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多种外切酶 III 辅助循环扩增单元的紧密集成用于 MRSA 的高效比率型电化学发光检测。

The Compact Integration of Multiple Exonuclease III-Assisted Cyclic Amplification Units for High-Efficiency Ratiometric Electrochemiluminescence Detection of MRSA.

机构信息

School of Chemistry and Chemical Engineering, Anhui University of Technology, Ma Xiang Road, Ma 'anshan, Anhui 243032, PR China.

Key Laboratory of Optic-electric Sensing and Analytical Chemistry for Life Science, MOE, Qingdao University of Science and Technology, Qingdao 266042, PR China.

出版信息

Anal Chem. 2024 Jan 16;96(2):943-948. doi: 10.1021/acs.analchem.3c05410. Epub 2024 Jan 2.

DOI:10.1021/acs.analchem.3c05410
PMID:38166359
Abstract

Methicillin-resistant (MRSA) exhibits multiresistance to a plethora of antibiotics, therefore, accurate detection methods must be employed for timely identification to facilitate effective infection control measures. Herein, we construct a high-efficiency ratiometric electrochemiluminescent (ECL) biosensor that integrates multiple exonuclease (Exo) III-assisted cyclic amplification units for rapid detection of trace amounts of MRSA. The target bacteria selectively bind to the aptamer, triggering the release of two single-stranded DNAs. One released DNA strand initiates the opening of a hairpin probe, inducing exonuclease cleavage to generate a single strand that can form a T-shaped structure with the double strand connecting the oxidation-reduction (O-R) emitter of -(4-aminobutyl)--ethylisoluminol gold (ABEI-Au). Consequently, ABEI-Au is released upon Exo III cleavage. The other strand unwinds the hairpin DNA structure on the surface of the reduction-oxidation (R-O) emitter ZIF-8@CdS, facilitating the subsequent release of a specific single strand through Exo III cleavage. This process effectively anchors the cathode-emitting material to the electrode. The Fe(III) metal-organogel (Fe-MOG) is selected as a substrate, in which the catalytic reduction of hydrogen peroxide by Fe(III) active centers accelerates the generation of reactive oxygen species and enhances signals from both ABEI-Au and ZIF-8@CdS. In this way, the two emitters cooperate to achieve bacterial detection at the single-cell level, and a good linear range is obtained in the range of 10-10 CFU/mL. Moreover, the sensor exhibited excellent performance in detecting MRSA across various authentic samples and accurately quantifying MRSA levels in serum samples, demonstrating its immense potential in addressing clinical bacterial detection challenges.

摘要

耐甲氧西林金黄色葡萄球菌(MRSA)对多种抗生素表现出多重耐药性,因此必须采用准确的检测方法进行及时鉴定,以利于采取有效的感染控制措施。在此,我们构建了一种高效的比率型电化学发光(ECL)生物传感器,该传感器集成了多个外切酶(Exo)III 辅助循环扩增单元,用于快速检测痕量 MRSA。目标细菌选择性地与适体结合,触发两种单链 DNA 的释放。其中一条释放的 DNA 链启动发夹探针的打开,诱导外切酶切割产生一条单链,该单链可以与连接氧化还原(O-R)发射体的双链形成 T 型结构-(4-氨基丁基)--乙基异鲁米诺金(ABEI-Au)。因此,ABEI-Au 在 Exo III 切割时被释放。另一条链解开表面还原氧化(R-O)发射体 ZIF-8@CdS 上的发夹 DNA 结构,通过 Exo III 切割促进特定单链的后续释放。这一过程有效地将阴极发射材料锚定在电极上。Fe(III) 金属有机凝胶(Fe-MOG)被选为基底,其中 Fe(III) 活性中心催化过氧化氢还原加速活性氧物质的生成,并增强 ABEI-Au 和 ZIF-8@CdS 的信号。这样,两个发射器在单细胞水平上协同进行细菌检测,并在 10-10 CFU/mL 的范围内获得良好的线性范围。此外,该传感器在检测各种真实样本中的 MRSA 方面表现出优异的性能,并能够准确定量血清样本中的 MRSA 水平,表明其在解决临床细菌检测挑战方面具有巨大的潜力。

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