Assessment of DDR2, BRAF, EGFR and KRAS mutations as therapeutic targets in non-adenocarcinoma lung cancer patients
- Authors:
- Published online on: June 3, 2014 https://doi.org/10.3892/mco.2014.302
- Pages: 714-718
Abstract
Introduction
Lung cancer is the leading cause of cancer-related mortality worldwide, accounting for 1.37 million deaths in 2008 (1). Lung cancer is generally treated with surgical resection, chemotherapy, radiation therapy, or combined modality approaches with curative intent. Among these treatments, chemotherapy is the only applicable and recommended treatment for patients with metastatic or relapsed lung cancer. However the clinical efficacy of conventional cytotoxic chemotherapy is insufficient, with a response rate (RR) of 20–40% (2–4). Recently, ~80% of non-smoker Asian adenocarcinoma lung cancer (AdLC) patients were found to have at least one genetic abnormality in the epidermal growth factor receptor (EGFR), v-Ki-ras2 Kirsten rat sarcoma viral oncogene homolog (KRAS), echinoderm microtubule-associated protein-like 4-anaplastic lymphoma kinase (EML4-ALK), or human EGFR-related 2 genes (5). Treatment targeting the aberrant proteins encoded by these genes has been the focus of treatment for AdLC, which accounts for 45% of lung cancer cases. In particular, patients harboring an EGFR mutation and an EML4-ALK fusion respond remarkably to the EGFR tyrosine kinase inhibitors (TKIs) erlotinib (RR, 70–83%) or gefitinib (RR, 62–73%) and the ALK inhibitor crizotinib (RR, 57%), respectively (6). Thus, drugs targeting these aberrant proteins have significantly improved the treatment outcome for lung cancer patients. Similarly, an EGFR mutation is frequently encountered among patients with adenosquamous carcinoma (ASC) (7) and Iwanaga et al (8) reported a case with ASC harboring an EGFR mutation that responded significantly to EGFR-TKI treatment. Conversely, in patients with pulmonary squamous cell carcinoma (SCC), which accounts for 35% of lung cancer cases, mutations in the EGFR or KRAS genes are extremely rare (9,10). Marchetti et al (9) could not find any mutations in the area encoding the tyrosine kinase domain of EGFR in 454 SCC patients. Thus, in the treatment of SCC, molecular-targeted therapy is not considered to be a suitable approach and chemotherapy is limited to the use of conventional cytotoxic antineoplastic drugs. Similarly, in other histological subtypes, such as ASC, large-cell carcinoma (LCC), large-cell neuroendocrine carcinoma (LCNEC) and small-cell lung carcinoma (SCLC), the use of molecular-targeted drugs is not recommended, as only a limited number of patients harbor targetable mutations (11).
Recently, the concomitant administration of dasatinib (a Src family protein TKI) and erlotinib reportedly achieved a partial response in SCC patients (12). Additionally, patients who achieve partial remission with dasatinib reportedly harbor mutations in the gene encoding discoidin domain receptor 2 (DDR2) (13), a transmembrane receptor activated by binding to extracellular collagen. In tumor cells, DDRs interrupt normal cell-matrix communication and initiate pro-migratory and pro-invasive cascades (14). Hammerman et al (13) recently reported that the proliferation of SCC cell lines harboring DDR2 mutations was inhibited by dasatinib in an in vitro study and that tumors established from DDR2 mutant cell lines were highly responsive to dasatinib in a xenograft model study. Those studies indicated the possibility of dasatinib as a highly effective drug for SCC patients harboring DDR2 mutations. In a study on European and North American subjects, the frequency of mutations in DDR2 was reported to be 3.2% in SCC (13), 0.5% in AdLC (15) and 17% in LCC (16), with no mutations identified in SCLC and LCNEC patients. In addition, DDR2 mutations were more often encountered in smokers compared to non-smokers (17). Those studies indicated that DDR2 may be a target molecule for the treatment of non-AdLC, at least in European and North American subjects. However, ethnic differences in the frequency of DDR2 mutations were not adequately assessed, despite the presence of considerable ethnic genetic variation, such as EGFR in AdLC, which has an exceptionally high prevalence in East Asian populations (30–60%) and a low occurrence in European and North American populations (10–20%) (18–21). Thus, to select an appropriate therapeutic strategy, accurate data on the frequencies of genetic mutations in non-AdLC (including SCC) patients of different ethnic groups are required. In a recent study, Sasaki et al (22) failed to identify a DDR2 mutation in 166 Japanese SCC patients; however, the authors only focused on mutations in the exons encoding the receptor or transmembrane region. The available data on the frequency of DDR2 mutations are not considered sufficient to support the possible use of DDR2 mutations as a therapeutic target for SCC patients, due to the lack of data in the region encoding the kinase domain, which is considered to directly affect the clinical efficacy of dasatinib. Thus, in the present study, we investigated the frequency of mutations in DDR2 exons 5, 8 and 12–17; v-raf murine sarcoma viral oncogene homolog B1 (BRAF) V600E; EGFR exons 19 and 21; and KRAS codons 12 and 13 in Japanese non-AdLC patients to assess their potential use as therapeutic biomarkers in the Japanese population.
Materials and methods
Patients and samples
We enrolled a total of 150 patients who had undergone surgery for non-AdLC at the Gunma University Hospital (Maebashi, Gunma, Japan) between December, 2003 and December, 2012, including 87 SCC and 2 ASC patients who were previously reported by Miyamae et al (23). This study was approved by the Institutional Review Board for Clinical Trials at the Gunma University Hospital and the Ethics Committee for Human Genome Analysis of the Gunma University. Written consent was obtained from all the participants after they had been informed of the experimental procedure and the purpose of this study. The resected tumor samples were immediately frozen and stored at −80°C until DNA extraction. All the tumor tissue samples were diagnosed as non-AdLC and the pathological subtype was determined by hematoxylin and eosin staining. For the cases of poorly differentiated and histologically atypical SCC or LCC and cases harboring KRAS or EGFR mutations, additional immunostaining for p63 and thyroid transcription factor 1 was performed to confirm the specific histological subtype. The cases diagnosed as SCLC or LCNEC were confirmed to exhibit neuroendocrinological differentiation by 3 types of staining for neural cell adhesion molecule, chromogranin A and synaptophysin.
Detection and characterization of mutations
DNA samples were extracted from resected tumor tissues using a QIAamp DNA mini kit (Qiagen, Hilden, Germany) and were serially diluted to 50 ng/μl for use as DNA templates. Mutations in EGFR exon 19 and KRAS codons 12 and 13 were detected using the Sanger sequencing method according to previous studies (24,25). Mutations in EGFR exon 21 were detected by the Smart Amplification Process 2 assay, using an EGFR mutation detection kit (K.K. DNAFORM, Kanagawa, Japan). BRAF V600E mutations were detected using a LightMix kit for BRAF V600E (TIB MolBiol, Berlin, Germany). Genetic variations in 8 exons of DDR2 (exons 5, 8 and 12–17), which reportedly affect the activity of the protein or disease onset, were analyzed using the Sanger sequencing method according to previous studies, with slight modifications (13,26). Briefly, amplification was performed using 0.5 U AmpliTaq Gold DNA polymerase (Applied Biosystems, Foster City, CA, USA), 2.5 nmol of each dNTP, 1X polymerase chain reaction buffer, 1.8 nmol MgCl2, 5 pmol of each forward and reverse primer set and 25 ng of genomic DNA template in a reaction volume of 12.5 μl. Polymerase chain reaction was performed with an initial 5 min denaturation step at 95°C, followed by 35 cycles at 95°C for 30 sec, at 62°C for 35 sec and at 72°C for 45 sec, with a final elongation step at 72°C for 10 min. The annealing temperature for exon 5 was set at 66°C to prevent non-specific amplification.
Sequencing was performed with the Sanger dideoxy method with fluorescent automated sequencing on an ABI 3130xl Genetic Analyzer (Applied Biosystems) and the sequence data were analyzed using Sequencing Analysis Software v5.4 (Applied Biosystems).
In the patients whose cancer tissues were found to harbor genetic mutations in EGFR, KRAS, BRAF or DDR2, genomic DNA obtained from blood samples or peritumoral normal tissue was also analyzed to confirm the mutations as somatic or germline.
Results
Patient characteristics and detection of mutations
The characteristics of the patients are listed in Table I. The patients’ age, gender, smoking history and histological subtypes were comparable to those of Japanese non-AdLC patients previously reported (22). Among the 150 samples, a previously unreported mutation in DDR2 (1:162748496) was identified (Table II) in exon 17, near the area encoding the tyrosine kinase domain and resulted in an amino acid alteration (Phe804Ile). The same mutation was also detected in the samples derived from the blood of each patient. Conversely, no somatic mutation of DDR2 was detected in Japanese SCC, LCC, ASC, LCNEC or SCLC patients (Table III), whereas an unreported nonsense mutation (1:162746130) was detected in 1 LCC patient (Table II). Among the LCNEC and SCLC patients, 2 different non-coding mutations, namely rs2271305 in exon 5 and rs3738807 in the upstream region of exon 13, were detected in DDR2 (Table II).
Genetic mutations of EGFR exon 19 were detected in 3 SCC and 3 ASC patients and a mutation of KRAS codon 12 in 3 SCC patients (including the cases that were previously reported by Miyamae et al) and 1 LCNEC patient (Fig. 1 and Table III) (23). The EGFR and KRAS mutations were mutually exclusive and their frequencies did not differ between central and peripheral SCCs (Table IV). BRAF V600E was not found in any of the patients (Table III).
Discussion
In a previous study on North American subjects, somatic mutations of DDR2 were detected in 3.2% of SCC patients (13). Similar to EGFR and KRAS mutations, DDR2 mutations, particularly in the area encoding the tyrosine kinase domain, are considered to affect the intracellular downstream signaling pathways and lead to aberrant cell proliferation. In the present study, we analyzed exons 5, 8 and 12–17 of DDR2, in which somatic mutations were identified in the previous study on North American subjects; however, we did not identify a somatic mutation in our Japanese patients. Moreover, Sasaki et al (22) assessed the genetic diversity of exons 3–7 and 9–12 of DDR2 in Japanese patients and found no mutations. According to our results and those of Sasaki et al, we concluded that, although DDR2 is considered to be a candidate as a therapeutic target in European or North American non-AdLC patients, DDR2 mutations may only rarely be used as therapeutic targets in Japanese SCC patients, due to their extremely low frequency. Moreover, if the previously reported DDR2 mutations found in North American subjects were defined as driver mutations, our results suggested the possibility of racial differences in the oncogenic mechanism underlying SCC, since there is a racial difference in the frequency of these mutations. Similar to SCC, we were unable to identify any DDR2 mutations in other non-AdLC subtypes; however, a larger study is required to determine the frequency of DDR2 mutations in LCC, SCLC, LCNEC and ASC patients, as the sample size of our study was quite limited.
We identified an unreported germline mutation in DDR2. Although this mutation cannot be a driver mutation, since it is congenital, it may change the clinical efficacy of dasatinib through altering the affinity of dasatinib to DDR2, as this mutation is located in the area encoding the dasatinib-binding site. Thus, a more detailed study is required to elucidate the effect of this mutation on the clinical efficacy of dasatinib.
Conversely, we identified 6 somatic mutations in EGFR and KRAS in Japanese SCC patients, despite the reportedly rare frequency of such mutations in European and North American SCC patients. Additionally, we detected EGFR mutations in 3 ASC patients and KRAS mutations in 1 LCNEC patient. To the best of our knowledge, this is first study including a LCNEC patient harboring a KRAS mutation (27). These mutations have been considered to be driver mutations and our results indicated that EGFR or KRAS inhibitors may be effective for a subset of SCC, LCNEC and ASC patients, at least in the Japanese population. Indeed, the superior clinical effect of EGFR-TKIs in Asian non-AdLC patients harboring an EGFR mutation was reported in several studies (8,28,29) and molecular-targeted therapy against the downstream effectors of activated KRAS was reportedly more effective in patients harboring a KRAS mutation (30,31). In certain studies, detection sensitivity was discussed in depth, since highly sensitive methods were required to detect somatic mutations in AdLC containing a subpopulation of mutant cells mixed within an excess of normal tissue. However, as we focused on non-AdLCs with a high cellularity of tumoral tissue and a lower percentage of normal cells compared to AdLC, we hypothesized that detection sensitivity did not affect the data.
In the present study, the frequencies of EGFR and KRAS mutations in peripheral SCCs, which are mainly encountered in the Japanese population, were not different from those in central SCCs, which are mainly encountered in European and North American populations (32). These data indicate that the difference in mutation frequency may be caused by a difference in the cancer or oncogenic pathway between Japanese and European and North American subjects, rather than by a difference in the affected site.
As candidate therapeutic targets for non-AdLCs other than DDR2, certain genetic aberrations have been reported, including fibroblast growth factor receptor 1 amplification, phosphatidylinositol-4,5-bisphosphate 3-kinase, catalytic subunit α mutations, v-akt murine thymoma viral oncogene homolog 1 mutations and phosphatase and tensin homolog mutations (33). Since our results suggested that carcinogenic genes in non-AdLCs exhibit ethnic differences, a more detailed evaluation of these candidate genes in different ethnicities is required to make more appropriate suggestions for personalized drug therapy. Furthermore, since dasatinib inhibits a number of tyrosine kinases, including DDR2 (34), the association between the expression level or mutations of tyrosine kinases and the efficacy of dasatinib requires more detailed assessment.
In conclusion, this study suggests that DDR2 mutations and the BRAF V600E mutation may only rarely be used as therapeutic targets, at least in Japanese non-AdLC patients; however, EGFR and KRAS mutations may represent candidate therapeutic targets in Japanese non-AdLC patients. The detection of EGFR and KRAS mutations may be used to select the optimal treatment for Japanese non-AdLC patients. Other genetic aberrations that may be used as therapeutic targets should be assessed in detail among different ethnic groups.
Acknowledgements
We would like to thank Ms. Aiko Matsumoto for the secretarial assistance.
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