The long noncoding RNA SUMO1P3 as urinary biomarker for monitoring bladder cancer progression

Silvia Galbiati, A. Bettiga, G. Colciago, C. Senti, Francesco Trevisani, Giulia Villa, Ilaria Marzinotto, Michele Ghidini, R. Passalacqua, Francesco Montorsi, A. Salonia, R. Vago
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Abstract

Urothelial Bladder Cancer (BC) is the ninth most common cancer worldwide. It is classified into Non Muscle Invasive (NMIBC) and Muscle Invasive Bladder Cancer (MIBC), which are characterized by frequent recurrences and progression rate, respectively. The diagnosis and monitoring are obtained through invasive methods as cystoscopy and post-surgery biopsies. Thus, a panel of biomarkers able to discriminate BC based on grading or staging represents a significant step forward in the patients’ workup. In this perspective, long non-coding RNAs (lncRNAs) are emerged as reliable candidates as potential biomarker given their specific and regulated expression. In the present work we propose two lncRNAs, the Small Ubiquitin Modifier 1 pseudogene 3 (SUMO1P3), a poorly characterized pseudogene, and the Urothelial Carcinoma Associated 1 (UCA1) as candidates to monitor the BC progression.This study was a retrospective trial enrolling NMIBC and MIBC patients undergoing surgical intervention: the expression of the lncRNA SUMO1P3 and UCA1 was evaluated in urine from 113 subjects (cases and controls). The receiver operating characteristic curve analysis was used to evaluate the performance of single or combined biomarkers in discriminating cases from controls.SUMO1P3 and UCA1 expression in urine was able to significantly discriminate low grade NMIBC, healthy control and benign prostatic hyperplasia subjects versus high grade NMIBC and MIBC patients. We also demonstrated that miR-320a, which binds SUMO1P3, was reduced in high grade NMIBC and MIBC patients and the SUMO1P3/miR-320a ratio was used to differentiate cases versus controls, showing a statistically significant power. Finally, we provided an automated method of RNA extraction coupled to ddPCR analysis in a perspective of clinical application.We have shown that the lncRNA SUMO1P3 is increased in urine from patients with high grade NMIBC and MIBC and that it is likely to be good candidate to predict bladder cancer progression if used alone or in combination with UCA1 or with miRNA320a.
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长非编码 RNA SUMO1P3 作为监测膀胱癌进展的尿液生物标记物
尿路上皮膀胱癌(BC)是全球第九大常见癌症。膀胱癌分为非肌层浸润性膀胱癌(NMIBC)和肌层浸润性膀胱癌(MIBC),其特点分别是复发率和进展率高。诊断和监测是通过膀胱镜检查和手术后活检等侵入性方法进行的。因此,能够根据分级或分期对 BC 进行鉴别的生物标志物小组代表着患者的工作向前迈进了一大步。从这个角度来看,长非编码 RNA(lncRNA)因其表达的特异性和调节性而成为潜在生物标志物的可靠候选者。在本研究中,我们提出了两种lncRNA,即小泛素修饰因子1假基因3(SUMO1P3)(一种特征不明显的假基因)和尿路上皮癌相关1(UCA1),作为监测BC进展的候选指标。本研究是一项回顾性试验,纳入了接受手术干预的NMIBC和MIBC患者:对113名受试者(病例和对照组)尿液中lncRNA SUMO1P3和UCA1的表达进行了评估。SUMO1P3和UCA1在尿液中的表达能够显著区分低级别NMIBC、健康对照和良性前列腺增生受试者与高级别NMIBC和MIBC患者。我们还证明,与 SUMO1P3 结合的 miR-320a 在高级别 NMIBC 和 MIBC 患者中的表达量减少,SUMO1P3/miR-320a 比值可用于区分病例和对照组,在统计学上具有显著的说服力。最后,我们从临床应用的角度提供了一种自动提取 RNA 并进行 ddPCR 分析的方法。我们的研究表明,在高级别 NMIBC 和 MIBC 患者的尿液中,lncRNA SUMO1P3 增高,如果单独使用或与 UCA1 或 miRNA320a 结合使用,它很可能成为预测膀胱癌进展的良好候选物。
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