Literature DB >> 25352138

Native purification and labeling of RNA for single molecule fluorescence studies.

Arlie J Rinaldi1, Krishna C Suddala, Nils G Walter.   

Abstract

The recent discovery that non-coding RNAs are considerably more abundant and serve a much wider range of critical cellular functions than recognized over previous decades of research into molecular biology has sparked a renewed interest in the study of structure-function relationships of RNA. To perform their functions in the cell, RNAs must dominantly adopt their native conformations, avoiding deep, non-productive kinetic traps that may exist along a frustrated (rugged) folding free energy landscape. Intracellularly, RNAs are synthesized by RNA polymerase and fold co-transcriptionally starting from the 5' end, sometimes with the aid of protein chaperones. By contrast, in the laboratory RNAs are commonly generated by in vitro transcription or chemical synthesis, followed by purification in a manner that includes the use of high concentrations of urea, heat and UV light (for detection), resulting in the denaturation and subsequent refolding of the entire RNA. Recent studies into the nature of heterogeneous RNA populations resulting from this process have underscored the need for non-denaturing (native) purification methods that maintain the co-transcriptional fold of an RNA. Here, we present protocols for the native purification of an RNA after its in vitro transcription and for fluorophore and biotin labeling methods designed to preserve its native conformation for use in single molecule fluorescence resonance energy transfer (smFRET) inquiries into its structure and function. Finally, we present methods for taking smFRET data and for analyzing them, as well as a description of plausible overall preparation schemes for the plethora of non-coding RNAs.

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Year:  2015        PMID: 25352138      PMCID: PMC4254587          DOI: 10.1007/978-1-4939-1896-6_6

Source DB:  PubMed          Journal:  Methods Mol Biol        ISSN: 1064-3745


  83 in total

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Journal:  Methods       Date:  2011-02-24       Impact factor: 3.608

8.  Biotin and fluorescent labeling of RNA using T4 RNA ligase.

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Journal:  Nucleic Acids Res       Date:  1983-09-24       Impact factor: 16.971

9.  Conformational capture of the SAM-II riboswitch.

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  10 in total

1.  Riboswitch structure and dynamics by smFRET microscopy.

Authors:  Krishna C Suddala; Nils G Walter
Journal:  Methods Enzymol       Date:  2014       Impact factor: 1.600

Review 2.  Coming Together: RNAs and Proteins Assemble under the Single-Molecule Fluorescence Microscope.

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3.  In vitro labeling strategies for in cellulo fluorescence microscopy of single ribonucleoprotein machines.

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Journal:  Protein Sci       Date:  2017-02-12       Impact factor: 6.725

4.  Single-Molecule Pull-Down FRET to Dissect the Mechanisms of Biomolecular Machines.

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Journal:  Methods Enzymol       Date:  2015-03-03       Impact factor: 1.600

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Journal:  Nucleic Acids Res       Date:  2021-06-04       Impact factor: 16.971

Review 6.  Thermostability, Tunability, and Tenacity of RNA as Rubbery Anionic Polymeric Materials in Nanotechnology and Nanomedicine-Specific Cancer Targeting with Undetectable Toxicity.

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8.  Amine-to-Azide Conversion on Native RNA via Metal-Free Diazotransfer Opens New Avenues for RNA Manipulations.

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9.  Diversity of bacterial small RNAs drives competitive strategies for a mutual chaperone.

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  10 in total

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