BRAF V600E 突变的黑色素瘤细胞系对 BRAF 抑制剂的差异反应性。
Differential responsiveness to BRAF inhibitors of melanoma cell lines BRAF V600E-mutated.
作者信息
Al Hashmi Muna, Sastry Konduru S, Silcock Lee, Chouchane Lotfi, Mattei Valentina, James Nicola, Mathew Rebecca, Bedognetti Davide, De Giorgi Valeria, Murtas Daniela, Liu Wei, Chouchane Aouatef, Temanni Ramzi, Seliger Barbara, Wang Ena, Marincola Francesco M, Tomei Sara
机构信息
Research Branch, Sidra Medical and Research Center, 26999, Doha, Qatar.
Department of Genetic Medicine, Weill Cornell Medical College in Qatar, Doha, Qatar.
出版信息
J Transl Med. 2020 May 11;18(1):192. doi: 10.1186/s12967-020-02350-8.
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.
背景
黑色素瘤中的大多数突变会影响BRAF基因上的一个关键氨基酸,导致V600E替代。患者管理通常基于使用针对该突变的特异性抑制剂。
方法
通过Sanger测序和RNA测序评估了15种黑色素瘤细胞系中的DNA和RNA突变状态。我们测试了这些细胞系对BRAF抑制剂(维莫非尼和PLX4720,BRAF特异性;索拉非尼,BRAF非特异性)的反应性。通过MTT比色法评估细胞增殖。通过qPCR评估BRAF V600E RNA表达。通过蛋白质印迹法评估磷酸化ERK蛋白的表达水平,作为BRAF激活的标志物。
结果
三个细胞系在突变检测中不一致(DNA水平/Sanger测序为BRAF V600E,RNA测序为BRAF野生型)。我们最初推测这些细胞系尽管在DNA水平发生了突变,但可能在RNA水平仅表达野生型等位基因。更仔细的分析表明,它们表达低水平的BRAF RNA,且表达可能有利于野生型等位基因。我们测试了不一致的细胞系对BRAF特异性抑制剂的反应是否不同。用维莫非尼和PLX4720处理后,它们的增殖率降低,但不受索拉非尼影响,表明具有BRAF V600E生物学行为。然而,与对照相比,对BRAF特异性抑制剂的反应性较低。蛋白质印迹分析显示,在用BRAF特异性抑制剂处理后,BRAF V600E对照细胞系和不一致的细胞系中p-ERK蛋白的表达降低。与BRAF V600E对照细胞系相比,不一致的细胞系对BRAF抑制剂的反应性较低。在另外三个细胞系中也证实了抑制实验和分子分析的结果。
结论
在DNA水平携带V600E突变的细胞系可能对BRAF靶向治疗有不同反应,这可能是由于V600E RNA表达较低。
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