Nucleic Acids Research, Vol 26, Issue 17 3933-3939, Copyright © 1998 by Oxford University Press
J Whittaker, WD McFadyen, G Wickham, LP Wakelin and V Murray
Cisplatin analogues were synthesised that consisted of platinum(II) diamine
complexes tethered via a polymethylene chain ( n = 3, 5, 8 and 10) to a
phenanthridinium cation. Both chloro and iodo leaving groups were examined.
DNA adduct formation was quantitatively analysed using a linear
amplification system with the plasmid pGEM-3Zf(+). This system utilised Taq
DNA polymerase to extend from an oligonucleotide primer to the damage site.
This damage site inhibited the extension of the DNA polymerase. The
products were electrophoresed on a DNA sequencing gel enabling adduct
formation to be determined at base pair resolution. The damage intensity at
each site was determined by densitometry. The platinum phenanthridinium
complexes were shown to damage DNA at shorter incubation times than
cisplatin. To produce similar levels of damage, an 18 h incubation was
required for cisplatin compared to 30 min for the n = 3 platinum
phenanthridinium complexes; this indicates that the intercalating
chromophore causes a large increase in the rate of platination. A reaction
mechanism involving direct displacement of the chloride by the N-7 of
guanine may account for the rate increase. These results indicate that
further development of these compounds could lead to more effective cancer
chemotherapeutic agents.
ARTICLES
The interaction of DNA-targeted platinum phenanthridinium complexes with DNA
School of Biochemistry and Molecular Genetics and School of Chemistry, University of New South Wales, Sydney, NSW 2052, Australia.
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