Abstract
Aims. To develop a fast and robust DNA-based assay to detect insertions and deletions mutations in exon 34 that encodes the PEST domain of NOTCH1 in order to evaluate patients with chronic lymphocytic leukemia (CLL). Methods. We designed a multiplexed allele-specific polymerase chain reaction (PCR) combined with a fragment analysis assay to detect specifically the mutation c.7544_7545delCT and possibly other insertions and deletions in exon 34 of NOTCH1. Results. We evaluated our assay in peripheral blood samples from two cohorts of patients with CLL. The frequency of NOTCH1 mutations was 8.4% in the first cohort of 71 unselected CLL patients. We then evaluated a second cohort of 26 CLL patients with known cytogenetic abnormalities that were enriched for patients with trisomy 12. NOTCH1 mutations were detected in 43.7% of the patients with trisomy 12. Conclusions. We have developed a fast and robust assay combining allele-specific PCR and fragment analysis able to detect NOTCH1 PEST domain insertions and deletions.
1. Introduction
Chronic lymphocytic leukemia (CLL) is a neoplastic disorder of B lymphocytes characterized by progressive increase in CD5+ B cells in the peripheral blood (PB), bone marrow, and lymph nodes. The clinical course of CLL is highly heterogeneous, with some patients experiencing indolent disease, with no treatment requirement for several years, and others showing aggressive course and decreased overall survival (OS) [1].
Although several prognostic factors have been identified in CLL, such as TP53 mutation, cytogenetic abnormalities, IGVH mutational status, the only biomarkers utilized to inform clinical decisions nowadays are 17p or TP53 mutations [1]. Since these alterations are present in a minority of patients, most CLL cases are treated based on clinical criteria.
Recently, novel prognostic relevant recurrent mutations in genes such as NOTCH1, SF3B1, and BIRC3 have been identified in CLL [2, 3]. The most common of these alterations are NOTCH1 and SF3B1 mutations, which are present in around 10% of CLL patients at diagnosis [2].
NOTCH1 mutations in CLL occur almost exclusively in the genic region encoding the PEST domain and are characterized by frameshift insertions and deletions, with the mutation c.7544_7545delCT representing more than 75% of the mutations [4, 5]. In addition, NOTCH1 mutations have been associated with decreased OS and treatment-free survival (TFS) in several independent studies [3–6]. The goal of this work was to develop a simple, robust, and cost-effective assay to identify NOTCH1 PEST domain mutations and also to evaluate the frequency of NOTCH1 mutations in a cohort of CLL patients.
2. Methods
This study was approved by the Institutional Review Board of Hospital Israelita Albert Einstein (protocol 1699-13). Consent form was waived, since the samples were deidentified and the researchers did not have access to clinical information. Peripheral blood mononuclear cells were isolated (PBMC) by Ficoll-Paque gradient centrifugation and genomic DNA was extracted with QIAamp DNA Mini Kit (Qiagen). Fragment analysis and sequencing with BigDye Terminator v3.1 Cycle Sequencing Kit were performed in the equipment 3500XL Genetic Analyzer (Applied Biosystems).
Polymerase chain reaction (PCR) amplification and sequence analysis of IGHV-D-J rearrangements were performed on genomic DNA from PB samples, using VH framework region 1 (FR1) consensus family specific primers (VH1–VH6) and a JH primer, according to the BIOMED-2 protocol [7]. When amplification was unsuccessful, an alternative set of primers that anneal to the leader region (LH1–LH6) and a JH consensus primer were used. Clonal PCR products were purified using Wizard SV Gel and PCR Clean-Up System (Promega), and both strands were directly sequenced with BigDye Terminator v3.1 Cycle Sequencing Kit (Applied Biosystems, Carlsbad, CA) on a 3130XL Genetic Analyzer (Applied Biosystems). The sequences were aligned to the closest matching germ line gene by using IMGT's V-QUEST analysis tool (http://www.imgt.org/IMGT_vquest/share/textes/) and NCBI's IgBLAST tool (https://www.ncbi.nlm.nih.gov/igblast/). Sequences with a germ line identity greater than or equal to 98% were considered unmutated and those with an identity less than 98% were considered mutated [8].
Exact Fisher's test was used to compare patients with mutated and wild-type NOTCH1 regarding IGVH mutational status.
3. Results
The assay we developed had two main goals: to detect insertions and deletions in the region of NOTCH1 exon 34 encoding the PEST domain and also to specifically detect the mutation c.7544_7545delCT, which accounts for around 80% of all NOTCH1 mutations in CLL [4]. To accomplish this, we designed a fragment analysis PCR with three primers: a forward primer (N1F) labeled with FAM (CATCCAGCAGCAGCAAAGC), a nonspecific reverse primer (NWR) (GTCGGAGACGTTGGAATGC) that amplifies the wild-type sequence, and another allele-specific reverse primer that amplifies only the mutation c.7544_7545delCT (NMR) (CCACTGGTCAGGGGACTCG). We then performed a single PCR reaction with the three primers. Samples with wild-type NOTCH1 would produce a single product of 391 bp; samples harboring heterozygous c.7544_7545delCT would generate three products: 391 bp (wild-type allele), 389 bp (amplification of the mutated allele with primers N1F and NWR), and 356 bp (amplification of the mutated allele with N1F and NMR) (Figures 1(a) and 1(b)). Finally, samples with another heterozygous insertion or deletion in the PEST domain would yield two products, 391 bp from the wild-type allele and another variable product, depending on the size of the insertion or deletion.
To validate our assay, we evaluated two groups of CLL patients. The initial group consisted of consecutive deidentified samples from 71 patients with CLL in distinct disease stages that had PB flow cytometry evaluation at our laboratory, for which we had no clinical or cytogenetic information. We identified NOTCH1 mutations in 6 patients (8.4%). To confirm that our test was indeed detecting the expected mutations, we performed Sanger sequencing of all 6 positive cases and 3 negative cases, confirming the specificity of our assay (Figure 1(c)).
We then analyzed a second group of 26 consecutive CLL patients that had been successfully evaluated with fluorescent in situ hybridization (FISH) at our laboratory. All these patients had recurrent cytogenetic abnormalities (trisomy 12, 13q, 17p, and 11q present in 16, 6, 3, and 1 patient, resp.). This group was enriched for patients with trisomy 12, since this population is known to harbor NOTCH1 mutations frequently [9]. We found NOTCH1 mutations in 10 patients of the second cohort (38.4%). Among patients with trisomy 12 (n = 16), the prevalence of NOTCH1 mutations was 43.7% (n = 7), in agreement with previous reports [9]. All mutations identified in these patients (n = 16) were c.7544_7545delCT. We did not find other NOTCH1 mutations in CLL patients. While 15 patients had heterozygous mutation, 1 patient presented with a homozygous mutation.
Since the presence of NOTCH1 mutations has been associated with unmutated IGVH [5], we performed IGVH mutational status analysis in 63 out of the 97 analyzed patients, based on DNA availability. Among these samples, 9 had NOTCH1 mutation and 54 had wild-type NOTCH1. IGVH mutational status was inconclusive in 10 patients due to low numbers of CLL cells in PB. Among the 53 evaluable patients, unmutated IGVH was detected in 100% of NOTCH1 mutated cases (n = 7) and in 37% (n = 17) of patients with wild-type NOTCH1 (p = 0.002), confirming previous findings [10].
We next determined the sensitivity of our test with serial dilutions of the cell line MOLT4 which carries a heterozygous c.7544_7545delCT NOTCH1 mutation, using normal peripheral blood mononuclear cells. We diluted samples in the following way: 1 : 2, 1 : 5, 1 : 10, 1 : 20, and 1 : 40. The sensitivity of our test was 5%, meaning we can detect NOTCH1 mutations when 5% of cells harboring NOTCH1 heterozygous mutations are mixed with 95% of cells with wild-type NOTCH1.
In order to calculate the sensitivity of our assay to other exon 34 NOTCH1 insertions and deletions, given that the only mutation detected in CLL patients in our study was c.7544_7545delCT, we evaluated three samples from patients with T-acute lymphoblastic leukemia (T-ALL), known to harbor insertions and deletions in NOTCH1 exon 34. Our test correctly identified all three mutations in these samples (see Figure 2).
4. Discussion
Mutated NOTCH1 is a biomarker associated with Richter transformation, chemoresistance, and reduced overall and progression-free survival in CLL [10, 11]. These mutations are characterized by frameshift insertions and deletions in exon 34, with c.7544_7545delCT occurring in around 80% of mutated cases [4, 10]. The functional consequence of such NOTCH1 mutations is the disruption of the PEST domain and stabilization of the NOTCH1 protein leading to constitutive activation of NOTCH1 pathway [12]. For these reasons, the evaluation of NOTCH1 mutational status may have implications for the clinical management of CLL patients. We have thus developed a fast, robust, and sensitive assay for detection of NOTCH1 PEST domain insertions and deletions.
Our data is consistent with previous findings of around 10% prevalence of NOTCH1 mutations in unselected CLL patients and around 40% prevalence in CLL with trisomy 12 [6, 9]. Of note, mutations in the gene FBXW7, which belongs to NOTCH1 pathway, also seem to be more prevalent in patients with trisomy 12 and are associated with a worse outcome [13]. In addition, the previously described high correlation between unmutated IGVH and NOTCH1 mutations was confirmed in our cohort [4, 10].
The identification of NOTCH1 mutations in CLL can be useful as a prognostic marker [4] and also as a potential therapeutic target in the future [14]. The analysis of NOTCH1 mutations in patients from the German CLL8 trial suggests that CLL patients harboring NOTCH1 mutations may not benefit from the addition of rituximab to fludarabine and cyclophosphamide, indicating that NOTCH1 may also become a predictive marker of response to rituximab in CLL [15].
While our test was developed to detect any insertions and deletions in exon 34, in our CLL cohort, we only identified the most common deletion, c.7544_7545delCT, in agreement with previous findings [3, 7]. Nevertheless, the identification of other insertions and deletions in T-ALL samples validates our assay to other mutations that are rarer and may be found in CLL (see Figure 2). Our assay does not detect single nucleotide variations that may be found on NOTCH1 exon 34; nevertheless, the pathogenic significance of such mutations remains to be defined [16].
In conclusion, we have developed a simple and robust assay combining allele-specific PCR and fragment analysis for the identification of NOTCH1 PEST domain mutations. We have also shown that, among Brazilian patients analyzed, the prevalence of NOTCH1 mutations and the correlation with unmutated IGVH in CLL are in agreement with previous reports [3–6].
Acknowledgments
The authors would like to thank Dr. Maria do Socorro Pombo-de-Oliveira, Head of Paediatric Haematology-Oncology Program, for providing DNA material used in the assay sensitivity tests.
Ethical Approval
Institutional Review Board of Hospital Israelita Albert Einstein approved this study (protocol 1699-13).
Competing Interests
The authors declare that there are no competing interests regarding the publication of this paper.
Authors' Contributions
Paulo Vidal Campregher designed the study, developed the assay, and wrote the manuscript. Flavia Pereira de Carvalho, Rocio Hassan, and Davi Coe Torres performed the IGHLM mutational status assays and interpreted the results. Roberta Cardoso Petroni and Nair Hideko Muto performed experiments (data acquisition), revised the manuscript critically, and revised and approved the final version to be published. Roberta Sitnik contributed with study design and supervised experiments (data acquisition), revised the manuscript critically, and revised and approved the final version to be published. Nydia Strachman Bacal, Elvira Deolinda Rodrigues Pereira Velloso, Gislaine Borba Oliveira, Irene Gyongyvér Heidemarie Lorand-Metze, Carlos Sérgio Chiattone, and Nelson Hamerschlak contributed with samples from patients (data acquisition), revised the manuscript critically, and revised and approved the final version to be published. João Renato Rebello Pinho and Cristovão Luis Pitangueira Mangueira contributed with study design and interpretation of results, revised the manuscript critically, and revised and approved the final version to be published. Marcela Braga Mansur helped with ALL samples and revised the manuscript.
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