Differential responsiveness to BRAF inhibitors of melanoma cell lines BRAF V600E-mutated

被引:6
|
作者
Al Hashmi, Muna [1 ]
Konduru, Seetharama S. [1 ]
Silcock, Lee [1 ]
Chouchane, Lotfi [2 ]
Mattei, Valentina [1 ]
James, Nicola [1 ]
Mathew, Rebecca [1 ]
Bedognetti, Davide [1 ]
De Giorgi, Valeria [3 ]
Murtas, Daniela [4 ]
Liu, Wei [1 ]
Chouchane, Aouatef [1 ]
Temanni, Ramzi [1 ]
Seliger, Barbara [5 ]
Wang, Ena [1 ]
Marincola, Francesco M. [1 ,6 ]
Tomei, Sara [1 ]
机构
[1] Sidra Med & Res Ctr, Res Branch, Doha 26999, Qatar
[2] Weill Cornell Med Coll Qatar, Dept Genet Med, Doha, Qatar
[3] NIH, Infect Dis & Immunogenet Sect IDIS, Dept Transfus Med, Clin Ctr, Bethesda, MD USA
[4] Univ Cagliari, Dept Biomed Sci, Sect Cytomorphol, Cagliari, Italy
[5] Martin Luther Univ Halle Wittenberg, Inst Med Immunol, Halle, Germany
[6] Refuge Biotechnol, Menlo Pk, CA USA
基金
美国国家卫生研究院;
关键词
Next-generation sequencing; QPCR; Sanger sequencing; BRAF mutation; MUTATIONS; EXPRESSION; CANCER; GENE; SURVIVAL; THERAPY; KRAS;
D O I
10.1186/s12967-020-02350-8
中图分类号
R-3 [医学研究方法]; R3 [基础医学];
学科分类号
1001 ;
摘要
Background Most mutations in melanoma affect one critical amino acid on BRAF gene, resulting in the V600E substitution. Patient management is often based on the use of specific inhibitors targeting this mutation. Methods DNA and RNA mutation status was assessed in 15 melanoma cell lines by Sanger sequencing and RNA-seq. We tested the cell lines responsiveness to BRAF inhibitors (vemurafenib and PLX4720, BRAF-specific and sorafenib, BRAF non-specific). Cell proliferation was assessed by MTT colorimetric assay. BRAF V600E RNA expression was assessed by qPCR. Expression level of phosphorylated-ERK protein was assessed by Western Blotting as marker of BRAF activation. Results Three cell lines were discordant in the mutation detection (BRAF V600E at DNA level/Sanger sequencing and BRAF WT on RNA-seq). We initially postulated that those cell lines may express only the WT allele at the RNA level although mutated at the DNA level. A more careful analysis showed that they express low level of BRAF RNA and the expression may be in favor of the WT allele. We tested whether the discordant cell lines responded differently to BRAF-specific inhibitors. Their proliferation rate decreased after treatment with vemurafenib and PLX4720 but was not affected by sorafenib, suggesting a BRAF V600E biological behavior. Yet, responsiveness to the BRAF specific inhibitors was lower as compared to the control. Western Blot analysis revealed a decreased expression of p-ERK protein in the BRAF V600E control cell line and in the discordant cell lines upon treatment with BRAF-specific inhibitors. The discordant cell lines showed a lower responsiveness to BRAF inhibitors when compared to the BRAF V600E control cell line. The results obtained from the inhibition experiment and molecular analyses were also confirmed in three additional cell lines. Conclusion Cell lines carrying V600E mutation at the DNA level may respond differently to BRAF targeted treatment potentially due to a lower V600E RNA expression.
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页数:9
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