Development of resistance to a trinuclear platinum complex in ovarian carcinoma cells

Paola Perego; Laura Gatti; Sabina C Righetti; Giovanni L Beretta; Nives Carenini; Elisabetta Corna; Laura Dal Bo; Stella Tinelli; Donato Colangelo; Roberto Leone; Piero Apostoli; Luciano Lombardi; Gino Beggiolin; Laura Piazzoni; Franco Zunino

doi:10.1002/ijc.11140

Development of resistance to a trinuclear platinum complex in ovarian carcinoma cells

Int J Cancer. 2003 Jul 10;105(5):617-24. doi: 10.1002/ijc.11140.

Authors

Paola Perego¹, Laura Gatti, Sabina C Righetti, Giovanni L Beretta, Nives Carenini, Elisabetta Corna, Laura Dal Bo, Stella Tinelli, Donato Colangelo, Roberto Leone, Piero Apostoli, Luciano Lombardi, Gino Beggiolin, Laura Piazzoni, Franco Zunino

Affiliation

¹ Istituto Nazionale Tumori, via Venezian 1, 20133 Milan, Italy. paola.perego@istitutotumori.mi.it

PMID: 12740909
DOI: 10.1002/ijc.11140

Abstract

BBR3464 is a trinuclear platinum complex that exhibits a potent cytotoxicity and efficacy against cisplatin-resistant tumors. To better understand the determinants of cellular resistance to BBR3464, we selected a resistant ovarian carcinoma cell line after exposure to the complex. The resistant cells (A2780/BBR3464) exhibited a high level of resistance to the selecting agent, but a marginal cross-resistance to cisplatin. Although cellular accumulation of BBR3464 was similar in parental and in resistant cells, DNA platination was decreased in A2780/BBR3464 cells, suggesting a reduced drug accessibility to DNA. This behavior reflected a partial drug inactivation at cytoplasmic level, as a consequence of increased levels of nucleophilic molecules including metallothioneins and human neurofilament low, but not glutathione. A2780/BBR3464 cells also exhibited a reduced susceptibility to apoptosis, which was consistent with reduced expression of Bax, and an alteration of DNA mismatch repair system, as reflected by lack of expression of MLH1 and PMS2, which could impair the recognition/repair of DNA lesions. Whereas both platinum drugs induced G2/M arrest in the parental cells, BBR3464, but not cisplatin, caused a late G1 arrest of resistant cells. Cisplatin induced an appreciable increase of p21(WAF1) levels in both models, in contrast to BBR3464 that produced a substantial upregulation of p21(WAF1) only in parental cells. An inverse relationship with p21(WAF1) modulation was found for CHK1 in parental cells treated with both agents and in resistant cells treated with cisplatin. This pattern of response is consistent with a regulatory loop involving p53 and p21(WAF1) at G2 checkpoint. In contrast, no modulation of CHK1 was found in A2780/BBR3464 treated with the triplatinum compound. These findings, indicating a different activation of regulatory pathways at DNA damage checkpoints in response to cisplatin and BBR3464, support an altered ability of resistant cells to recognize or tolerate sublethal lesions induced by BBR3464.

Publication types

Comparative Study
Research Support, Non-U.S. Gov't

MeSH terms

Antineoplastic Agents / pharmacology*
Apoptosis / drug effects
Base Pair Mismatch
Carmustine / pharmacology
Checkpoint Kinase 1
Cisplatin / pharmacology
Cyclin-Dependent Kinase Inhibitor p21
Cyclins / biosynthesis
DNA Adducts
DNA Damage
DNA Repair
DNA, Neoplasm / drug effects
Doxorubicin / pharmacology
Drug Resistance, Multiple
Drug Resistance, Neoplasm*
Female
G1 Phase / drug effects
Glutathione / metabolism
Humans
Melphalan / pharmacology
Metallothionein / biosynthesis
Organoplatinum Compounds / pharmacology*
Ovarian Neoplasms / pathology*
Paclitaxel / pharmacology
Protein Kinases / biosynthesis
Tumor Cells, Cultured / drug effects

Substances

Antineoplastic Agents
CDKN1A protein, human
Cyclin-Dependent Kinase Inhibitor p21
Cyclins
DNA Adducts
DNA, Neoplasm
Organoplatinum Compounds
Doxorubicin
Metallothionein
Protein Kinases
CHEK1 protein, human
Checkpoint Kinase 1
Glutathione
BBR 3464
Paclitaxel
Cisplatin
Melphalan
Carmustine