Literature DB >> 11553468

2-Aminopurine as a real-time probe of enzymatic cleavage and inhibition of hammerhead ribozymes.

S R Kirk1, N W Luedtke, Y Tor.   

Abstract

The design, synthesis and study of internally fluorescent hammerhead (HH) ribozymes, where changes in fluorescence parameters directly reflect the progress of the ribozyme's cleavage chemistry, are described. The approach relies on a HH substrate modified at position 1.1, proximal to the cleavage site, with 2-aminopurine (2AP), an intensely fluorescent adenosine isoster. The incorporation of 2AP, an unnatural nucleoside, does not interfere with the ribozyme folding and catalysis. Since 2AP is highly sensitive to environmental changes, its fluorescence is dramatically altered upon ribozyme-mediated cleavage of the substrate. This generates a measurable signal that directly reflects the progress of the ribozyme's reaction in real time. Identical pseudo first order rate constants are obtained for HH constructs using both continuous fluorescence monitoring and radioactive labeling. This rapid and real-time monitoring facilitates the study of ribozyme activity under different conditions (e.g., ionic strength, pH, etc.), and provides a useful assay to rapidly screen potential inhibitors. Three hitherto unknown HH inhibitors are presented and compared to neomycin B and chlortetracycline, two previously studied HH inhibitors. All three new small molecules, neo-acridine, guanidino-neomycin B, and [Delta-(Eilatin)Ru(bpy)(2)](2+), prove to be better inhibitors than neomycin B or chlortetracycline. Investigating HH inhibition under different ionic strengths reveals that the binding of neo-acridine, [Delta-(Eilatin)Ru(bpy)(2)](2+), and chlortetracycline to the HH involves hydrophobic interactions as their RNA affinities are largely unaffected by increasing salt concentrations. In contrast, neomycin B loses more than 50-fold of its inhibitory ability as the NaCl concentration is increased from 50 to 500mM.

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Year:  2001        PMID: 11553468     DOI: 10.1016/s0968-0896(01)00123-7

Source DB:  PubMed          Journal:  Bioorg Med Chem        ISSN: 0968-0896            Impact factor:   3.641


  20 in total

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2.  Fluorescent pyrimidine ribonucleotide: synthesis, enzymatic incorporation, and utilization.

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Review 3.  Fluorescent analogs of biomolecular building blocks: design, properties, and applications.

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Journal:  Chem Rev       Date:  2010-05-12       Impact factor: 60.622

4.  Polymerase-Mediated Site-Specific Incorporation of a Synthetic Fluorescent Isomorphic G Surrogate into RNA.

Authors:  Yao Li; Andrea Fin; Lisa McCoy; Yitzhak Tor
Journal:  Angew Chem Int Ed Engl       Date:  2016-12-21       Impact factor: 15.336

5.  Emissive RNA alphabet.

Authors:  Dongwon Shin; Renatus W Sinkeldam; Yitzhak Tor
Journal:  J Am Chem Soc       Date:  2011-09-02       Impact factor: 15.419

Review 6.  Fluorescent nucleobases as tools for studying DNA and RNA.

Authors:  Wang Xu; Ke Min Chan; Eric T Kool
Journal:  Nat Chem       Date:  2017-10-16       Impact factor: 24.427

7.  Enzymatic incorporation of emissive pyrimidine ribonucleotides.

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Journal:  Chem Asian J       Date:  2009-03-02

8.  Ligand-induced changes in 2-aminopurine fluorescence as a probe for small molecule binding to HIV-1 TAR RNA.

Authors:  Thomas D Bradrick; John P Marino
Journal:  RNA       Date:  2004-07-23       Impact factor: 4.942

Review 9.  Covalent labeling of nucleic acids.

Authors:  Nils Klöcker; Florian P Weissenboeck; Andrea Rentmeister
Journal:  Chem Soc Rev       Date:  2020-10-21       Impact factor: 54.564

10.  Fluorescence probing of T box antiterminator RNA: insights into riboswitch discernment of the tRNA discriminator base.

Authors:  John A Means; Crystal M Simson; Shu Zhou; Aaron A Rachford; Jeffrey J Rack; Jennifer V Hines
Journal:  Biochem Biophys Res Commun       Date:  2009-09-13       Impact factor: 3.575

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