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一种基于结合触发的杂交链式反应级联多靶激活 CRISPR/Cas12a 信号放大策略,用于灵敏检测 α-突触核蛋白。

A binding-triggered hybridization chain reaction cascade multi-site activated CRISPR/Cas12a signal amplification strategy for sensitive detection of α-synuclein.

机构信息

School of Chemistry and Chemical Engineering, Shandong University, 250100, Jinan, PR China.

Department of Oncology, Central Hospital Affiliated to Shandong First Medical University, 250013, Jinan, PR China.

出版信息

Analyst. 2024 Jul 8;149(14):3725-3731. doi: 10.1039/d4an00453a.

Abstract

Alpha-synuclein (α-syn) is closely related to the pathological process of Parkinson's disease (PD). Sensitive detection of α-syn is important for the early diagnosis and disease progression monitoring of PD. Herein, we report a binding-triggered hybridization chain reaction (HCR) cascade multi-site activated CRISPR/Cas12a signal amplification strategy for sensitive detection of α-syn. In this method, antibody-DNA capture probes recognized α-syn and bound with it to increase the local effective concentrations of two DNA strands, promoting their hybridization to form a split HCR trigger. Then the trigger initiated an HCR to generate a long double-stranded structure which contained abundant periodically repeated Cas12a/crRNA target sequences. Finally, the Cas12a/crRNA recognized the target sequence in HCR products and then the cleavage activity toward fluorescent reporters was activated, leading to the recovery of appreciable fluorescence signals. Our method provided a detection limit as low as 9.33 pM and exhibited satisfactory applicability in human serum samples. In summary, this study provides a homogeneous strategy for convenient, sensitive, and accurate detection of α-syn, showing great potential in the early diagnosis of PD.

摘要

α-突触核蛋白(α-syn)与帕金森病(PD)的病理过程密切相关。敏感检测α-syn 对于 PD 的早期诊断和疾病进展监测非常重要。在此,我们报告了一种结合触发的杂交链式反应(HCR)级联多位点激活 CRISPR/Cas12a 信号放大策略,用于敏感检测 α-syn。在该方法中,抗体-DNA 捕获探针识别α-syn 并与之结合,以增加两条 DNA 链的局部有效浓度,促进它们杂交形成分裂的 HCR 触发物。然后,触发物引发 HCR 生成包含丰富周期性重复 Cas12a/crRNA 靶序列的长双链结构。最后,Cas12a/crRNA 识别 HCR 产物中的靶序列,然后激活对荧光报告物的切割活性,导致可观的荧光信号恢复。我们的方法提供了低至 9.33 pM 的检测限,并在人血清样本中表现出令人满意的适用性。总之,本研究为方便、敏感和准确地检测 α-syn 提供了一种均相策略,在 PD 的早期诊断中显示出巨大的潜力。

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