THE EFFECT OF DIFFERENTIATION ON PHOTOSENSITIZER UPTAKE BY HL60 CELLS

The capability of human promyelocytic leukemia cells HL60 to be induced to differentiate to various stages along the monocytic or myelocytic pathway was exploited for investigation of the uptake of selected photo-sensitizers by diverse types of cells of the same origin. The results showed that there was no substantial difference in photofrin uptake between noninduced HL60 cells, immature monocytes, immature neutrophils and cells differentiated along the eosinophilic pathway. In contrast, HL60 cells differentiated into macrophages (HL609) exhibited markedly increased photofrin uptake, which was further enhanced by their pretreatment with bacterial lipopolysaccharide. Similar results were obtained with other photosensitizers tested: di-and tetrasulfonated aluminum phthalocyanines (AIPcS₂ and AIPcS₄), tetrasulfonated zinc phthalocyanine (ZnPcS₄), tetraphenylporphine tetrasulfonate (TPPS₄) and benzoporphyrin derivative monoacid (BPD). Despite marked differences in the state of self-aggregation and other chemical properties of these compounds, the degree of their preferential uptake by HL60 PH cells showed very little variation. In a typical experiment, the uptake of these photosensitizers by HL60 PH cells was four to five times higher than the uptake by noninduced HL60 cells. In addition to the fluorometric assay employed in most of the experiments, cellular concentration of AlPcS₄ was determined by measurement of elementary aluminum using atomic absorption spectroscopy.     

PHOTOFRIN ACCUMULATION IN MALIGNANT AND HOST CELL POPULATIONS OF A MURINE FIBROSARCOMA

Abstract— Photofrin (25 mg/kg) was administered to the FsaR fibrosarcoma-bearing mice (either syngeneic or severe combined immunodeficient [SOD]) and the tumors were excised 24 h later. The photosensitizer content in the cells dissociated from tumor tissue was analyzed using flow cytometry. Staining the cell suspensions with the monoclonal antibodies against specific membrane markers served to identify the malignant cells and various types of host immune cells infiltrating the tumor. Photofrin content was also examined in the cells from normal tissues of the tumor-bearing mice (spleen, heart muscle, peritoneal macrophages). The results show a marked heterogeneity in the Photofrin cellular content of FsaR tumor, particularly within the population of tumor-associated macrophages (TAM). The Photofrin levels in some TAM were lower or similar to those in the malignant cells. In contrast, a subpopulation of TAM accumulated very high levels of the photosensitizer, which exceeded by far the levels found in the other tumor cell populations. This TAM fraction was characterized by particularly high expression of interleukin-2 receptors and increased cell size and granularity when compared to the other TAM, which suggests that these macrophages are in the activated state. Their average Photofrin content was almost 13 times higher than in the malignant cells. The lowest photosensitizer levels in the tumor were found in tumor-infiltrating leukocytes other than TAM. In FsaR tumors growing in SCID mice, the pattern of Photofrin distribution in TAM and other cellular populations was similar to that found in tumors growing in syngeneic mice. Due to a presumably better perfusion, these tumors accumulated higher levels of Photofrin in all cellular populations. The findings of this study suggest that the tumor-localizing effect of Photofrin can be attributed to the accumulation of extremely high levels of the photosensitizer in a subpopulation of TAM.     

ENHANCED MACROPHAGE CYTOTOXICITY AGAINST TUMOR CELLS TREATED WITH PHOTODYNAMIC THERAPY

Abstract— Sulfamethoxazole (SMX) in its nonionized form in aqueous solution has ultraviolet (UV) absorption that is maximal at 268 nm but extends through the ultraviolet-B (UVB) region. It was found to be extremely susceptible to photodegradation when exposed to artificial UV radiation through a Pyrex filter or to unfiltered natural sunlight. The SMX anion was more stable. The quantum yields of the photodegradation of both forms were determined by use of monochromatic light and ferrioxalate chemical actinometry, the values of 0.47 (pH 3.0) and 0.084 (pH 9.0) at the maximum absorption wavelengths (268 and 257 nm, respectively) being obtained. Using literature data on sunlight intensity, the photochemical shelf-life of SMX solutions exposed to direct sunlight was calculated for Sydney (latitude 33.5°S) as a function of season of the year and verified experimentally. A fixed correlation was established between the rate constant for SMX degradation and UVB intensity measured by a radiometer, suggesting the capacity of this chemical system to monitor changes in the UVB region of sunlight.