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Methylation-Powered Assembly of a Single Quantum Dot-Based FRET Nanosensor for Antibody-Free and Enzyme-Free Monitoring of Locus-Specific N 6 -Methyladenosine in Clinical Tissues.

Jinping HuYa-Ting ZhangYun HanFei MaChen-Zhong LiLin CuiShuangshuang Zhang
Published in: Analytical chemistry (2023)
N 6 -Methyladenosine (m 6 A) is the most pervasive and evolutionarily conserved epitranscriptomic modification in long noncoding RNA (lncRNA), and its dysregulation may induce aberrant transcription and translation programs. Herein, we demonstrate the methylation-powered assembly of a single quantum dot (QD)-based fluorescence resonance energy transfer (FRET) nanosensor for antibody- and enzyme-free monitoring of locus-specific m 6 A in clinical tissues. The m 6 A-sensitive DNAzyme VMC10 is employed to identify a specific m 6 A site in lncRNA, and it catalyzes the hydrolytic cleavage of unmethylated lncRNA. The cleaved lncRNA fails to trigger the subsequent catalytic hairpin assembly (CHA) reaction due to the energy barrier. In contrast, when m 6 A-lncRNA is present, the methyl group in m 6 A protects lncRNA from VMC10-mediated cleavage. With the aid of an assistant probe, the retained intact m 6 A-lncRNA is released from the VMC10/lncRNA complex and subsequently triggers the CHA reaction, generating abundant AF647/biotin dual-labeled duplexes. The assembly of AF647/biotin dual-labeled duplexes onto 605QD results in efficient FRET between 605QD and AF647. The FRET signal can be simply quantified by single-molecule detection. Notably, this assay can be implemented in an antibody-free and enzyme-free manner. This nanosensor can sensitively quantify target m 6 A with a detection limit of 0.47 fM, and it can discriminate as low as a 0.001% m 6 A level from excess coexisting counterparts. Importantly, this nanosensor can monitor the cellular m 6 A level with single-cell sensitivity and profile target m 6 A expression in breast cancer and healthy para-cancerous tissues, providing a powerful tool for studying the physiological and pathological functions of m 6 A.
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