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Literature DB >> 16957279

An accurate fluorescent assay for quantifying the extent of RNA editing.

Loretta M Roberson¹, Joshua J C Rosenthal.

Abstract

Recent data suggest that small differences in editing efficiency can have significant functional consequences. Here we present a fluorescent poisoned primer extension assay that is capable of distinguishing editing efficiency differences as low as 5%. For a poison-primer extension assay to be accurate, the extension product must stop at the intended base. Sometimes, however, it runs beyond. We tested the effect of specific enzyme-terminator combinations on the amount of run through. In the worst cases it accounted for 70% of the total signal, and in the best cases <5%. In addition, the specific base can affect run through, with G producing the least. The accuracy of the assay was demonstrated on templates derived from mixed plasmids and then verified on two biological substrates. Using either a K(+) channel mRNA that contains a site for adenosine deamination or an ndhB mRNA that contains a site for cytidine deamination, the editing efficiency predicted by the assay closely matched that predicted by bulk sequencing of individual cDNA clones. This assay should prove useful for analyzing small changes in editing efficiency or for quantifying single nucleotide polymorphisms.

Entities: Chemical

Mesh：

Substances：

Year: 2006 PMID： 16957279 PMCID： PMC1581973 DOI： 10.1261/rna.166906

Source DB: PubMed Journal: RNA ISSN： 1355-8382 Impact factor: 4.942

32 in total

1. A quantitative method to detect RNA editing events.

Authors: H H Schiffer; S F Heinemann
Journal: Anal Biochem Date: 1999-12-15 Impact factor: 3.365

2. Comparative analysis of RNA editing sites in higher plant chloroplasts.

Authors: T Tsudzuki; T Wakasugi; M Sugiura
Journal: J Mol Evol Date: 2001 Oct-Nov Impact factor: 2.395

3. RNA editing of the 5-HT(2C) receptor is reduced in schizophrenia.

Authors: M S Sodhi; P W Burnet; A J Makoff; R W Kerwin; P J Harrison
Journal: Mol Psychiatry Date: 2001-07 Impact factor: 15.992

4. Transcript abundance supercedes editing efficiency as a factor in developmental variation of chloroplast gene expression.

Authors: Nemo M Peeters; Maureen R Hanson
Journal: RNA Date: 2002-04 Impact factor: 4.942

5. Extensive editing of mRNAs for the squid delayed rectifier K+ channel regulates subunit tetramerization.

Authors: Joshua J C Rosenthal; Francisco Bezanilla
Journal: Neuron Date: 2002-05-30 Impact factor: 17.173

6. Editing of plastid RNA in Arabidopsis thaliana ecotypes.

Authors: Michael Tillich; Helena T Funk; Christian Schmitz-Linneweber; Peter Poltnigg; Bartolomé Sabater; Mercedes Martin; Rainer M Maier
Journal: Plant J Date: 2005-09 Impact factor: 6.417

7. Altered editing of serotonin 2C receptor pre-mRNA in the prefrontal cortex of depressed suicide victims.

Authors: Ilona Gurevich; Hadassah Tamir; Victoria Arango; Andrew J Dwork; J John Mann; Claudia Schmauss
Journal: Neuron Date: 2002-04-25 Impact factor: 17.173

8. The role of RNA editing of kainate receptors in synaptic plasticity and seizures.

Authors: B Vissel; G A Royle; B R Christie; H H Schiffer; A Ghetti; T Tritto; I Perez-Otano; R A Radcliffe; J Seamans; T Sejnowski; J M Wehner; A C Collins; S O'Gorman; S F Heinemann
Journal: Neuron Date: 2001-01 Impact factor: 17.173

9. RNA hairpins in noncoding regions of human brain and Caenorhabditis elegans mRNA are edited by adenosine deaminases that act on RNA.

Authors: Daniel P Morse; P Joseph Aruscavage; Brenda L Bass
Journal: Proc Natl Acad Sci U S A Date: 2002-06-04 Impact factor: 11.205

10. RNA editing of serotonin 2C receptor in human postmortem brains of major mental disorders.

Authors: Kazuya Iwamoto; Tadafumi Kato
Journal: Neurosci Lett Date: 2003-08-07 Impact factor: 3.046

11 in total

1. Substitution of the use of radioactivity by fluorescence for biochemical studies of RNA.

Authors: Bei-Wen Ying; Dominique Fourmy; Satoko Yoshizawa
Journal: RNA Date: 2007-09-11 Impact factor: 4.942

2. A conserved glutamate residue in the C-terminal deaminase domain of pentatricopeptide repeat proteins is required for RNA editing activity.

Authors: Michael L Hayes; Kim N Dang; Michael F Diaz; R Michael Mulligan
Journal: J Biol Chem Date: 2015-03-04 Impact factor: 5.157

3. An Organelle RNA Recognition Motif Protein Is Required for Photosystem II Subunit psbF Transcript Editing.

Authors: Justin B Hackett; Xiaowen Shi; Amy T Kobylarz; Meriah K Lucas; Ryan L Wessendorf; Kevin M Hines; Stephane Bentolila; Maureen R Hanson; Yan Lu
Journal: Plant Physiol Date: 2017-02-17 Impact factor: 8.340

4. Stable native RIP9 complexes associate with C-to-U RNA editing activity, PPRs, RIPs, OZ1, ORRM1 and ISE2.

Authors: Rafael Sandoval; Robert D Boyd; Alena N Kiszter; Yeva Mirzakhanyan; Paola Santibańez; Paul D Gershon; Michael L Hayes
Journal: Plant J Date: 2019-06-26 Impact factor: 6.417

5. RNA editing underlies temperature adaptation in K+ channels from polar octopuses.

Authors: Sandra Garrett; Joshua J C Rosenthal
Journal: Science Date: 2012-01-05 Impact factor: 47.728

6. Regulation of Na+/K+ ATPase transport velocity by RNA editing.

Authors: Claudia Colina; Juan Pablo Palavicini; Deepa Srikumar; Miguel Holmgren; Joshua J C Rosenthal
Journal: PLoS Biol Date: 2010-11-23 Impact factor: 8.029

7. A comparative genomics approach identifies a PPR-DYW protein that is essential for C-to-U editing of the Arabidopsis chloroplast accD transcript.

Authors: John C Robbins; Wade P Heller; Maureen R Hanson
Journal: RNA Date: 2009-04-24 Impact factor: 4.942