In-particle stem-loop RT-qPCR for specific and multiplex microRNA profiling

Authors
Jung, SeungwonKim, Won JinKim, Bong KyunKim, JunsunKim, Mi JungKim, Kwang PyoKim, Sang Kyung
Issue Date
2020-09-01
Publisher
ELSEVIER ADVANCED TECHNOLOGY
Citation
BIOSENSORS & BIOELECTRONICS, v.163
Abstract
Here we report a novel method of microRNA (miRNA) profiling with particle-based multiplex quantitative reverse transcription polymerase chain reaction (RT-qPCR). To achieve target-specific reaction in a particle, the stem-loop RT primer and forward primer for each target miRNA were chemically immobilized to the particle. Target-specific cDNA synthesis proceeds with the stem-loop RT primer and then qPCR subsequently proceeds with the forward primer to rapidly achieve a quantitative result. High-fidelity multiplex assay was also accomplished in a single PCR process by loading multiple particles for each specific miRNA. The method for primer supply in the particles, involving confinement of the target-specific RT and PCR primers in the matrix of particles, led to the reduction of nonspecific reactions and improved the selectivity of the miRNA assay while minimizing labor in a multiple target assay. Specifically, this particle-based assay enabled the differentiation of mature miRNA from precursor with selectivity of 270:1 in terms of amplification speed. This advanced method also showed good discrimination among highly homologous let-7 family members, with cross-reaction rates of less than 5%. We demonstrated a very simple process of five-plex miRNA profiling in total RNA, and the measured changes in expression level were consistent with those from a conventional singleplex method.
Keywords
SMALL RNAS; EXPRESSION; PCR; QUANTIFICATION; SMALL RNAS; EXPRESSION; PCR; QUANTIFICATION; microRNA; Quantitative reverse-transcription PCR; Stem-loop reverse transcription; Hydrogel; Multiplex assay
ISSN
0956-5663
URI
https://pubs.kist.re.kr/handle/201004/118142
DOI
10.1016/j.bios.2020.112301
Appears in Collections:
KIST Article > 2020
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