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Characterization of the dimerization process of HIV-1 reverse transcriptase heterodimer using intrinsic protein fluorescence

G. Divita, T. Restle, R. S. Goody

    Abstract

    Intrinsic protein fluorescence has been used to study dimerization of the HIV-1 reverse transcriptase (RT). We observed a 25% increase of the tryptophan fluorescence of the enzyme during dissociation of the subunits induced by the addition of acetonitrile. Upon reassociation of the separated subunits, the original fluorescence emission of the heterodimer is restored. A two-state transition model for the RT dimerization process in which the dimers are in equilibrium with folded monomers is proposed. The free energy of dissociation was determined to be 12.2 (± 0.2) kcal mol. In the absence of Mg2+ ions a decrease of this value was observed, whereas the addition of a synthetic primer/template (18/36mer) results in an increase of dimer stability. Analyzing the effect of Mg2+ on the establishment of the binding equilibrium, a dramatic effect with a 100-fold acceleration of the association by the divalent ion was observed.

    OriginalspracheEnglisch
    ZeitschriftFEBS Letters
    Jahrgang324
    Ausgabenummer2
    Seiten (von - bis)153-158
    Seitenumfang6
    ISSN0014-5793
    DOIs
    PublikationsstatusVeröffentlicht - 14.06.1993

    Fördermittel

    Acknu~v1edgenwntW.se thank Sabine Zimmermann and Ursula Ruhl for excellent techmcal assistance. This work was supported by the Bundesministerium fiir Forschung und Technologie (BMFT), Grant FKS 111/007/90.

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    1. SDG 3 – Gesundheit und Wohlergehen
      SDG 3 – Gesundheit und Wohlergehen

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