Relating the structure of HIV-1 reverse transcriptase to its processing step

Author:

Jernigan, R. L.

Bahar, I.

Covell, D. G.

Atilgan, A. R.

Erman, B.

Flatow, D. T.
Author Address

NCI, Mol Struct Sect, Lab Expt & Computat Biol, Div Basic Sci, NIH, MSC 5677, Bethesda, MD 20892 USA. NCI, Mol Struct Sect, Lab Expt & Computat Biol, Div Basic Sci, NIH, Bethesda, MD 20892 USA. Bogazici Univ, Ctr Polymer Res, TR-80815 Bebek, Turkey. TUBITAK Adv Polymer Mat ResCtr, TR-80815 Bebek, Turkey. NCI, Frederick Canc Res & Dev Ctr, Sci Applicat Int Corp, Frederick, MD 21702 USA. Sabanci Univ, Sabanci Ctr, TR-80745 Istanbul, Turkey.

Abstract:

By treating an enzyme as a coarse-grained uniform block of material, utilizing only the alpha -Carbon positions, the normal modes of motion can be obtained. For reverse transcriptase the slower of these motions are suggestive of being involved in the processing step, where the RNA or DNA strand is copied onto a new DNA strand at a polymerase site, and the RNA strand is subsequently cut up at the distant Ribonuclease H site. The slowest mode of motion involves hinge bending about a site midway between the polymerase and Ribonuclease H sites, suggesting that it can push or pull the RNA strand between these two sites. Pulling the nucleic acid strand would require tight binding to the RNase H site. The next slowest mode involves a hinge that opens and closes the protein like a clamp, which could facilitate the release of the nucleic acids for their step-wise progression. The third mode could rotate the substrate. An overall description of the step- wise processing step would involve close coordination among these steps. Results suggest that the smaller p51 subunit serves only as ballast to support the various modes of motion involving the different parts of the p66 subunit.

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