Literature DB >> 27645507

Boronate affinity electrophoresis for the purification and analysis of cofactor-modified RNAs.

Gabriele Nübel1, Frieda A Sorgenfrei2, Andres Jäschke3.   

Abstract

RNA modifications are widely distributed in Nature, and their thorough analysis helps answering fundamental biological questions. Nowadays, mass spectrometry or deep-sequencing methods are often used for the analysis. With the raising number of newly discovered RNA modifications, such as the 5'-NAD cap in Escherichia coli, there is an important need for new, less complex and fast analytical tools to analyze the occurrence, amount, and distribution of modified RNAs in cells. To accomplish this task, we have revisited the previously developed affinity gel electrophoresis principles and copolymerized acryloylaminophenyl boronic acid (APB) in standard denaturing polyacrylamide gels to retard the NAD- or FAD-modified RNAs compared to the unmodified RNAs in the gels. The boronyl groups inside the gel form relatively stable complexes with 1,2-cis diols, occurring naturally at the 3'-end of RNA, and also in the nicotinamide riboside of NAD-modified RNA at the 5'-end. The transient formation of diesters between the immobilized boronic acid and the diols causes lower mobility of the modified RNAs, compared to unmodified RNAs, resulting in two distinct bands for one RNA sequence. We used APB affinity gel electrophoresis to preparatively purify in vitro transcribed NAD-RNA from triphosphorylated RNA, to study the enzyme kinetics of the NAD-RNA decapping enzyme NudC, and to determine the NAD modification ratios of various cellular sRNAs. In summary, APB affinity gels can be used to study cofactor-modified RNAs with low amounts of material, and to rapidly screen for their occurrence in total RNA while avoiding complex sample treatments.
Copyright © 2016 Elsevier Inc. All rights reserved.

Entities:  

Keywords:  Affinity electrophoresis; Boronic acid; FAD; FAD-RNA; NAD; NAD-RNA; RNA modification

Mesh:

Substances:

Year:  2016        PMID: 27645507     DOI: 10.1016/j.ymeth.2016.09.008

Source DB:  PubMed          Journal:  Methods        ISSN: 1046-2023            Impact factor:   3.608


  13 in total

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Authors:  Hector Gabriel Morales-Filloy; Yaqing Zhang; Gabriele Nübel; Shilpa Elizabeth George; Natalya Korn; Christiane Wolz; Andres Jäschke
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2.  CapZyme-Seq Comprehensively Defines Promoter-Sequence Determinants for RNA 5' Capping with NAD<sup/>.

Authors:  Irina O Vvedenskaya; Jeremy G Bird; Yuanchao Zhang; Yu Zhang; Xinfu Jiao; Ivan Barvík; Libor Krásný; Megerditch Kiledjian; Deanne M Taylor; Richard H Ebright; Bryce E Nickels
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3.  SPAAC-NAD-seq, a sensitive and accurate method to profile NAD+-capped transcripts.

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4.  Is mRNA decapping by ApaH like phosphatases present in eukaryotes beyond the Kinetoplastida?

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Journal:  RNA Biol       Date:  2016-11-30       Impact factor: 4.652

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Authors:  Jeremy G Bird; Urmimala Basu; David Kuster; Aparna Ramachandran; Ewa Grudzien-Nogalska; Atif Towheed; Douglas C Wallace; Megerditch Kiledjian; Dmitry Temiakov; Smita S Patel; Richard H Ebright; Bryce E Nickels
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Review 7.  RNA Modifications in Pathogenic Bacteria: Impact on Host Adaptation and Virulence.

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8.  CapZyme-Seq: A 5'-RNA-Seq Method for Differential Detection and Quantitation of NAD-Capped and Uncapped 5'-Triphosphate RNA.

Authors:  Irina O Vvedenskaya; Bryce E Nickels
Journal:  STAR Protoc       Date:  2020-06-03

9.  DXO/Rai1 enzymes remove 5'-end FAD and dephospho-CoA caps on RNAs.

Authors:  Selom K Doamekpor; Ewa Grudzien-Nogalska; Agnieszka Mlynarska-Cieslak; Joanna Kowalska; Megerditch Kiledjian; Liang Tong
Journal:  Nucleic Acids Res       Date:  2020-06-19       Impact factor: 16.971

10.  A Novel NAD-RNA Decapping Pathway Discovered by Synthetic Light-Up NAD-RNAs.

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Journal:  Biomolecules       Date:  2020-03-28
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