24664954[PMID] - PMC

Figure 5. From: Identification of dendritic cells, B cell and T cell subsets in Tasmanian devil lymphoid tissue; evidence for poor immune cell infiltration into devil facial tumors.

Immunohistochemical labeling with T cell subset markers in Tasmanian devil bronchus‐associated lymphoid tissue. (A) anti‐CD3, (B) anti‐CD4 (C), anti‐CD8 and (D) isotype control. Br, bronchus. Scale bar represents 100 μm.

Lauren J. Howson, et al. Anat Rec (Hoboken). 2014 Apr 22;297(5):925-938.

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Figure 9. From: Identification of dendritic cells, B cell and T cell subsets in Tasmanian devil lymphoid tissue; evidence for poor immune cell infiltration into devil facial tumors.

Immunohistochemical labeling with B cell subset markers in Tasmanian devil bronchus‐associated lymphoid tissue. (A) anti‐CD79b, (B) anti‐devil IgM, (C) anti‐devil IgG and (D) isotype control. Br, bronchus. Scale bar represents 100 μm.

Lauren J. Howson, et al. Anat Rec (Hoboken). 2014 Apr 22;297(5):925-938.

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Figure 10. From: Identification of dendritic cells, B cell and T cell subsets in Tasmanian devil lymphoid tissue; evidence for poor immune cell infiltration into devil facial tumors.

Immunohistochemical labeling with B cell subset markers in Tasmanian devil gut‐associated lymphoid tissue. (A) anti‐CD79b, (B) anti‐devil IgM, (C) anti‐devil IgG and (D) isotype control. Fl, follicle; Vi villus. Scale bar represents 100 μm.

Lauren J. Howson, et al. Anat Rec (Hoboken). 2014 Apr 22;297(5):925-938.

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Figure 12. From: Identification of dendritic cells, B cell and T cell subsets in Tasmanian devil lymphoid tissue; evidence for poor immune cell infiltration into devil facial tumors.

Immunohistochemical labeling with dendritic cell markers in Tasmanian devil spleen. (A) anti‐HLA‐DR (MHC class II), (B) anti‐CD1a, (C) anti‐CD83 and (D) isotype control. RP, red pulp; WP, white pulp. Scale bar represents 100 μm.

Lauren J. Howson, et al. Anat Rec (Hoboken). 2014 Apr 22;297(5):925-938.

Citation Full text

Figure 11. From: Identification of dendritic cells, B cell and T cell subsets in Tasmanian devil lymphoid tissue; evidence for poor immune cell infiltration into devil facial tumors.

Immunohistochemical labeling with dendritic cell markers in Tasmanian devil lymph node. (A) anti‐HLA‐DR (MHC class II), (B) anti‐CD1a (C) anti‐CD83 and (D) isotype control. Cx, cortex; Pcx, paracortex. Scale bar represents 100 μm.

Lauren J. Howson, et al. Anat Rec (Hoboken). 2014 Apr 22;297(5):925-938.

Citation Full text

Figure 6. From: Identification of dendritic cells, B cell and T cell subsets in Tasmanian devil lymphoid tissue; evidence for poor immune cell infiltration into devil facial tumors.

Immunohistochemical labeling with T cell subset markers in Tasmanian devil gut associated lymphoid tissue. (A) anti‐CD3, (B) anti‐CD4, (C) anti‐CD8 and (D) isotype control. Fl, follicle; Vi, villus. Scale bar represents 100 μm.

Lauren J. Howson, et al. Anat Rec (Hoboken). 2014 Apr 22;297(5):925-938.

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Figure 1. From: Identification of dendritic cells, B cell and T cell subsets in Tasmanian devil lymphoid tissue; evidence for poor immune cell infiltration into devil facial tumors.

Western blot of anti‐IgM, IgG, CD4 and CD8 antibodies against devil protein extracted from devil lymph node lymphocytes. Some non‐specific staining at high molecular weight occurred with antibodies to CD4 and CD8. Scale bar (molecular weight) at the right of panel is in kDa.

Lauren J. Howson, et al. Anat Rec (Hoboken). 2014 Apr 22;297(5):925-938.

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Figure 15. From: Identification of dendritic cells, B cell and T cell subsets in Tasmanian devil lymphoid tissue; evidence for poor immune cell infiltration into devil facial tumors.

Immunohistochemical labeling with dendritic cell markers in Tasmanian devil DFTD tumors. (A) anti‐periaxin (DFTD tumor cell marker), (B) anti‐HLA‐DR (MHC class II), (C) anti‐CD1a and (D) isotype control. S, stroma; T, tumor. Scale bar represents 100 μm.

Lauren J. Howson, et al. Anat Rec (Hoboken). 2014 Apr 22;297(5):925-938.

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Figure 14. From: Identification of dendritic cells, B cell and T cell subsets in Tasmanian devil lymphoid tissue; evidence for poor immune cell infiltration into devil facial tumors.

Immunohistochemical labeling with T cell markers in Tasmanian devil DFTD tumors. (A) anti‐periaxin (DFTD tumor cell marker), (B) anti‐CD3, (C) anti‐CD4 (no positive cells), (D) anti‐CD8. The isotype control is shown in figure 15. S, stroma; T, tumor. Scale bar represents 100 μm.

Lauren J. Howson, et al. Anat Rec (Hoboken). 2014 Apr 22;297(5):925-938.

Citation Full text

10.

Figure 18. From: Identification of dendritic cells, B cell and T cell subsets in Tasmanian devil lymphoid tissue; evidence for poor immune cell infiltration into devil facial tumors.

Immunohistochemical labeling with B cell markers in eastern quoll lymph node. (A) anti‐CD79b, (B) anti‐devil IgM and (C) anti‐devil IgG and (D) isotype control. Cross species reactivity is shown for all three antibodies. Cx, cortex; Fl, follicle. Scale bar represents 100 μm..

Lauren J. Howson, et al. Anat Rec (Hoboken). 2014 Apr 22;297(5):925-938.

Citation Full text

11.

Figure 2. From: Identification of dendritic cells, B cell and T cell subsets in Tasmanian devil lymphoid tissue; evidence for poor immune cell infiltration into devil facial tumors.

Immunohistochemical labeling with T cell subset markers in Tasmanian devil thymus. (A) anti‐CD3, (B) anti‐CD4 (C) anti‐CD8 and (D) isotype control. CD4⁺ T cells appear to be more prevalent than CD8⁺ T cells. Cx, cortex; M, medulla. Scale bar represents 100 μm.

Lauren J. Howson, et al. Anat Rec (Hoboken). 2014 Apr 22;297(5):925-938.

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12.

Figure 13. From: Identification of dendritic cells, B cell and T cell subsets in Tasmanian devil lymphoid tissue; evidence for poor immune cell infiltration into devil facial tumors.

Immunohistochemical labeling with dendritic cell markers in Tasmanian devil skin. (A) anti‐HLA‐DR (MHC class II), (B) anti‐CD1a (arrow indicates positive cell), (C) anti‐CD83 (no positive cells) and (D) isotype control. E, epidermis; D, dermis. Scale bar represents 100 μm.

Lauren J. Howson, et al. Anat Rec (Hoboken). 2014 Apr 22;297(5):925-938.

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13.

Figure 19. From: Identification of dendritic cells, B cell and T cell subsets in Tasmanian devil lymphoid tissue; evidence for poor immune cell infiltration into devil facial tumors.

Immunohistochemical labeling with B cell subset markers in brushtail possum lymph node. (A) anti‐CD79b, (B) anti‐devil IgM and (C) anti‐devil IgG and (D) isotype control. Cross species reactivity is shown for all three antibodies. Cx, cortex; Fl, follicle. Scale bar represents 100 μm.

Lauren J. Howson, et al. Anat Rec (Hoboken). 2014 Apr 22;297(5):925-938.

Citation Full text

14.

Figure 16. From: Identification of dendritic cells, B cell and T cell subsets in Tasmanian devil lymphoid tissue; evidence for poor immune cell infiltration into devil facial tumors.

Immunohistochemical labeling with T cell subset markers in eastern quoll lymph node. (A) anti‐CD3, (B) anti‐devil CD4, (C) anti‐devil CD8 and (D) isotype control. Cross species reactivity is shown for all three antibodies. Cx, cortex; Fl, follicle. Scale bar represents 100 μm.

Lauren J. Howson, et al. Anat Rec (Hoboken). 2014 Apr 22;297(5):925-938.

Citation Full text

15.

Figure 8. From: Identification of dendritic cells, B cell and T cell subsets in Tasmanian devil lymphoid tissue; evidence for poor immune cell infiltration into devil facial tumors.

Immunohistochemical labeling with B cell subset markers in Tasmanian devil spleen. (A) anti‐CD79b, (B) anti‐devil IgM, (C) anti‐devil IgG and (D) isotype control. B cells were predominantly identified in the white pulp. IgM⁺ cells appeared to be more prevalent than IgG⁺ cells. RP, red pulp; WP, white pulp. Scale bar represents 100 μm.

Lauren J. Howson, et al. Anat Rec (Hoboken). 2014 Apr 22;297(5):925-938.

Citation Full text

16.

Figure 17. From: Identification of dendritic cells, B cell and T cell subsets in Tasmanian devil lymphoid tissue; evidence for poor immune cell infiltration into devil facial tumors.

Immunohistochemical labeling with T cell subset markers in brushtail possum lymph node. (A) anti‐CD3, (B) anti‐devil CD4, (C) anti‐devil CD8 and (D) isotype control. Cross species reactivity is shown for all three antibodies. Cx, cortex; Fl, follicle. Scale bar represents 100 μm.

Lauren J. Howson, et al. Anat Rec (Hoboken). 2014 Apr 22;297(5):925-938.

Citation Full text

17.

Figure 7. From: Identification of dendritic cells, B cell and T cell subsets in Tasmanian devil lymphoid tissue; evidence for poor immune cell infiltration into devil facial tumors.

Immunohistochemical labeling with B cell subset markers in Tasmanian devil lymph node. (A) anti‐CD79b, (B) anti‐devil IgM, (C) anti‐devil IgG and (D) isotype control. B cells were predominantly identified in the follicles. IgM⁺ cells appeared to be more prevalent than IgG⁺ cells. Cx, cortex; Fl, follicle. Scale bar represents 100 μm.

Lauren J. Howson, et al. Anat Rec (Hoboken). 2014 Apr 22;297(5):925-938.

Citation Full text

18.

Figure 4. From: Identification of dendritic cells, B cell and T cell subsets in Tasmanian devil lymphoid tissue; evidence for poor immune cell infiltration into devil facial tumors.

Immunohistochemical labeling with T cell subset markers in Tasmanian devil spleen. (A) anti‐CD3, (B) anti‐CD4, (C) anti‐CD8 and (D) isotype control. T cells were predominantly identified in the white pulp. CD4⁺ T cells appeared to be more prevalent than CD8⁺ T cells. RP, red pulp; WP, white pulp. Scale bar represents 100 μm.

Lauren J. Howson, et al. Anat Rec (Hoboken). 2014 Apr 22;297(5):925-938.

Citation Full text

19.

Figure 3. From: Identification of dendritic cells, B cell and T cell subsets in Tasmanian devil lymphoid tissue; evidence for poor immune cell infiltration into devil facial tumors.

Immunohistochemical labeling with T cell subset markers in Tasmanian devil lymph node. (A) anti‐CD3, (B) anti‐CD4, (C) anti‐CD8 and (D) isotype control. T cells were predominantly identified in the cortex. CD4⁺ T cells appear to be more prevalent than CD8⁺ T cells. Cx, cortex; Fl, follicle. Scale bar represents 100 μm.

Lauren J. Howson, et al. Anat Rec (Hoboken). 2014 Apr 22;297(5):925-938.

Citation Full text

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