Ultrasensitive fluorescent aptasensor for CRP detection based on the RNase H assisted DNA recycling signal amplification strategy |
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| Authors: | Zhongzhi Liu Dan Luo Fangling Ren Fengying Ran Wei Chen Bingqiang Zhang Ceming Wang Hao Chen Jian Wei Qinhua Chen |
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| Affiliation: | Affiliated Dongfeng Hospital, Hubei University of Medicine, Hubei Shiyan 442008 China, +86 0719 8272283 ; College of Pharmacy, Hubei University of Medicine, Hubei Shiyan 442008 China ; Hubei Key Laboratory of Wudang Local Chinese Medicine Research, Hubei University of Medicine, Hubei Shiyan 442008 China |
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| Abstract: | An aptamer-based method for the ultrasensitive fluorescence detection of C-reactive protein (CRP) was developed using the ribonuclease H (RNase H) assisted DNA recycling signal amplification strategy. In this assay, CRP can specifically bind to the aptamer of CRP and the DNA chain of P1 is released from the aptamer/P1 (Ap/P1) complexes. After the addition of the fluorescence labeled (5-FAM) RNA, P1 hybridizes with fluorescence labeled RNA to form a P1/RNA double strand. When RNase H is added, the RNA with fluorescence labeling in the double strand is specifically cut into nucleotide fragments, which cannot be adsorbed on the surface of the GO, so as to generate a fluorescence signal. In the absence of CRP, fluorescence labeled RNA cannot hybridize with P1 to form double strands, which is able to directly adsorb on the surface of GO, resulting in no fluorescence signal. The detection limit is as low as 0.01 ng mL−1, with a linear dynamic range from 50 pg mL−1 to 100 ng mL−1. This sensor is able to detect CRP in spiked human serum, urine and saliva. Thus, it shows a great application prospect in disease diagnosis and prognosis.An aptamer-based method for the ultrasensitive fluorescence detection of C-reactive protein (CRP) was developed using the ribonuclease H (RNase H) assisted DNA recycling signal amplification strategy. |
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