Centromere-associated protein E expresses a novel mRNA isoform in acute lymphoblastic leukemia.

International journal of molecular epidemiology and genetics Pub Date : 2018-10-20 eCollection Date: 2018-01-01
Cindy E Jiménez-Ávila, Vanessa Villegas-Ruíz, Marta Zapata-Tarres, Alejandra E Rubio-Portillo, Eleazar I Pérez López, Juan C Zenteno, Sergio Juárez-Méndez
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Abstract

The alternative splicing plays an important role to generate protein diversity. Recent studies have shown alterations in alternative splicing, resulting in loss, gain or changes of functions in the resulting protein. Specific products of alternative splicing are known to contribute in cancer-related mechanisms, such as angiogenesis, migration, adhesion and cell proliferation, among others. We using high-density microarrays reported a CENP-E as a one of significant transcript expressed and potentially is alternatively spliced in cancer. We focus in validate alternative splicing of CENP-E transcript using RT-PCR and sequencing in different cancer cell lines. We performed RT-PCR using specific primers designed to delimit the non-reported alternative splicing in CENP-E transcript. Our results showed the co-expression of the variant one and two of CENP-E in all cell lines evaluated. We detected more expression of variant one than two. Moreover, we identify an alternative 5'splice site of CENP-E in the exon 38 and was observed in RoVa cell line. Additionally, we characterized alternative skipping from exon 20 (NAT-CENP-E), these alternative splicing was observed in all cell lines evaluated except RoVa. Finally, we corroborate alternative mRNA splicing in leukemia patients using quantitative RT-PCR, in 71.8% of the patients NAT-CENP-E is downregulated and 28.2% is overexpressed.

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着丝粒相关蛋白E在急性淋巴细胞白血病中表达一种新的mRNA亚型。
选择性剪接在蛋白质多样性的产生中起着重要作用。最近的研究表明,选择性剪接的改变会导致蛋白质功能的丧失、获得或改变。已知选择性剪接的特定产物参与癌症相关机制,如血管生成、迁移、粘附和细胞增殖等。我们使用高密度微阵列报道了一个CENP-E作为一个重要的转录物表达,并可能在癌症中选择性剪接。我们着重于利用RT-PCR和测序技术在不同的癌细胞系中验证CENP-E转录物的选择性剪接。我们使用设计的特定引物进行RT-PCR,以分隔CENP-E转录物中未报道的选择性剪接。我们的结果显示CENP-E变体1和变体2在所有被评估的细胞系中共表达。我们发现变异1的表达比变异2更多。此外,我们在38号外显子中发现了另一个5'剪接位点,并在RoVa细胞系中观察到。此外,我们还发现了20号外显子(NAT-CENP-E)上的选择性跳变,这些选择性剪接在除RoVa外的所有细胞系中都观察到了。最后,我们使用定量RT-PCR证实了白血病患者的mRNA剪接,在71.8%的患者中,NAT-CENP-E下调,28.2%的患者过表达。
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