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Open AccessJournal ArticleDOI

In vitro Selection of Chemically Modified DNAzymes.

Po-Jung Jimmy Huang, +1 more
- 01 Oct 2020 - 
- Vol. 9, Iss: 10, pp 1046-1059
TLDR
Examples of RNA‐cleaving DNAzymes are summarized and modifications introduced to mimic RNase A that can cleave RNA substrates in the absence of divalent metal ions are focused on.
Abstract
DNAzymes are in vitro selected DNA oligonucleotides with catalytic activities. RNA cleavage is one of the most extensively studied DNAzyme reactions. To expand the chemical functionality of DNA, various chemical modifications have been made during and after selection. In this review, we summarize examples of RNA-cleaving DNAzymes and focus on those modifications introduced during in vitro selection. By incorporating various modified nucleotides via polymerase chain reaction (PCR) or primer extension, a few DNAzymes were obtained that can be specifically activated by metal ions such as Zn2+ and Hg2+. In addition, some modifications were introduced to mimic RNase A that can cleave RNA substrates in the absence of divalent metal ions. In addition, single modifications at the fixed regions of DNA libraries, especially at the cleavage junctions, have been tested, and examples of DNAzymes with phosphorothioate and histidine-glycine modified tertiary amine were successfully obtained specific for Cu2+, Cd2+, Zn2+, and Ni2+. Labeling fluorophore/quencher pair right next to the cleavage junction was also used to obtain signaling DNAzymes for detecting various metal ions and cells. Furthermore, we reviewed work on the cleavage of 2'-5' linked RNA and L-RNA substrates. Finally, applications of these modified DNAzymes as biosensors, RNases, and biochemical probes are briefly described with a few future research opportunities outlined at the end.

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Citations
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Biosensing with DNAzymes

TL;DR: A comprehensive review of biosensing with DNAzymes, providing an overview of different sensing applications while highlighting major progress and seminal contributions to the field of portable biosensor devices and point-of-care diagnostics is provided in this paper.
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Recent progress in non-native nucleic acid modifications.

TL;DR: A review of non-native modifications and the challenges faced in the design, synthesis, application and outlook of novel modified oligonucleotides can be found in this article, where the authors provide an overview of nonnative modifications.
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A Threose Nucleic Acid Enzyme with RNA Ligase Activity.

TL;DR: The identified TNA enzyme T8-6 catalyzes the formation of a 2'-5' phosphoester bond between a 2',3'-diol and a 5'-triphosphate group, with a kobs of 1.1 × 10-2 min-1 (40 mM Mg2+, pH 9.0) as discussed by the authors.
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Porphyrin metalation catalyzed by DNAzymes and nanozymes

TL;DR: This review summarizes the progress in DNAzymes and nanozymes due to their excellent stability and low cost and reviews the applications of porphyrin metalation reactions for the detection of various metal ions, improving photocatalytic activity, and removing heavy metal ions in water.
Journal ArticleDOI

In vitro evolution of ribonucleases from expanded genetic alphabets

TL;DR: Results from comparative experiments suggest that DNA libraries with increased chemical diversity, higher information density, and larger searchable sequence spaces are one order of magnitude richer reservoirs of molecules that catalyze the cleavage of a phosphodiester bond in RNA than DNA libraries built from a standard four-nucleotide alphabet.
References
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Journal ArticleDOI

Compilation of tRNA sequences and sequences of tRNA genes

TL;DR: Alignment of the sequences, which is most compatible with the tRNA phylogeny and known three-dimensional structures of tRNA, is used.
Journal ArticleDOI

A General Purpose RNA-Cleaving DNA Enzyme

TL;DR: An in vitro selection procedure was used to develop a DNA enzyme that can be made to cleave almost any targeted RNA substrate under simulated physiological conditions, and its activity is dependent on the presence of Mg2+ ion.
Journal ArticleDOI

A DNA enzyme that cleaves RNA

TL;DR: Using in vitro selection techniques, a DNA enzyme is obtained that catalyzes the Pb(2+)-dependent cleavage of an RNA phosphoester in a reaction that proceeds with rapid turnover, and compares favorably to that of known RNA enzymes.
Journal ArticleDOI

DNAzymes for sensing, nanobiotechnology and logic gate applications

TL;DR: The use of catalytic nucleic acids for amplified biosensing was accomplished by designing aptamer-DNAzyme conjugates that combine recognition units and amplifying readout units as in integrated biosensing materials.
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