Department of Biological Sciences, St. John's University, New York, NY, USA .
Norwegian Center for Movement Disorders, Stavanger University Hospital, Stavanger, Norway.
Parkinsonism Relat Disord. 2019 Jul;64:202-210. doi: 10.1016/j.parkreldis.2019.04.010. Epub 2019 Apr 11.
As current clinical diagnostic protocols for Parkinson's disease (PD) may be prone to inaccuracies there is a need to identify and validate molecular biomarkers, such as circulating microRNAs, which will complement current practices and increase diagnostic accuracy. This study identifies, verifies and validates combinatory serum microRNA signatures as diagnostic classifiers of PD across different patient cohorts.
370 PD (drug naïve) and control serum samples from the Norwegian ParkWest study were used for identification and verification of differential microRNA levels in PD which were validated in a blind study using 64 NY Parkinsonism in UMeå (NYPUM) study serum samples and tested for specificity in 48 Dementia Study of Western Norway (DemWest) study Alzheimer's disease (AD) serum samples using miRNA-microarrays, and quantitative (q) RT-PCR. Proteomic approaches identified potential molecular targets for these microRNAs.
Using Affymetrix GeneChip miRNA 4.0 arrays and qRT-PCR we comprehensively analyzed serum microRNA levels and found that the microRNA (PARKmiR)-combinations, hsa-miR-335-5p/hsa-miR-3613-3p (95% CI, 0.87-0.94), hsa-miR-335-5p/hsa-miR-6865-3p (95% CI, 0.87-0.93), and miR-335-5p/miR-3613-3p/miR-6865-3p (95% CI, 0.87-0.94) show a high degree of discriminatory accuracy (AUC 0.9-1.0). The PARKmiR signatures were validated in an independent PD cohort (AUC ≤ 0.71) and analysis in AD serum samples showed PARKmiR signature specificity to PD. Proteomic analyses showed that the PARKmiRs regulate key PD-associated proteins, including alpha-synuclein and Leucine Rich Repeat Kinase 2.
Our study has identified and validated unique miRNA serum signatures that represent PD classifiers, which may complement and increase the accuracy of current diagnostic protocols.
由于当前帕金森病 (PD) 的临床诊断方案可能存在不准确的情况,因此需要识别和验证分子生物标志物,例如循环 microRNA,这将补充当前的实践并提高诊断准确性。本研究确定、验证和验证了组合血清 microRNA 特征作为不同患者队列中 PD 的诊断分类器。
使用来自挪威 ParkWest 研究的 370 例 PD(药物未治疗)和对照血清样本,鉴定和验证 PD 中 microRNA 水平的差异,使用 64 例 Umeå 纽约帕金森病 (NYPUM) 研究血清样本进行盲法研究验证,并在 48 例 Western Norway 痴呆症研究 (DemWest) 阿尔茨海默病 (AD) 血清样本中测试特异性,使用 miRNA 微阵列和定量 (q) RT-PCR。蛋白质组学方法鉴定了这些 microRNA 的潜在分子靶标。
使用 Affymetrix GeneChip miRNA 4.0 阵列和 qRT-PCR,我们全面分析了血清 microRNA 水平,发现 microRNA (PARKmiR)-组合,hsa-miR-335-5p/hsa-miR-3613-3p(95%CI,0.87-0.94),hsa-miR-335-5p/hsa-miR-6865-3p(95%CI,0.87-0.93)和 miR-335-5p/miR-3613-3p/miR-6865-3p(95%CI,0.87-0.94)显示出高度的区分准确性(AUC 0.9-1.0)。PARKmiR 特征在独立的 PD 队列中得到验证(AUC≤0.71),并且在 AD 血清样本中的分析表明 PARKmiR 特征对 PD 具有特异性。蛋白质组学分析表明,PARKmiRs 调节关键的 PD 相关蛋白,包括 alpha-synuclein 和 Leucine Rich Repeat Kinase 2。
我们的研究已经确定和验证了独特的 miRNA 血清特征,这些特征代表 PD 分类器,这可能补充并提高当前诊断方案的准确性。
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