Acoustic Levitation Synthesis of Ultrahigh‐Density Spherical Nucleic Acid Architectures for Specific SERS Analysis

Author:

Ding Zhongxiang1,Gao Heng1,Wang Chao2,Li Yuzhu1,Li Ning1,Chu Leiming1,Chen Haijie1,Xie Haijiao3,Su Mengke1,Liu Honglin1ORCID

Affiliation:

1. Key Laboratory for Animal Food Green Manufacturing and Resource Mining of Anhui Province, China Light Industry Key Laboratory of Meat Microbial Control and Utilization, School of Food and Biological Engineering Hefei University of Technology Hefei 230009 China

2. National Synchrotron Radiation Laboratory University of Science and Technology of China Hefei 230027 China

3. Hangzhou Yanqu Information Technology Co., Ltd. Hangzhou City, Zhejiang Province 310003 P.R.O.C., China

Abstract

AbstractControllably regulating the electrostatic bilayer of nanogold colloids is a significant premise for synthesizing spherical nucleic acid (SNA) and building ordered plasmonic architectures. We develop a facile acoustic levitation reactor to universally synthesize SNAs with an ultra‐high density of DNA strands, which is even higher than those of various state‐of‐the‐art methods. Results reveal a new mechanism of DNA grafting via acoustic wave that can reconfigure the ligands on colloidal surfaces. The acoustic levitation reactor enables substrate‐free three‐dimentional (3D) spatial assembly of SNAs with controllable interparticle nanogaps through regulating DNA lengths. This kind of architecture may overcome the plasmonic enhancement limits by blocking electron tunneling and breaking electrostatic shielding in dried aggregations. Finite element simulations support the architecture with 3D spatial plasmonic hotspot matrix, and its ultrahigh surface‐enhanced Raman scattering (SERS) capability is evidenced by in situ untargeted tracking of biomolecular events during photothermal stimulation (PTS)‐induced cell death process. For biomarker diagnosis, the conjugation of adenosine triphosphate (ATP) aptamer onto SNAs enables in situ targeted tracking of ATP during PTS‐induced cell death process. Particularly, the CD71 receptor and integrin α3β1 protein on PL45 cell membrance could be well distinguished by label‐free SERS fingerprints when using specific XQ‐2d and DML‐7 aptamers, respectively, to synthesize SNA architectures. Our current acoustic levitation reactor offers a new method for synthesizing SNAs and enables both targeted and untargeted SERS analysis for tracking molecular events in living systems. It promises great potentials in biochemical synthesis and sensing in future.

Funder

National Natural Science Foundation of China

Fundamental Research Funds for the Central Universities

Publisher

Wiley

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