Figure 6
Figure 6. Immunohistochemical analysis and EM of tumors. Serial sections of representative tumors (n = 8) of Th1 cell–treated and control mice from day 18. (A) Tumors were stained with monoclonal anti-CD4 antibody (i,ii) showing a strong increase in CD4+ cells in tumors of Th1 cell–treated mice. indicates CD4+ cells. Staining with H&E (iii,iv) showed no major differences in the morphology of the tumors. Necrosis (N) was detected in tumors of Th1 cell–treated and PBS-treated mice. Ki-67 staining (v,vi) showed no obvious differences in the proliferation rate of the tumors. indicates Ki-67–positive cells. Pictures, ×100 magnification. Inlays, ×200 original magnification. (B) Quantitative analysis of (Av,vi). Ki-67+ cells of 500 total cells in tumor sections (n = 60) of Th1 cell–treated and PBS-treated mice were counted. Error bars denote SEM. (C) Tumors were stained with monoclonal anti–PECAM-1 antibody (i-iv) showing homogenous vascularization in both groups. However, minor changes in vessel morphology (white arrows) and a minor decrease of tumor vessel density were detectable in tumors of Th1 cell–treated mice (ii,iv) compared with control mice (i,iii). Staining of tumors with monoclonal anti–VEGFR-2 antibody (v,vi) revealed no obvious change in the receptor expression pattern between both groups. Pictures, ×200 original magnification. (D) EM of blood vessels. (i) Blood vessels with a bulged EC body (E), tight junctions (), and the basal lamina (labeled with *). (ii) Blood lacuna without limiting ECs, but with extracellular matrix–like collagen fibrils (*) that are located between tumor cells and blood cells. (iii) Blood vessel with leukocyte transendothelial migration. (iv) Higher magnification of panel iii, showing a transcellularly transmigrated leukocyte (L) still covered by a basal lamina (). (v) Obliterated vessel. The left arrow labels a tight junction; the right arrow, the rest of the lumen. (vi) Vessels in adjacent muscle of Th1 cell–treated tumors appear normal. In summary, blood vessels of PBS-treated (i,ii) tumors were seen as normal tumor vessels. In contrast, degenerated ECs were observed more frequently in tumors of Th1 cell–treated mice (iii-v). In addition, strong inflammatory processes (iii,iv) and more obliterated vessels (v) were seen in tumors of Th1 cell–treated mice. Experiments were performed as described in “Methods.”

Immunohistochemical analysis and EM of tumors. Serial sections of representative tumors (n = 8) of Th1 cell–treated and control mice from day 18. (A) Tumors were stained with monoclonal anti-CD4 antibody (i,ii) showing a strong increase in CD4+ cells in tumors of Th1 cell–treated mice. indicates CD4+ cells. Staining with H&E (iii,iv) showed no major differences in the morphology of the tumors. Necrosis (N) was detected in tumors of Th1 cell–treated and PBS-treated mice. Ki-67 staining (v,vi) showed no obvious differences in the proliferation rate of the tumors. indicates Ki-67–positive cells. Pictures, ×100 magnification. Inlays, ×200 original magnification. (B) Quantitative analysis of (Av,vi). Ki-67+ cells of 500 total cells in tumor sections (n = 60) of Th1 cell–treated and PBS-treated mice were counted. Error bars denote SEM. (C) Tumors were stained with monoclonal anti–PECAM-1 antibody (i-iv) showing homogenous vascularization in both groups. However, minor changes in vessel morphology (white arrows) and a minor decrease of tumor vessel density were detectable in tumors of Th1 cell–treated mice (ii,iv) compared with control mice (i,iii). Staining of tumors with monoclonal anti–VEGFR-2 antibody (v,vi) revealed no obvious change in the receptor expression pattern between both groups. Pictures, ×200 original magnification. (D) EM of blood vessels. (i) Blood vessels with a bulged EC body (E), tight junctions (), and the basal lamina (labeled with *). (ii) Blood lacuna without limiting ECs, but with extracellular matrix–like collagen fibrils (*) that are located between tumor cells and blood cells. (iii) Blood vessel with leukocyte transendothelial migration. (iv) Higher magnification of panel iii, showing a transcellularly transmigrated leukocyte (L) still covered by a basal lamina (). (v) Obliterated vessel. The left arrow labels a tight junction; the right arrow, the rest of the lumen. (vi) Vessels in adjacent muscle of Th1 cell–treated tumors appear normal. In summary, blood vessels of PBS-treated (i,ii) tumors were seen as normal tumor vessels. In contrast, degenerated ECs were observed more frequently in tumors of Th1 cell–treated mice (iii-v). In addition, strong inflammatory processes (iii,iv) and more obliterated vessels (v) were seen in tumors of Th1 cell–treated mice. Experiments were performed as described in “Methods.”

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