The mechanisms of chemoresistance in ovarian cancer patients remain largely to be elucidated. Paclitaxel/cisplatin combination is the standard chemotherapeutic treatment for this disease, although some patients do not respond to therapy. Our goals were to investigate whether TUBB mutations and mismatch repair defects underlie paclitaxel and cisplatin resistance.
Methods
Thirty-four patients with primary ovarian carcinomas (26 serous and eight clear cell carcinomas) treated with paclitaxel/cisplatin were analysed. TUBB exon 4 was analysed by nested PCR after a first round PCR using intronic primers. Microsatellite analysis was performed with the quasimonomorphic markers BAT 26 and BAT 34.
Results
Twenty-two of the 34 ovarian cancers (64.7%) presented residual tumour after surgery, seven of which (7/22; 31.8%) were shown to be chemoresistant (five serous and two clear cell tumours). Sequence analysis did not find any mutation in TUBB exon 4. Microsatellite instability was not detected in any of the ovarian carcinomas.
Conclusion
We conclude that TUBB exon 4 mutations and mismatch repair defects do not play a significant role in paclitaxel/cisplatin resistance.
The online version of this article (doi:10.1186/1471-2407-5-101) contains supplementary material, which is available to authorized users.
Competing interests
The author(s) declare that they have no competing interests.
Authors' contributions
BM carried out the molecular genetic studies and drafted the manuscript. IV participated in the design of the study and coordination. DP was responsible for clinical surveillance. AS was responsible for paraffin slides. IMP was responsible for the histopathologic analysis. CP carried out sequence alignment. MT coordinated the study. SC conceived the study and participated in its design and coordination.
Background
Ovarian cancer is the fourth most common cancer in women [1]. The standard treatment for ovarian cancer is cytoreductive surgery followed by combination systemic chemotherapy [2]. Since the middle 90's, the combination paclitaxel/cisplatin became the standard chemotherapeutic treatment for poor prognosis ovarian cancer [3]. Nevertheless, some patients are resistant to this chemotherapeutic treatment, making it important to clarify the underlying mechanisms of resistance [4].
Paclitaxel binds to microtubules and causes kinetic suppression (stabilisation) of microtubule dynamics, promoting their polymerisation and cell cycle arrest in mitosis (antimitotic activity), which probably leads to apoptosis [5, 6]. Microtubules are composed of a dimeric protein, tubulin, with alpha (α) and beta (β) tubulin heterodimers in dynamic equilibrium. The β-tubulin gene (TUBB), mapped to 6p21.3 [7], is composed of four exons and encodes a 445-aminoacid protein with GTPase function to which paclitaxel preferentially binds [8]. Cisplatin is activated intracellularly and establishes inter- and intra-strand DNA adducts that block replication and translation. The fate of cells after cisplatin exposure depends both on the extent of DNA damage and the cellular response to it, and apoptosis can be induced as a consequence [5, 9]. Although the specific mechanism that triggers apoptosis is not totally clear, some evidence suggests that this process can be mediated by the DNA mismatch repair system (MMR) [5, 9].
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Drug resistance is considered a multifactorial process, but the detailed mechanisms are still unknown. Recently, point mutations in the β-tubulin gene, predominantly in exon 4, were associated with resistance to paclitaxel [10‐12]. Resistance to cisplatin was linked with anomalies in the DNA MMR system resulting in microsatellite instability (MSI) [13‐16]. In order to evaluate the relevance of these mechanisms to ovarian cancer chemoresistance, we screened TUBB exon 4 for mutations and performed MSI analysis in 34 ovarian carcinomas treated with paclitaxel/cisplatin and evaluated patients' response to chemotherapy.
Methods
Patient data
Thirty-four primary ovarian carcinoma patients, of serous (26 cases) or clear cell (eight cases) histological types (invasive or borderline), consecutively admitted at the Portuguese Oncology Institute – Porto and treated with the adjuvant chemotherapy scheme paclitaxel/cisplatin, were analysed. Patients previously treated with other chemotherapeutic regimens or radiotherapy were excluded from the study.
Evaluation of treatment responses was done by an oncologist using computerized tomography or magnetic resonance and CA125 quantification, according to international guidelines [17]. Investigators performing laboratory analysis were not aware of chemotherapy response or resistance until the study was completed.
DNA extraction
Genomic DNA was extracted from chemo-naïve, paraffin embedded tumours, after dissection. Tissue blocks were sectioned, mounted on glass slides, deparaffinised, and stained with haematoxylin and eosin. Tumour areas were identified under the microscope on each slide and marked. Areas with at least 70% of cancer cells were identified on tissue sections. Selected paraffin blocks were sectioned (5μm sections) and mounted in microscope slides. Marked tumour areas were selected with a sterile razor blade. Three sections of tissue were incubated in a solution of 10 mM Tris-HCl buffer (pH 8.0), 2.5 mM MgCl2, 50 mM KCl, 0.5% (p/v) Tween 20, and 1 mg/mL proteinase K for 48 hours at 55°C.
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TUBBexon 4 sequencing
For polymerase chain reaction (PCR) assays, different sets of oligonucleotides were designed to amplify specific regions of TUBB exon 4 that code for the GTP and paclitaxel binding sites. To assure that the amplicon was not a pseudogene, the following intronic primer set was used in the first round PCR: 5'AAG-GAG-ATA-CAT-CCG-AGG-GAA-TT3' and 5'AAG-GTA-TTC-ATG-ATG-CGA3'. After checking for first round PCR product in an agarose gel, a 1:10 dilution was used for nested PCRs with the following primers: set 1, 5'AGA-GAG-CTG-TGA-CTG-CCT-G3' and 5'AAG-GTA-TTC-ATG-ATG-CGA3'; set 2, 5'GCT-CTG-GAA-TGG-GCA-CTC3' and 5'CCG-TAG-GTT-GGT-TGT-GGT-CA3'; set 3, 5'CGG-GGA-TCT-GAA-CCA-CCT-T3' and 5'GAG-TGT-CAC-GGC-CTG-GAG-T3'. The PCR products were separated by electrophoresis in agarose gels stained with ethidium bromide and analysed in a transiluminator. All DNA samples were analysed in an automatic DNA sequencer ABI PRISM 310™ Genetic Analyser. The sequences were compared with the genomic sequence GenBank AF070600.
MSI evaluation
For microsatellite analysis, tumour DNA was amplified with primers for two quasimonomorphic markers BAT 26 (5'GAG-TGT-CAC-GGC-CTG-GAG-T3'; 5'AAC-CAT-TCA-ACA-TTT-TTA-ACC-C3') and BAT 34 (5'ACC-CTG-GAG-GAT-TTC-ATC-TC3'; 5'AAC-AAA-GCG-AGA-CCC-AGT-CT3') [18‐20]. Fragments were analysed in an ABI PRISM 310™ Genetic Analyser.
Results
Twenty-two of the 34 ovarian cancers (64.7%) presented residual tumour after surgery, seven of which (7/22; 31.8%) were shown to be chemoresistant (five serous and two clear cell tumours) (Table 1).
Table 1
Clinical, pathological and genetic data of 34 ovarian cancer patients.
Patient
Histological type
Stage
Grade
Residual tumour
Treatment response
Exon 4 TUBB mutation
MSI status
1
Serous
III
1
> 2 cm
CR
Not present
Stable
2
Serous
III
2
< 2 cm
CR
Not present
Stable
3
Serous
III
3
> 2 cm
CR
Not present
Stable
4
Serous
III
1
> 2 cm
WR
Not present
Stable
5
Serous
III
2
> 2 cm
CR
Not present
Stable
6
Serous
III
2
< 2 cm
CR
Not present
Stable
7
Serous
III
3
> 2 cm
CR
Not present
Stable
8
Serous
III
3
> 2 cm
CR
Not present
Stable
9
Serous
III
3
> 2 cm
CR
Not present
Stable
10
Serous
III
3
> 2 cm
CR
Not present
Stable
11
Serous
III
3
> 2 cm
CR
Not present
Stable
12
Serous
III
3
> 2 cm
WR
Not present
Stable
13
Serous
III
3
> 2 cm
WR
Not present
Stable
14
Serous
IV
3
> 2 cm
PR
Not present
Stable
15
Serous
IV
3
> 2 cm
CR
Not present
Stable
16
Serous
IV
3
> 2 cm
WR
Not present
Stable
17
Serous
IV
3
> 2 cm
WR
Not present
Stable
18
Serous
IV
3
< 2 cm
CR
Not present
Stable
19
Serous
I
1
Absent
-
Not present
Stable
20
Serous
II
3
Absent
-
Not present
Stable
21
Serous
III
1
Absent
-
Not present
Stable
22
Serous
III
3
Absent
-
Not present
Stable
23
Serous
III
1
Absent
-
Not present
Stable
24
Serous
II
B
Absent
-
Not present
Stable
25
Serous
II
B
Absent
-
Not present
Stable
26
Serous
III
B
Absent
-
Not present
Stable
27
Clear cell
I
3
< 2 cm
CR
Not present
Stable
28
Clear cell
II
3
> 2 cm
WR
Not present
Stable
29
Clear cell
III
3
> 2 cm
PR
Not present
Stable
30
Clear cell
IV
3
> 2 cm
WR
Not present
Stable
31
Clear cell
I
3
Absent
-
Not present
Stable
32
Clear cell
I
3
Absent
-
Not present
Stable
33
Clear cell
II
3
Absent
-
Not present
Stable
34
Clear cell
III
3
Absent
-
Not present
Stable
B: borderline tumours; CR: complete response; PR: partial response; WR: without response. The stage classification was according to the Federation Internationale de Gynecologie [21] and grading was defined as well differentiated (1), moderately differentiated (2), and poorly differentiated (3).
Amplicons of 700 bp were observed for all cases after amplification with the intronic primers (data not shown). Nested PCR with primer sets 1–3 specific for TUBB exon 4 resulted in amplicons with 129, 254, and 201 bp, respectively (Figure 1). Sequencing analysis of all 34 cases showed no TUBB exon 4 mutations (Figure 2).
×
×
Microsatellite analysis with markers BAT 26 and BAT 34 (Figure 3) showed the normal pattern in all cases, so no evidence for microsatellite instability was detected in this series.
×
Discussion
Tumour resistance to chemotherapy or disease relapses resistant to further treatment after an initial response are common events in current cytotoxic cancer treatment regimens [5]. With regard to ovarian cancer chemotherapy, the current major challenge is to understand why histologically similar tumours behave so differently when treated with the same chemotherapeutic regimen. The action of a drug potentially depends on several mechanisms, namely, metabolisation, access into the tumour microenvironment, intracellular uptake, interaction with the target, and subsequent signalling events [5]. It is therefore important to study the different molecular mechanisms that can be involved in chemotherapy resistance.
The rationale for studying the relationship between TUBB gene mutations with paclitaxel resistance came from the studies of Giannakakou et al and Gonzalez-Garay et al [10, 11], who found TUBB mutations in ovarian cancer cell lines and in hamster cells, respectively. Subsequently, Monzó et al [12] reported TUBB mutations in 16 out of 36 (44.4%) paclitaxel resistant tumour samples from patients with advanced non-small cell lung cancer and proposed that TUBB mutations could represent a possible mechanism of paclitaxel resistance in that tumour type.
However, our findings in the present study argue against a significant role of TUBB gene mutations in paclitaxel resistance in ovarian cancer. In keeping with our results, Sale et al [22] and Lamendola et al [23] did not detect TUBB gene mutations in ovarian cancer samples. Similar findings have recently been obtained for several other tumour types, namely, lung [24], breast [25, 26], and gastric cancer [27]. Taken together, our and several other investigations concur that TUBB exon 4 mutations are not an important mechanism underlying paclitaxel resistance. To explain the early findings of Monzó et al [12], which were not reproduced by other authors, including the present study, Kelley et al [24] suggested that the primers used by Monzó et al [12] did not allow to discriminate TUBB from its pseudogenes [24]. Furthermore, the first studies reporting TUBB gene mutations were made in hamster cells [11] and in ovarian cancer cell lines [10] after selection by paclitaxel exposure, something that makes difficult a direct extrapolation of these findings to human tumours.
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We have also evaluated the MSI status of the 34 ovarian carcinomas with quasimonomorphic BAT 26 and BAT 34 markers, but did not find any microsatellite unstable tumours. Some authors have described an association between cisplatin resistance and MMR system anomalies in ovarian adenocarcinomas [28‐30], as well as in colon cancer cell lines [31‐33]. Additionally, other studies found MSI in ovarian cancer, namely, in serous and clear cell histological types [34‐40]. However, the frequency of MSI identified in those studies was quite low (0–14.3%), which is in agreement with our findings. To completely rule out any relationship between deficient mismatch repair and cisplatin resistance, one would have to analyse more microsatellite markers in a larger series of tumours paired with normal DNA.
Conclusion
We conclude that, contrarily to earlier suggestions, TUBB exon 4 mutations and MMR defects are not major mechanisms underlying paclitaxel and/or cisplatin resistance in ovarian cancer. Further investigation on alternative mechanisms of resistance to these drugs is warranted. Possible mechanisms to paclitaxel resistance are P-glycoprotein overexpression [5, 41], differential β-tubulin isotype expression [5, 42, 43], and apoptosis deregulation [5, 44‐46]. Decrease in intracellular cisplatin level, increase of tolerance or repair of DNA lesions, and alterations in the apoptotic cascade have also been related with cisplatin resistance [5, 47]. These studies are necessary to predict individual response of patients to these chemotherapeutic agents.
Acknowledgements
We thank the Portuguese Health Ministry for the financial support (Project nr. 191/99). B. Mesquita was a fellow of Fundação para Ciência e Tecnologia. We thank Mariano Monzó and collaborators for useful discussions during this work.
Open Access
This article is published under license to BioMed Central Ltd. This is an Open Access article is distributed under the terms of the Creative Commons Attribution License (
https://creativecommons.org/licenses/by/2.0
), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
Competing interests
The author(s) declare that they have no competing interests.
Authors' contributions
BM carried out the molecular genetic studies and drafted the manuscript. IV participated in the design of the study and coordination. DP was responsible for clinical surveillance. AS was responsible for paraffin slides. IMP was responsible for the histopathologic analysis. CP carried out sequence alignment. MT coordinated the study. SC conceived the study and participated in its design and coordination.
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