In vivo biological activity of the components of haematoporphyrin derivative

Berenbaum, M. C.; Bonnett, Raymond; Scourides, Panayiotis A.

doi:10.1038/bjc.1982.94

Cited by 167 publications

(64 citation statements)

References 12 publications

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“…The model (Patterson et al, 1990) was derived from the observation of a sharp boundary that usually occurs between PDT-induced tissue necrosis and undamaged adjacent tissue (Berenbaum et al, 1982;Potter, 1989). The model states that, for a given tissue and photosensitiser combination, necrosis will occur if the number of photons absorbed by the photosensitiser per unit tissue volume exceeds a threshold value (1).…”

mentioning

confidence: 99%

The sensitivity of normal brain and intracranially implanted VX2 tumour to interstitial photodynamic therapy

Lilge

Olivo²,

Schatz³

et al. 1996

Br J Cancer

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mentioning

confidence: 99%

The sensitivity of normal brain and intracranially implanted VX2 tumour to interstitial photodynamic therapy

Lilge

Olivo²,

Schatz³

et al. 1996

Br J Cancer

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“…after alkali treatment, see Materials and methods) contains at least 4 defined porphyrins (haematoporphyrin (Hp), two isomers of monohydroxy-monovinyldeuteroporphyrin (HvD) and protoporphyrin (PP)) (Bonnett et al, 1980;Moan & Sommer 1981). In addition to these compounds, a certain amount of unknown material is found, somewhat dependent on the method used to separate the components (Moan et al, , 1982aBerenbaum et al, 1982;Dougherty et al, 1983). A large fraction of these unknown components are aggregates, some of which may be composed of porphyrins bound strongly together with, for instance, covalent bonds (Moan et al, 1982a, Berenbaum et al, 1982.…”

Section: Discussionmentioning

confidence: 99%

“…In addition to these compounds, a certain amount of unknown material is found, somewhat dependent on the method used to separate the components (Moan et al, , 1982aBerenbaum et al, 1982;Dougherty et al, 1983). A large fraction of these unknown components are aggregates, some of which may be composed of porphyrins bound strongly together with, for instance, covalent bonds (Moan et al, 1982a, Berenbaum et al, 1982. This conclusion is supported by the present findings that the 360-370nm absorption, characteristic of aggregated porphyrins, is still present at low concentration and in a variety of solvents.…”

Section: Discussionmentioning

confidence: 99%

Retention and photodynamic effects of haematoporphyrin derivative in cells after prolonged cultivation in the presence of porphyrin

Christensen¹,

Sandquist²,

Feren³

et al. 1983

Br J Cancer

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“…The more hydrophilic porphyrin species of HpD, such as the isomers of haematoporphyrin and hydroxyethylvinyldeuteroporphyrin, were probably present in sufficient levels in the cytosol soon after injection such that exposure to light caused oxidative damage to cytosolic proteins. On the other hand, Photofrin II, a mixture of porphyrins enriched in the hydrophobic species (80-90% as reported by Dougherty (1987)), presumably dihaematoporphyrin ethers and/or esters (Berenbaum et al, 1982;Byrne et al, 1987;Dougherty, 1987;Kessel et al, 1987), would be expected to accumulate primarily in the more hydrophobic regions, such as cell membranes. If this were the case, the lower concentration of hydrophilic components (20%) in Photofrin II would be less able to produce sufficient 102 in the cytosol to cause inhibition of pyruvate kinase, the result we observed.…”

Section: Enzyme Activity Analysismentioning

confidence: 96%

In vitro photosensitization of tumour cell enzymes by Photofrin II administered in vivo

Murant²,

Chazen³

et al. 1989

Br J Cancer

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Dougherty, 1979). After 24-72h, to allow clearance of the photosensitiser from normal tissues, the malignant lesions are exposed to visible light, usually by laser irradiation. Tumour necrosis and regression ensue from photoradiation. It is generally agreed that cytotoxicity is mediated via formation of the highly reactive oxygen species, singlet oxygen, 102, (Weishaupt et al., 1976;Gibson et al., 1984;Parker, 1987). Since the original promising clinical results utilised HpD, a crude preparation composed of at least seven different porphyrin species (Gibson et al., 1984; Kessel, 1986;Moan et al., 1987), subsequent investigations were directed towards determination of the chemical structure of the 'active component' of HpD (Moan et al., 1982;Kessel and Chou, 1983;Dougherty et al., 1984). Methods developed to purify HpD produced a porphyrin mixture enriched in the hydrophobic components, reported to be mainly dihaematoporphyrin ethers or esters (Byrne et al., 1987;Dougherty, 1987;Kessel et al., 1987). This enriched preparation, Photofrin II, is now commercially produced for clinical and laboratory studies.In our earlier studies we utilised HpD as the photosensitiser (Hilf et al., , 1984Gibson et al., 1984). Because of the complex nature of HpD, the intracellular localisation and effects of various photosensitising components relative to time after administration could differ from the pharmacokinetics that would be observed with Photofrin II. We therefore undertook a study of Photofrin II employing the same in vivo-in vitro protocol used previously for HpD (Hilf et al., 1984). In this protocol, the photosensitiser is injected into tumour-bearing animals, tumours are removed and subcellular organelles are prepared. These preparations are then exposed to visible light in vitro, and various biochemical endpoints are analysed, such as site-specific enzyme activities. One advantage of this protocol is that it takes into account any metabolism of the sensitiser by the tumour-bearing host. In this report, using Photofrin II as the photosensitiser, data are presented on the time-course and drug dose response of photosensitisation of selected mitochondrial and cytosolic enzymes in the R3230AC mammary carcinoma. Materials and methods MaterialsPhotofrin II was kindly provided by Photomedica Inc., Raritan, NJ. All other reagents were obtained from Sigma Chemical Co., St Louis, MO, unless otherwise noted. Animals and tumoursThe R3230AC mammary adenocarcinoma was maintained by subcutaneous transplantation in the axillary region of 60-80g female Fischer rats, using the sterile trochar procedure described previously (Hilf et al., 1965).Preparation of subcellular organelles from tumours For in vitro studies, tumour-bearing rats were killed 17-24 days after implantation of the R3230AC mammary adenocarcinoma. From excised tumours, mitochondria were prepared according to methods described earlier . Briefly, R3230AC tumours were removed, weighed, placed in a dish on ice in 0.9% NaCl solution and minced with scissors. Approximately 2g...

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In vivo biological activity of the components of haematoporphyrin derivative

Cited by 167 publications

References 12 publications

The sensitivity of normal brain and intracranially implanted VX2 tumour to interstitial photodynamic therapy

The sensitivity of normal brain and intracranially implanted VX2 tumour to interstitial photodynamic therapy

Retention and photodynamic effects of haematoporphyrin derivative in cells after prolonged cultivation in the presence of porphyrin

In vitro photosensitization of tumour cell enzymes by Photofrin II administered in vivo

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