Abstract:
:The reaction of the antitumor agent leinamycin with thiols converts this natural product into an episulfonium ion that alkylates the N7-position of guanine residues in double-stranded DNA. It is reported here that depurination of this adduct is unusually facile, occurring with a half-life of about 3.5 h at pH 7 and 37 degrees C in duplex DNA. This is one of the most rapid depurination reactions ever observed for an N7-alkylguanine residue. The rate constant for the depurination reaction was measured at several temperatures, and the activation parameters were calculated from the data. The energy of activation (E(a)) for this reaction is 24.6 kcal/mol, and the Arrhenius A value is 1.2 x 10(13) s(-1). These values correspond to a DeltaH(++) = 24.0 kcal/mol and DeltaS(++) = -0.78 eu and are consistent with the expected unimolecular (D(N) + A(N)) mechanism for the depurination reaction. Changes in ionic strength (0-500 mM NaCl) or pH (3-8) do not significantly alter the rate of depurination, and the base excision repair protein Aag, which removes a variety of N7-alkylguanine residues from duplex DNA, does not excise the leinamycin-guanine adduct. Possible biological implications of this rapid depurination process are considered. Finally, during the course of these studies, the release of hydrolyzed leinamycin (4; Scheme 1) from leinamycin-modified DNA was observed. This result suggests that leinamycin may be a reversible DNA alkylating agent.
journal_name
Chem Res Toxicoljournal_title
Chemical research in toxicologyauthors
Nooner T,Dutta S,Gates KSdoi
10.1021/tx049964ksubject
Has Abstractpub_date
2004-07-01 00:00:00pages
942-9issue
7eissn
0893-228Xissn
1520-5010journal_volume
17pub_type
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