4.7 Article

Determination of RNase H activity via real-time monitoring of target-triggered rolling circle amplification

Journal

MICROCHIMICA ACTA
Volume 185, Issue 1, Pages -

Publisher

SPRINGER WIEN
DOI: 10.1007/s00604-017-2610-8

Keywords

DNA; Enzyme; Isothermal nucleic acid amplification; DNA polymerase; Primer; Amino group; SYBR green II dye; Fluorescent biosensors

Funding

  1. National Research Foundation (NRF) - Ministry of Science, ICT and Future planning (MSIP) of Korea [2015R1A2A1A01005393]
  2. Center for BioNano Health-Guard - MSIP of Korea [H-GUARD_2013M3A6B2078964]
  3. NRF - MSIP of Korea [2017R1C1B5017724]

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The authors describe a method for real-time monitoring of the activity of ribonuclease H (RNase H). It is based on target-triggered rolling circle amplification (RCA). It utilizes a specially designed primer that contains a RNA sequence in the center and an amino group at the 3'-end. In the absence of RNase H, the primer when hybridized to a circular DNA template is not extended by DNA polymerase due to the amino group at the 3'-end. In contrast, the presence of RNase H specifically degrades the RNA sequence of the primer hybridized to the circular DNA template. This results in the conversion of the 3'-amino group to a 3'-hydroxy group and thereby enables the extension reaction promoted by DNA polymerase. This, consequently, leads to efficient RCA producing a long concatenated DNA strand. Its generation can be monitored in real-time by using the fluorescent dye SYBR green II which is specific for single-stranded DNA. Based on this RNase H-triggered RCA, RNase H activity can be selectively determined at levels as low as 0.019 U.mL(-1) with a total assay time of <5 min. The diagnostic capability of this assay was demonstrated by monitoring the activity of RNase H in tumor cells.

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