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Hiv-1 reverse transcriptase-pseudoknot RNA aptamer interaction has a binding affinity in the low picomolar range coupled with high specificity

Oliver Kensch, Bernard A. Connolly, Heinz Jürgen Steinhoff, Alistair McGregor, Roger S. Goody, Tobias Restle*

*Korrespondierende/r Autor/-in für diese Arbeit

    Abstract

    Systematic evolution of ligands by exponential enrichment (SELEX) is a powerful method for the identification of small oligonucleotides that bind with high affinity and specificity to target proteins. Such DNAs/RNAs are a new class of potential chemotherapeutics that could block the enzymatic activity of pathologically relevant proteins. We have conducted a detailed biochemical study of the interaction of human immunodeficiency virus 1 (HIV- 1) reverse transcriptase (RT) with a SELEX-derived pseudoknot RNA aptamer. Electron paramagnetic resonance spectroscopy of site-directed spin-labeled RT mutants revealed that this aptamer was selected for binding to the 'closed' conformation of the enzyme. Kinetic analysis showed that the RNA inhibitor bound to HIV RT in a two-step process, with association rates similar to those described for model DNA/DNA and DNA/RNA substrates. However, the dissociation of the pseudoknot RNA from RT was dramatically slower than observed for model substrates. Equilibrium binding studies revealed an extraordinarily low K(d), of about 25 pM, for the enzyme-aptamer interaction, presumably a consequence of the slow off-rates. Additionally, this pseudoknot aptamer is highly specific for HIV-1 RT, with the closely related HIV-2 enzyme showing a binding affinity close to 4 orders of magnitude lower.

    OriginalspracheEnglisch
    ZeitschriftJournal of Biological Chemistry
    Jahrgang275
    Ausgabenummer24
    Seiten (von - bis)18271-18278
    Seitenumfang8
    ISSN0021-9258
    DOIs
    PublikationsstatusVeröffentlicht - 16.06.2000

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