Comparison of the blood-brain barrier and liver penetration of acridine antitumor drugs |
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| Authors: | Eain M. Cornford Deborah Young James W. Paxton |
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| Affiliation: | (1) Southwestern Regional V. A. Epilepsy Center, Research and Neurology Services, Veterans Administration West Los Angeles Medical Center, 90073 Los Angeles, CA, USA;(2) Department of Neurology, Brain Research Institute, UCLA School of Medicine, 90024 Los Angeles, CA, USA;(3) Department of Pharmacology and Clinical Pharmacology, Auckland University School of Medicine, Auckland, New Zealand |
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| Abstract: | ![]()
Summary The blood-brain barrier penetration of amsacrine and its analogs 9-({2-methoxy-4-[(methylsulfonyl)-amino]phenyl}amino)-,5-dimethyl-4-acridine carboxamide (CI-921) and M-[2-(dimethylamino)ethyl]-acridine-4-carboxamide (AC) was measured in the barbiturate-anesthetized mouse. After intracarotid administration, AC was almost completery extracted (90%) in a single transit through the brain capillaries, whereas CI-921 (20%) and amsacrine (15%) were moderately extracted. AC is retained in the brain; no loss of AC from the brain was apparent at 1, 2, 4, or 8 min after injection. In contrast, after intraportal administration, 75% of the AC, 94% of the CI-921, and 57% of the amsacrine was extracted in a single transit through the hepatic vasculature. Rather than being retained in the mouse liver, these acridine antitumor agents show time-dependent loss (t1/2=10 min for amsacrine and AC, 24 min for CI-921). We conclude that unlike most antitumor agents, these acridine drugs appear to penetrate the blood-brain barrier readily.This study was supported by the Auckland Medical Research Foundation (New Zealand), by the Medical Research Foundation (New Zealand), by the National Science Foundation (United States/New Zealand Cooperative Science Program), by the United States Veterans Administration, and by NIH grant NS 25554 |
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