4.8 Article

Controllable design of a nano-bio aptasensing interface based on tetrahedral framework nucleic acids in an integrated microfluidic platform

期刊

BIOSENSORS & BIOELECTRONICS
卷 176, 期 -, 页码 -

出版社

ELSEVIER ADVANCED TECHNOLOGY
DOI: 10.1016/j.bios.2020.112943

关键词

Tetrahedral DNA nanostructure; Pathogenic microorganism; Aptasensor; Antibiotic resistance; Food safety detection

资金

  1. National Natural Science Foundation of China [21775102, 21775104]
  2. Natural Science Foundation of Shanghai Municipal [20ZR1424100, 19ZR1422900]
  3. Agricultural Science and Technology Innovation Program of CAAS [CAAS-ZDRW202009]
  4. National Quality Infrastructure Program of China [2018YFF0212800]

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This study investigates the self-assembling of tetrahedral framework nucleic acids in microfluidic devices, creating a three-dimensional reaction space at nanoscale and improving reaction kinetics during molecular recognition. The novel FNA-engineered microfluidic interface enables a one-stop assay of E. coli O157:H7 with high bacterial detection efficiency, selectivity, and precision. The application of the FNA interface shows promising potential for developing microfluidic biosensors for other pathogenic microorganisms or circulating tumor cells by changing the aptamers.
The limited reaction time and sample volume in the confined space of microfluidic devices give considerable importance to the development of more effective biosensing interfaces. Herein, the self-assembling of tetrahedral framework nucleic acids (FNAs) with controllable size on the interface of the microfluidic microchannels is studied. Compared with macroscopic turbulence control on traditional micro-structured microfluidic surface, the novel FNA-engineered microfluidic interface successfully constructs a 3D reaction space at nanoscale by raising DNA probes away from the surface. This FNA interface dramatically improves the reaction kinetics during molecular recognition due to extremely ordered orientation, configuration and density of DNA probes on the surface. Finally, the FNA-engineered interface is applied in a novel multi-functional microfluidic platform, towards a one-stop assay of Escherichia coli O157: H7 (E. coli O157: H7), integrating capture, release, enrichment, cell culture and antimicrobial susceptibility testing (AST). With the FNA-aptamer probe, we achieved an enhanced bacterial detecting efficiency (10 CFU/mL) plus excellent selectivity and precision. The appicability was strongly demonstrated when the biosensor was successfully applied in real samples, including the analysis of antibiotic susceptibility and minimum inhibitory concentration (MIC) of E. coli O157: H7 among different antibiotics. The application of FNA interface will open a wide avenue for the development of microfluidic biosensors for other pathogenic microorganisms or circulating tumor cells (CTC) simply by changing the aptamers.

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