehicle alone.