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首页> 外文期刊>Gastroenterology research and practice >A Downmodulated MicroRNA Profiling in Patients with Gastric Cancer
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A Downmodulated MicroRNA Profiling in Patients with Gastric Cancer

机译:胃癌患者的次调制MicroRNA分析

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Objective. Here, we aim to investigate the microRNA (miR) profiling in human gastric cancer (GC). Methods. Tumoral and matched peritumoral gastric specimens were collected from 12 GC patients who underwent routine surgery. A high-throughput miR sequencing method was applied to detect the aberrantly expressed miRs in a subset of 6 paired samples. The stem-loop quantitative real-time polymerase chain reaction (qRT-PCR) assay was subsequently performed to confirm the sequencing results in the remaining 6 paired samples. The profiling results were also validated in vitro in three human GC cell lines (BGC-823, MGC-803, and GTL-16) and a normal gastric epithelial cell line (GES-1). Results. The miR sequencing approach detected 5 differentially expressed miRs, hsa-miR-132-3p, hsa-miR-155-5p, hsa-miR-19b-3p, hsa-miR-204-5p, and hsa-miR-30a-3p, which were significantly downmodulated between the tumoral and peritumoral GC tissues. Most of the results were further confirmed by qRT-PCR, while no change was observed for hsa-miR-30a-3p. The in vitro finding also agreed with the results of both miR sequencing and qRT-PCR for hsa-miR-204-5p, hsa-miR-155-5p, and hsa-miR-132-3p. Conclusion. Together, our findings may serve to identify new molecular alterations as well as to enrich the miR profiling in human GC.
机译:客观的。在这里,我们的目的是探讨人胃癌(GC)中的microRNA(miR)分析。方法。从12个GC患者接受常规手术的患者中收集肿瘤和匹配的腹膜胃标本。应用高通量MIR测序方法以检测6个配对样品的子集中的异常表达的miR。随后进行茎环定量实时聚合酶链反应(QRT-PCR)测定以确认剩余的6个配对样品中的测序结果。在三种人GC细胞系(BGC-823,MGC-803和GTL-16)和正常胃上皮细胞系(GES-1)中也验证了分析结果。结果。检测到5种差异表达的MIR,HSA-MIR-132-3P,HSA-MIR-155-5P,HSA-MIR-19B-3P,HSA-MIR-204-5P和HSA-MIR-30A-3P的MIR测序方法,这在肿瘤和腹腔内GC组织之间显着折叠。大多数结果通过QRT-PCR进一步证实,而HSA-miR-30a-3p没有观察到任何变化。体外发现还同意了HSA-MIR-204-5P,HSA-MIR-155-5P和HSA-MIR-132-3P的MIR测序和QRT-PCR的结果。结论。我们的研究结果在一起可以用于鉴定新的分子改变,并丰富人GC中的MIR谱分析。

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