Figure 1
Figure 1. Immunological features of the patient. (A) Lymphocytes subpopulations. Serum immunoglobulin levels. (B) Liver histopathology. Immunohistochemistry was performed on fixed tissues with a peroxidase-based method (Dako). Antibodies used were raised against CD20, CD3, CD8, CD4 and granzyme B (Dako). EBV-encoded RNA (EBER) was probed on some specimen with the use of in situ hybridization technique. Slides were observed using a Leica DM LB microscope with ×20, ×40, and ×100 objectives and a 10× eyepiece. Aquisition of images was with IM50 software (Leica Microsystems). First line: CD8+ lymphocytic infiltrates in lobular (left) and portal (middle) area. Negative EBER staining (right). Second line: positive granzyme B staining in lobular and portal area (left and right panels, respectively). These infiltration could result of the trapping of the activated CD8+ T cells in liver during the immune response.10 (C) Immunoscope quantitative T-cell repertoire analysis. Most significant specific T-cell clonal expansion is shown. The x-axis indicates CDR3 length (in amino acid), and the y-axis displays the fluorescence intensity of the run-off products (in arbitrary units). Percentages indicate the frequency of occurrence for each Vβ family. (D) CD8+ maternal engrafted T cells express IFN-γ in response to EBV latent antigen LMP-2A antigen. Freshly isolated mononuclear cells of the patient and his mother were incubated without stimulation (NS) or in the presence of latent antigen LMP-2A, latent antigen EBNA-1, and lytic antigen BZLF-2, then stained for the expression of IFN-γ, CD3 and CD8. Numbers are the percentage of cells in the lymphoid gate expressing the indicated surface markers.

Immunological features of the patient. (A) Lymphocytes subpopulations. Serum immunoglobulin levels. (B) Liver histopathology. Immunohistochemistry was performed on fixed tissues with a peroxidase-based method (Dako). Antibodies used were raised against CD20, CD3, CD8, CD4 and granzyme B (Dako). EBV-encoded RNA (EBER) was probed on some specimen with the use of in situ hybridization technique. Slides were observed using a Leica DM LB microscope with ×20, ×40, and ×100 objectives and a 10× eyepiece. Aquisition of images was with IM50 software (Leica Microsystems). First line: CD8+ lymphocytic infiltrates in lobular (left) and portal (middle) area. Negative EBER staining (right). Second line: positive granzyme B staining in lobular and portal area (left and right panels, respectively). These infiltration could result of the trapping of the activated CD8+ T cells in liver during the immune response.10  (C) Immunoscope quantitative T-cell repertoire analysis. Most significant specific T-cell clonal expansion is shown. The x-axis indicates CDR3 length (in amino acid), and the y-axis displays the fluorescence intensity of the run-off products (in arbitrary units). Percentages indicate the frequency of occurrence for each Vβ family. (D) CD8+ maternal engrafted T cells express IFN-γ in response to EBV latent antigen LMP-2A antigen. Freshly isolated mononuclear cells of the patient and his mother were incubated without stimulation (NS) or in the presence of latent antigen LMP-2A, latent antigen EBNA-1, and lytic antigen BZLF-2, then stained for the expression of IFN-γ, CD3 and CD8. Numbers are the percentage of cells in the lymphoid gate expressing the indicated surface markers.

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