Structural mechanism of GTPase-powered ribosome-tRNA movement

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作者
Valentyn Petrychenko
Bee-Zen Peng
Ana C. de A. P. Schwarzer
Frank Peske
Marina V. Rodnina
Niels Fischer
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[1] Max Planck Institute for Biophysical Chemistry,Department of Structural Dynamics
[2] Max Planck Institute for Biophysical Chemistry,Department of Physical Biochemistry
[3] University Medical Center Göttingen,Department of Molecular Biology
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GTPases are regulators of cell signaling acting as molecular switches. The translational GTPase EF-G stands out, as it uses GTP hydrolysis to generate force and promote the movement of the ribosome along the mRNA. The key unresolved question is how GTP hydrolysis drives molecular movement. Here, we visualize the GTPase-powered step of ongoing translocation by time-resolved cryo-EM. EF-G in the active GDP–Pi form stabilizes the rotated conformation of ribosomal subunits and induces twisting of the sarcin-ricin loop of the 23 S rRNA. Refolding of the GTPase switch regions upon Pi release initiates a large-scale rigid-body rotation of EF-G pivoting around the sarcin-ricin loop that facilitates back rotation of the ribosomal subunits and forward swiveling of the head domain of the small subunit, ultimately driving tRNA forward movement. The findings demonstrate how a GTPase orchestrates spontaneous thermal fluctuations of a large RNA-protein complex into force-generating molecular movement.
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