"Estudos espectroscópicos e citotóxicos do Photogem® fotodegradado e dos fotoprodutos formados pela irradiação com laser" / "Spectroscopics and cytotoxics studies of Photogem® photodegradate and of photoproducts formated by irradiation with laser"

AUTOR(ES)
DATA DE PUBLICAÇÃO

2006

RESUMO

Photodynamic therapy (PDT) is a technique for inducing tumor tissue damage following administration of a drug that can be selectively retained in malignant tissue and produce singlet oxygen when irradiated in adequate wavelengths in the presence of molecular oxygen. Photosensitizers of porphyrin type can be degraded by light (photobleaching), modifying the concentration ratio of the photosensitizer (PS) in the tumor vs. normal tissue. This process, usually called photobleaching, is characterized by a decrease in the absorption and fluorescence intensities. It has been shown that, during photobleaching, the formation of redshifted absorbing photoproducts takes place. In this study the PS used was Photogem®, a hematoporphyrin derivative produced in Russia and being used in PDT in Brazil. The sensitizer photobleaching and photoproduct formation was monitored by fluorescence and absorption properties changes as well as by the photoproducts formation evidenced by the appearance of a new absorption band around 640nm in PBS and in 660nm in Triton X-100 and Brij-35 solution. Photogem® photobleaching and photoproducts formation was induced by laser and LED irradiation in different concentrations, irradiation wavelengths (351, 488, 514 and 630nm), in different time intervals and intensities of irradiation. The cytotoxicity of Photogem® and its photoproducts in tumor (HEp-2) and non-tumor (VERO) cell lines were analyzed in the dark and in the light. Experiments in animals were performed in order to access the depth of necrosis caused by Photogem® and its photoproducts in rat liver tissue. The results suggest that the photoproducts of Photogem® are less cytotoxic than Photogem® either in the dark or in the light, and the cytotoxicity decreases with the previous irradiation time of Photogem®. The photoproducts of Photogem® obtained at 514nm need one-hour irradiation for both cell lines to have the same cytotoxicity of Photogem® irradiated for 14min in tumor cells and 25min in non-tumor cells. The results suggest that different processes occurs in the PS degradation when in different environments (PBS, surfactants and solvents), in different concentrations and irradiation conditions (wavelength, potency, time). In PDT, the sensitizers are typically present in high concentrations in tumor cells. At the same time, the degradation of photosensitizers in properly elevate rates during the illumination in PDT, can lead to a decrease in the concentrations of these photosensitizers in normal tissue, decreasing the photosensibility and phototoxicity (skin), while adequate amount of photosensitizer can be maintained in tumor cells for photodestruction, resulting in a small damage for normal tissue. Photodegradation of photosensitizers is the fundamental connection of photodynamic dose distribution in the biological fluids, being related with the kinetic of photosensitizer elimination in the organism. For the data obtained in vivo for depth of necrosis of Photogem® x vii and its photoproducts obtained by degradation in 514nm and in 630nm, it was observed that in the irradiation dose of 150J/cm2 in both concentrations (1,5 and 2mg/Kg ), the depth of necrosis is greater for Photogem® followed by Photogem® previously degradated in 514 and then in 630nm. In the dose of 200J/cm2 and in the concentration 2,0mg/kg, there is no differences in the depth of necrosis for non-irradiated Photogem® as well as for its photoproducts, what can be correlated with the phototoxicity of the photoproducts, that in high concentrations and elevate irradiation doses, present a greater photodynamic activity. These results obtained in vivo are in agreement with the ones in vitro, since in the cytotoxic experiments the photoproducts are less cytotoxic than non irradiated Photogem® presenting in the animals a small depth of necrosis. These findings may be helpful for establishment of dosimetry for Photogem® in Photodynamic Therapy

ASSUNTO(S)

photogem porfirinas porphyrins photodynamic therapy terapia fotodinâmica photogem

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