Thermosensitive liposomes: Extravasation and release of contents in tumor microvascular networks
Purpose: The purpose of this study was to determine whether hyperthermic exposure would accelerate drug release from thermosensitive sterically stabilized liposomes and enhance their extravasation in tumor tissues. Materials and Methods: In vivo fluorescence video microscopy was used to measure the...
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Veröffentlicht in: | International journal of radiation oncology, biology, physics biology, physics, 1996-12, Vol.36 (5), p.1177-1187 |
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Zusammenfassung: | Purpose: The purpose of this study was to determine whether hyperthermic exposure would accelerate drug release from thermosensitive sterically stabilized liposomes and enhance their extravasation in tumor tissues.
Materials and Methods: In vivo fluorescence video microscopy was used to measure the extravasation of liposomes, as well as release of their contents, in a rat skin flap window chamber containing a vascularized mammary adenocarcinoma under defined thermal conditions (34°, 42°, and 45°C). Images of tissue areas containing multiple blood vessels were recorded via a SIT camera immediately before, and for upto 2 h after i.v. injection of two liposome populations with identical lipid composition: one liposome preparation was surface labeled with Rhodamine-PE (Rh-PE) and the other contained either Doxorubicin (Dox) or calcein at self-quenching concentrations. The light intensity of the entire tissue area was measured at 34°C (the physiological temperature of the skin) for 1 h, and at 42° or 45°C for a second hour. These measurements were then used to calculate the fluorescent light intensity arising from each tracer (liposome surface label and the released contents) inside the vessel and in the interstitial region.
Results: The calculated intensity of Rh-PE for the thermosensitive liposomes in the interstitial space (which represents the amout of extravasated liposomes) was low during the first hour, while temperature was maintained at 34°C and increased to 47 times its level before heating, when the tumor was heated at 42° or 45° C for 1 h. The calculated intensity of the liposome contents (Dox) in the interstitial space was negligible at 34°C, and increased by 38- and 76-fold, when the tumor was heated at 42° and 45° C for 1 h, respectively. Similar values were obtained when calcein was encapsulated in liposomes instead of Dox. A similar increase in liposome extravasation was seen with nonthermosensitive liposomes, but negligible release of Dox occurred when the window chamber was heated to 45°C for 1 h. Extravasation of liposomes continued after heating was stopped, but content release stopped after removal of heat. Release of Dox from extravasated liposomes was also seen if heating was applied 24 h after liposome administration, but no further enhancement of liposome extravasation occurred in this case.
Conclusions: Our data suggest that hyperthermia can be used to selectively enhance both the delivery and the rate of release of drugs from thermos |
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ISSN: | 0360-3016 1879-355X |
DOI: | 10.1016/S0360-3016(96)00389-6 |