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用于前列腺癌预后的液体活检中YAP1核酸、AR-FL和AR-V7 mRNA的手持式ISFET芯片实验室检测

Handheld ISFET Lab-on-Chip detection of YAP1 nucleic acid and AR-FL and AR-V7 mRNA from liquid biopsies for prostate cancer prognosis.

作者信息

Broomfield Joseph, Kalofonou Melpomeni, Gulli Costanza, Powell Sue M, Fernandes Rayzel C, Leach Damien A, Moser Nicolas, Sarwar Naveed, Mangar Stephen, Bevan Charlotte L, Georgiou Pantelis

机构信息

Centre for Bio-Inspired Technology, Department of Electrical and Electronic Engineering, Imperial College London, London, SW7 2AZ, United Kingdom; Imperial Centre for Translational and Experimental Medicine, Department of Surgery and Cancer, Imperial College London, London, W12 0NN, United Kingdom.

Centre for Bio-Inspired Technology, Department of Electrical and Electronic Engineering, Imperial College London, London, SW7 2AZ, United Kingdom.

出版信息

Biosens Bioelectron. 2025 Aug 1;281:117407. doi: 10.1016/j.bios.2025.117407. Epub 2025 Apr 8.

Abstract

Prostate cancer (PCa) is a highly prevalent disease, causing the second largest amount of male cancer deaths worldwide. Currently, the prostate specific antigen (PSA) test remains the standard serum prognostic and diagnostic monitoring biomarker but it lacks specificity and sensitivity. PSA testing can lead to invasive biopsies which can result in under detection of clinically significant disease and potential overtreatment of indolent disease. Promising circulating biomarkers could facilitate less invasive and more accurate tests, but present challenges in robust quantitation and deployment in clinical settings. This work presents the detection of circulating YAP1 nucleic acid, androgen receptor (AR-FL) and AR-V7 mRNA for PCa prognostics in blood plasma from PCa patients. Sensitive detection of circulating YAP1 nucleic acid, AR-FL and AR-V7 mRNA extracted from PCa clinical samples was achieved with a reverse transcription loop-mediated isothermal amplification (RT-LAMP) assay. Optimisation of mRNA extraction methodologies for reliable detection of circulating mRNA for RT-LAMP and RT-qPCR detection took place. Multiplex testing of circulating AR-FL mRNA and YAP1 nucleic acid on an ISFET Lab-on-Chip platform was readily achieved with bio-electronic signal detection taking place within 15 min. Detection of AR-V7 and AR-FL mRNA could also be achieved simultaneously with the handheld device. Evaluation of clinical data indicated that circulating YAP1 nucleic acid presence in extracted RNA from the blood plasma of patients correlated with more advanced clinical cancer staging (p = 0.043) and PSA at diagnosis (p = 0.035). The work presents potential for Point-of-Care detection of circulating mRNA from clinical samples for PCa prognostics.

摘要

前列腺癌(PCa)是一种高度常见的疾病,在全球男性癌症死亡原因中位列第二。目前,前列腺特异性抗原(PSA)检测仍是标准的血清预后和诊断监测生物标志物,但它缺乏特异性和敏感性。PSA检测可能导致侵入性活检,这可能会导致临床显著疾病的漏诊以及惰性疾病的潜在过度治疗。有前景的循环生物标志物可以促进侵入性更小、更准确的检测,但在可靠定量和临床应用方面存在挑战。这项工作展示了在前列腺癌患者血浆中检测循环YAP1核酸、雄激素受体(AR-FL)和AR-V7 mRNA用于前列腺癌预后评估。通过逆转录环介导等温扩增(RT-LAMP)测定法,实现了对从前列腺癌临床样本中提取的循环YAP1核酸、AR-FL和AR-V7 mRNA的灵敏检测。对mRNA提取方法进行了优化,以实现对用于RT-LAMP和RT-qPCR检测的循环mRNA的可靠检测。在ISFET芯片实验室平台上对循环AR-FL mRNA和YAP1核酸进行多重检测很容易实现,生物电信号检测在15分钟内即可完成。使用手持设备也可以同时检测AR-V7和AR-FL mRNA。临床数据评估表明,患者血浆提取RNA中循环YAP1核酸的存在与更晚期的临床癌症分期(p = 0.043)和诊断时的PSA水平(p = 0.035)相关。这项工作展示了从临床样本中即时检测循环mRNA用于前列腺癌预后评估的潜力。

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