Figure 1. Colocalization of hypoxia and macrophages. Colocalization in human squamous carcinoma of the uterine cervix (A-D) and human PC3 (prostate carcinoma) xenografted tumors grown in nude mice (E-F). (A) Hypoxic areas (arrow), visualized by immunolabeling of the reductively activated hypoxic-specific marker pimonidazole (red), are observed at a distance from the disorganized blood vessels (BV). (B) In some areas of these tumors, CD68+ TAMs (brown) accumulate in stromal (S) rather than tumor (T) areas. (C-D) Colocalization of TAMS (brown) and hypoxia (red) showing TAM accumulation in avascular, perinecrotic, necrotic (N), and hypoxia areas. (E-F) Serial sections showing F4/80-positive (brown; panel F) TAMs in hypoxic, perinecrotic areas (red; panel E) of PC3 tumors. N indicates necrosis; and T, tumor. The microscope used was a Leitz Orthoplan. Magnification of panel A, × 100; panel B, × 400; panel C, × 160; panel D, × 160; panel E, × 160; panel F, × 160 (panels D-F, cropped images). Slight adjustments were made in brightness and contrast on each whole image. The temperature was room temperature. The imaging medium was DPX. Chromogens used were DAB (brown) 3,3-diaminobenzene and vector red (red) (Vector Laboratories, Burlingame, CA). The camera was a Fuji HC 3002 digital camera. Image processing was performed by Photograb 3002 (Windows platform).
Figure 1.

Colocalization of hypoxia and macrophages. Colocalization in human squamous carcinoma of the uterine cervix (A-D) and human PC3 (prostate carcinoma) xenografted tumors grown in nude mice (E-F). (A) Hypoxic areas (arrow), visualized by immunolabeling of the reductively activated hypoxic-specific marker pimonidazole (red), are observed at a distance from the disorganized blood vessels (BV). (B) In some areas of these tumors, CD68+ TAMs (brown) accumulate in stromal (S) rather than tumor (T) areas. (C-D) Colocalization of TAMS (brown) and hypoxia (red) showing TAM accumulation in avascular, perinecrotic, necrotic (N), and hypoxia areas. (E-F) Serial sections showing F4/80-positive (brown; panel F) TAMs in hypoxic, perinecrotic areas (red; panel E) of PC3 tumors. N indicates necrosis; and T, tumor. The microscope used was a Leitz Orthoplan. Magnification of panel A, × 100; panel B, × 400; panel C, × 160; panel D, × 160; panel E, × 160; panel F, × 160 (panels D-F, cropped images). Slight adjustments were made in brightness and contrast on each whole image. The temperature was room temperature. The imaging medium was DPX. Chromogens used were DAB (brown) 3,3-diaminobenzene and vector red (red) (Vector Laboratories, Burlingame, CA). The camera was a Fuji HC 3002 digital camera. Image processing was performed by Photograb 3002 (Windows platform).

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