Background
Non-small cell lung cancer (NSCLC) is a leading cause of cancer-related death. Systemic chemotherapy remains palliative and modestly effective. Recently, multiple prospective clinical studies have shown that
EGFR mutation is a strong predictor of efficacy of epidermal growth factor receptor tyrosine kinase inhibitor (EGFR-TKIs) therapy in advanced NSCLC. More than 70 % of NSCLC patients carrying
EGFR mutations achieved marked and durable responses to treatment with the EGFR-TKIs gefinitib or erlotinib [
1,
2]. However, although several potential mechanisms of primary resistance, including Bim deletion polymorphism [
3], KRAS mutation [
4], and ALK fusion [
5] have been explored in several preclinical and retrospective studies, the molecular basis of primary resistance to EGFR-TKI remains unclear.
MicroRNA is a newly defined class of small noncoding RNAs of 21–25 nucleotides in length that has recently been implicated in cancer biology, which could post-transcriptionally regulate gene expression by binding to complementary sequences in the 3′ untranslated region (3′UTR) of the target messenger RNA [
6]. This could ultimately lead to repression of protein translation and down-regulation of protein expression [
7]. Deregulation of microRNAs (miRNAs) is emerging as an important area of study in carcinogenesis because their regulatory capabilities can drastically influence cell physiology [
8], and it was also reported to be with EMT which might be attributed to resistance to anti-tumor therapy [
9,
10]. Many studies have examined miRNA expression profiles with the goal of identifying miRNA using non-invasive blood samples as biomarkers for the diagnosis of lung cancer. Most of these studies have quantified miRNAs in free-cellular cfDNA of serum [
8,
11] or plasma [
12‐
14], and a new strategy could be investigated accordingly [
15]. Although all these studies have shown promising results, there are some limitations with the use of serum or plasma RNA for miRNA biomarker discovery. We proposed that miRNAs might regulate the
EGFR gene pathway and could be a predictor of response to EGFR-TKI therapy. Genomic loss of miRNAs capable of down-regulating EGFR would be expected to enable increased EGFR expression, thereby offering a more robust target for the EGFR-TKIs.
Based on the fact that primary resistance to EGFR-TKIs exists in a portion of patients with a sensitizing mutant-type, it is critical to identify potential biomarkers that can help determine the subgroup of patients with primary resistance to EGFR-TKIs therapy. In this study, we investigated the expression profiles of miRNAs in EGFR-mutated NSCLC patients with either dramatic responses or primary resistance to EGFR-TKI therapy, and explored which miRNA may play a role in primary resistance to EGFR-TKIs in EGFR-mutant patients. Finally, we propose strategies to avoid primary resistance to EGFR-TKIs in the near future.
Materials and methods
Patients enrolled in this study were diagnosed pathologically with NSCLC stage IIIB–IV or recurrent disease and received EGFR-TKIs treatment from April 2004 to August 2012 at the Beijing Cancer Hospital. All of the patients harboring EGFR 19 deletion mutations detected in both plasma and tissues received 250 mg of gefitinib or 150 mg of erlotinib daily until disease progression, intolerable toxicity, or patient refusal. None of the patients had KRAS mutation, T790M mutation, or C-MET amplification. All of the patients had bi-dimensionally measurable disease and presented an Eastern Cooperative Oncology Group (ECOG) performance status of 0 to 2. Blood samples were collected prior to EGFR-TKI treatment for biomarker analysis. All patients provided written informed consent and a separate consent was obtained for the optional provision of a tumor sample for biomarker analysis. The Institutional Ethics Committee at Beijing Cancer Hospital approved the study protocol.
Study design
The study was designed to explore the potential role of miRNAs in primary resistance to EGFR-TKIs treatment. Tumor specimens were obtained at initial diagnosis. Clinical data were sealed during the laboratory analysis until all data were evaluated. Recorded variables included age, sex, smoking history, pathology, and ECOG performance status, stage at diagnosis, treatments, and toxicities. Outcome indicators included progression-free survival (PFS) and overall survival (OS). We defined primary resistance of EGFR-TKI as PFS ≤3 months (90 days) without any evidence of objective response while receiving EGFR-TKI [
16].
Although both EGFR exon 19 deletions and 21 mutations (L858R) are sensitive aberrances which present excellent efficacy to EGFR-TKIs treatment, recently, a serial of pooled and meta-analysis comparing first-line chemotherapy in patients with EGFR mutations with first- and second-generation EGFR-TKIs showed that patients with EGFR 19 del had significantly longer overall survival time (OS) or/and PFS compared to those treated with platinum-based chemotherapy. On the contrary, the patients with L858R mutation had longer OS or/and PFS in the chemotherapy group than in EGFR-TKIs treatment group [
17]. Thus, it has reached the consensus that EGFR19 del and L858R mutations are two different diseases and required different treatment strategies. We therefore speculated that primary resistant mechanism of EGFR exon 19 deletion and L858R mutant may be different. The current study focuses on EGFR 19 deletion mutant NSCLC.
Three cohorts of patients were selected randomly from our database:
-
Training group: There were 20 advanced NSCLC patients with EGFR 19 deletion treated with first-line EGFR-TKIs, 10 of whom responded dramatically with a PFS over 13 months, while the other 10 presented primary resistance with a relatively short PFS of less than 3 months. Matched plasma was collected for miRNA profile detection using TaqMan low-density array (TLDA).
-
Testing group: Real-time PCR was used to evaluate the differential expression of miRNAs identified in the training group. Bioinformatics analyses were applied to explore the possible miRNAs that could have been involved in the observed resistance.
-
Validation group: The set included two cohorts of 17 patients each harboring EGFR 19 deletion mutations, with dramatic responses and primary resistance to EGFR-TKIs in each cohort were used to confirm the miRNAs identified in the training and testing sets. Another cohort of 48 EGFR wild-type patients with dramatic response (24 patients) or primary resistance to EGFR-TKI was chosen to verify reversely that identified miRNAs in the first two groups attributing to primary resistance of EGFR-mutant NSCLC patients have no relation with resistance of EGFR wild-type NSCLC patients.
Assessments
Tumor assessments, including computed tomography scans of the chest, type-B ultrasonic inspection of bilateral cervical lymph nodes and upper abdomens, magnetic resonance imaging scans of brains, and emission computed tomography scans of bone, were performed at baseline and every 8 weeks until the investigators documented disease progression or unacceptable toxicity. The clinical responses to TKIs including complete response (CR), partial response (PR), stable disease (SD) and disease progression (PD) were determined on the basis of the Response Evaluation Criteria in Solid Tumors (RECIST 1.1) [
18]. PFS was defined as the time from the beginning of TKI treatment to PD or death, and OS was defined as the time from the beginning of TKI treatment to death. An independent radiologist (Dr. Ning Wang) assessed all films and was blinded to the
EGFR biomarker status.
Specimen collection and DNA extraction
Each enrolled patient from our database exhibited specific EGFR mutation status (exon 19 deletion) consistently in both tissue and blood. All patients provided sufficient blood samples for miRNA analysis. Prior to TKI or second-line chemotherapy, 4 mL of anticoagulated venous blood from each patient was collected and placed at 4 °C for 4 h, then centrifuged at 2500 rpm for 10 min at low temperature. The plasma was aspirated to a new centrifuge tube, and the high speed centrifugation was repeated. Of the plasma, 1.5 mL was obtained, to which 15 μL of protease K (20 mg/mL) and 50ro SDS (20 %) was added to 1.5 ml of plasma. DNA was extracted using phenol/chloroform/isopentanol after a 2-h incubation in a water bath at 60 °C. DNA was precipitated in alcohol and centrifuged the next day. After salt washing, the precipitate was dissolved in TE and then preserved at −20 °C.
EGFR activating mutation detection by denaturing high-performance liquid chromatography and amplification refractory mutation system
Specimen collection, DNA extraction, and denaturing high-performance liquid chromatography (DHPLC) were performed according to methods described in our previous publication [
19]. The amplification refractory mutation system (ARMS), a more sensitive method for detecting
EGFR activating mutation, was used to reevaluate the results detected by DHPLC [
20].
Quantification of circulating miRNAs from plasma
Total RNA was extracted from 350 μL of plasma using TRIzol LS reagent (Invitrogen) and dissolved in 10 μL of DEPC (diethylprocarbonate) water. The quantity and quality of total RNA were determined with the use of a spectrophotometer (GeneQuant pro, GE Healthcare). miRNAs were quantified by quantitative reverse transcriptase-polymerase chain reaction (qRT-PCR) TaqMan miRNA Assays (Applied Biosystems) according to the manufacturer’s instructions. Ten nomograms of total RNA were used to synthesize miRNA-specific complementary DNA (cDNA). PCR was performed in duplicates for 40 cycles using an ABI Prism 7900HT Sequence Detection System (Applied Biosystems). The Ct value was defined as the cycle number at which the fluorescence (ΔRn) exceeded the threshold. The threshold was 0.20, which was defined as the default setting. To evaluate the miRNA expression levels, PCR was carried out in duplicate, and the average of the Ct values was converted into 2−Ct. If the Ct value could not be determined because the PCR was run for up to 40 cycles and the miRNA expression level was still below the detection limit, the Ct value was treated as 40 (i.e., miRNA expression level = 2–40).
MicroRNA microarray analysis of plasma and microRNA quantification
Total RNA was isolated using mirVana miRNA isolation kit (Ambion). For miRNA cDNA synthesis, RNA was reverse transcribed using a miRNA reverse transcription kit (Applied Biosystems) in combination with the stem-loop Megaplex primer pool (Applied Biosystems). TLDA v2.0 (Applied Biosystems) was performed on the 7900HT real-time PCR system (Applied Biosystems) according to the manufacturer’s protocol (764 small RNAs were profiled for each cDNA sample). PCR cycling conditions were as follows: 95 °C for 10 min followed by 40 cycles of 95 °C for 15 s and 60 °C for 1 min. Human U6 small RNA was used as an internal control to normalize RNA input. The data were analyzed using SDS v2.3 software. The Ct value was defined as the fractional cycle number at which the fluorescence passed the fixed threshold. The fold change was calculated using the 2-ΔΔCt method and presented as the fold-expression change in tumors and their adjacent normal tissues after normalization to the endogenous control. Significance was considered to be the p < 0.05 level.
Target gene prediction
The target genes of the deregulated miRNAs were predicted with TargetScan; conserved and non-conserved targets of miRNAs were identified using TargetScan 3.1. The list of predicted targets was obtained via download from TargetScan (
http://www.targetscan.org/).
Ingenuity Pathway Analysis (IPA) 3.0 (Ingenuity Systems 4) was used to analyze the list of predicted miRNAs targets. Filtering was performed to remove duplicates and to remove genes with no annotation in the Ingenuity Pathways Knowledge Base, resulting in a list of 765 network eligible genes. Each gene identifier was mapped to its corresponding gene object in the Ingenuity Pathways Knowledge Base. Networks of genes were then algorithmically generated. GO analysis was also performed using IPA.
Quantitative PCR
To verify the accuracy of our microarray and TLDA data, we performed single qRT-PCR for representative miRNAs using TaqMan miRNA Assays (Applied Biosystems) according to the manufacturer’s instructions. Briefly, total RNA was extracted from plasma using TRIzol Reagent (Invitrogen, Carlsbad, CA, USA) and used to synthesize cDNA with gene-specific primers. Reverse transcriptase reactions contained 100 ng RNA, 50 nmol/L stem-loop RT primers, 1 × RT buffer, 0.25 mmol/L each of the dNTPs, 3.33 U/μL MultiScribe reverse transcriptase, and 0.25 U/μL RNase inhibitor. The 15-μL reactions were incubated for 30 min at 16 °C, 30 min at 42 °C, 5 min at 85 °C, and then kept at 4 °C. The cDNA products were used for the subsequent qRT-PCR analysis. The 20-μL PCR reaction included 1.33 μL RT product, 1 × TaqMan universal PCR master mix, and 1 μL primers and probe mix of the TaqMan miRNA assay kit. Reactions were incubated in a 96-well optical plate at 95 °C for 5 min, followed by 40 cycles at 95 °C for 15 s, and 60 °C for 1 min. PCR reactions were run on a StepOne Plus real-time PCR machine (Applied Biosystems), and the data were analyzed using SDS v2.3 software. Triplicate samples, validated endogenous controls, and interassay controls were used throughout these experiments. miRNA expression levels were calculated using the 2-ΔΔCt method. The relative expression of the miRNA of interest corresponded to the 2-miR value.
Statistical analyses
SPSS 16.0 was used to calculate the statistical significance. Wilcoxon tests were applied to compare the differences of expression for miRNA between the different response groups.
Discussion
The mechanism of primary resistance to EGFR-TKIs in EGFR-mutant NSCLC is not clearly understood. In this study, we analyzed miRNA expression signatures related to primary resistance to EGFR-TKIs in EGFR-mutant NSCLC patients. Our results indicate the existence of miRNA expression patterns that could distinguish between sensitive and resistant NSCLC patients with EGFR activating exon 19 deletion mutations, therefore identifying those who could benefit from EGFR-TKIs and providing promising therapeutic opportunities.
In the present study, we identified three miRNAs potentially related with primary resistance to EGFR-TKIs in exon 19-mutated NSCLC. We subsequently utilized another cohort of 19 exon-mutated patients to validate this result. Moreover, we thought it is necessary to use another subgroup of patients with wild-type EGFR who had matched short and long PFS to verify reversely that the identified miRNAs in the first two groups contribute to primary resistance of EGFR 19 del NSCLC patients, but have no relation with resistance of EGFR wild-type NSCLC patients. Forty-eight EGFR wild-type patients came from our database; we intentionally chose this subgroup of patients with the matched longest and shortest PFS. Multiple studies have suggested that a small subgroup of patients without EGFR mutation (around 10 %) also can benefit from EGFR-TKIs therapy; it might attribute to some uncommon mutations of EGFR (such as G719 and L861) [
21] or other unknown mechanisms for now. What is more, in our database, we found that around 50 % of patients in this study underwent EML4-ALK detection (FISH or VATANA), and no positive cases were found. As we know, EML4-ALK fusion and EGFR mutation are often exclusive for most patients, and incidence rate of overlapping EML4-ALK fusion and EGFR sensitive mutation was only about 0–8 % in NSCLC patients [
5,
22].
In our study with TaqMan miRNA array and qRT-PCR confirmation, 12 deregulated miRNAs were predicted by TargetScan in conjunction with bioinformatics methods (miR-448, miR-605, miR-628-5p, miR-561, miR-520f, miR-409-3p, has-miR-138, miR-296-5p, miR-218, miR-1274B, miR-21, and miR-27a) in a training set. Three up-regulated miRNAs (miR-21, miR-27a, and miR-218) were identified in EGFR-mutant NSCLC patients resistant to EGFR-TKIs in the testing and validating cohorts.
High levels of miR-21 expression have been reported in various types of human tumors including lung cancer [
23‐
25]. However, the mechanism that up-regulates miR-21 during carcinogenesis has not been identified yet. Seike et al. reported in 2009 that miRNA microarray data showed higher levels of miR-21 in
EGFR-mutant cases [
26], and in vitro analyses using NSCLC cell lines showed that activated EGFR signaling up-regulated miR-21 expression. A statistically significant positive correlation was observed between miR-21 expression levels and p-EGFR levels in NSCLC cell lines. Furthermore, treatment with the EGFR-TKI (AG1478) inhibited miR-21 expression in two NSCLC cell lines with elevated p-EGFR,
EGFR-mutant H3255, and
EGFR wild-type H441, providing a mechanistic link between an activated EGFR signaling pathway and the aberrant up-regulation of miR-21, and a therapeutic basis for the inhibition of miR-21 in lung cancers with EGFR activation. Following antisense oligonucleotide-mediated knockdown of miR-21, induced or enhanced apoptotic responses in two NSCLC cell lines, H3255 and H441, suggested that miR-21 could also be a therapeutic target in resistant
EGFR-mutant NSCLC. Recent reports suggested that miR-21 overexpression was associated with resistance to cytotoxic agents, including gemcitabine [
27], docetaxel [
28], temozolomide [
29], and taxan [
30]. A recent study [
31] based on animal model and clinical samples clarified that miR-21 overexpression was associated with acquired resistance to EGFR-TKI in NSCLC, which might be caused by miR-21’s function in activating the PI3K/AKT pathway through PTEN and PDCD4 inhibition. In our study, we identified miR-21 as a potential biomarker of resistance to EGFR-TKIs in
EGFR-mutant patients. This is the first study that identified a potential association between miR-21 and primary resistance to EGFR-TKIs in
EGFR-mutant patients. This finding needs to be further verified with in vitro and in vivo studies of molecular mechanisms and in larger clinical studies.
Studies involving associations of miR-27a and miR-218 with resistance to EGFR-TKIs in NSCLC are extremely limited for now. T790M mutation and
MET gene amplification have been considered as important acquired resistant mechanisms. Recently, several studies also reported that T790M mutation or
MET gene amplification could co-exist with
EGFR sensitive mutation in therapy-naïve patients [
20,
32], suggesting that these two mechanisms may play important roles in primary resistance to EGFR-TKIs. Yoon and his colleagues [
33] identified a mechanism linking miR-27a, MET, and EGFR that involves Sprouty2, and thus illustrating cross-talk between MET and EGFR in NSCLC. This study also showed that EGFR and MET receptor tyrosine kinases, through regulation of expression of specific miRNAs such as miR-218, control the metastatic behavior and gefitinib resistance of NSCLCs. Garofalo et al. [
34] reported that the modulation of specific miRNAs, such as miR-30b, miR-30c, miR-221, and miR-222, might play a role in acquired resistance to EGFR-TKIs and could have therapeutic applications to sensitize lung tumors to TKI therapy [
35]. However, these studies mainly focused on the association of plasma miRNA and MET in acquired resistance to EGFR-TKIs. The present study is the first to identify that miR-27a, miR-218, and miR-27a might play a role in primary resistance to EGFR-TKI in advanced NSCLC patients with
EGFR exon 19 deletion mutations treated with EGFR-TKI, independent of c-MET amplification and T790M mutation. Other relevant mechanisms should be further investigated in basic research [
36‐
38].
Competing interests
The author(s) declare that they have no competing interests.
Authors’ contributions
SW disign the study, compose the manuscript. XS carry out research in lab, sumarize data, compose the manuscript. HB carry out research in lab, sumarize data. JZhao collect clinical sample and data. JD collect clinical sample and data. TA collect clinical sample and data. MZ collect clinical sample and data. ZW collect clinical sample and data. MW collect clinical sample and data. ZL edit the manuscript. JZhu edit the manuscript. JW disign the study, direct the research, compose the manuscript. All authors read and approved the final manuscript.