Choreography of molecular movements during ribosome progression along mRNA

Belardinelli, Riccardo; Sharma, Heena; Caliskan, Neva; Cunha, C. E.; Peske, Frank; Wintermeyer, Wolfgang; Rodnina, Marina V.

doi:10.1038/nsmb.3193

Cited by 90 publications

(274 citation statements)

References 46 publications

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“…Translocation, the movement of the mRNA•tRNA pairs from the ribosomal A and P sites to the P and E sites, respectively, resets the ribosome for acceptance of a new tRNA after every round of amino acid addition. Translocation is catalyzed by the binding and subsequent GTP hydrolysis of eEF2 (EF-G in bacteria), and involves a series of concerted conformational changes largely in the small subunit (Belardinelli et al, 2016; Frank et al, 2007; Munro et al, 2010; Ratje et al, 2010; Zhou et al, 2014). First, rotation of the body of the small subunit relative to the large subunit, and swiveling of the head leads to the formation of the so-called hybrid or rotated state, which is thermodynamically stabilized by peptidyl-tRNA and binding of eEF2 (Munro et al, 2009).…”

Section: (Introduction)mentioning

confidence: 99%

The ATPase Fap7 Tests the Ability to Carry Out Translocation-like Conformational Changes and Releases Dim1 during 40S Ribosome Maturation

et al. 2017

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SUMMARY Late in their maturation, nascent small (40S) ribosomal subunits bind 60S subunits to produce 80S-like ribosomes. Due to the analogy of this translation-like cycle to actual translation, and because 80S-like ribosomes do not produce any protein, it was suggested that this represents a quality-control mechanism for subunit functionality. Here, we use genetic and biochemical experiments to show that the essential ATPase Fap7 promotes formation of the rotated state, a key intermediate in translocation, thereby releasing the essential assembly factor Dim1 from pre-40S subunits. Bypassing this quality control step produces defects in reading frame maintenance. These results show how progress in the maturation cascade is linked to a test for a key functionality of 40S ribosomes, their ability to translocate the mRNA•tRNA pair. Furthermore, our data demonstrate for the first time that the translation-like cycle is a quality control mechanism that ensures the fidelity of the cellular ribosome pool.

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Section: (Introduction)mentioning

confidence: 99%

The ATPase Fap7 Tests the Ability to Carry Out Translocation-like Conformational Changes and Releases Dim1 during 40S Ribosome Maturation

et al. 2017

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“…This is elegantly demonstrated by the recent advances in time-resolved cryo-electron microscopy, based on insights from single-molecule fluorescence measurements. The studies provided a detailed insight into the structure of the ribosome in real time as it transitions through different functional states during protein biosynthesis (Fischer et al, 2010;Tsai et al, 2014;Chen et al, 2015;Belardinelli et al, 2016).…”

Section: Introductionmentioning

confidence: 99%

The ribosome and its role in protein folding: looking through a magnifying glass

Javed

Christodoulou

Cabrita

et al. 2017

Acta Crystallogr D Struct Biol

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Protein folding, a process that underpins cellular activity, begins cotranslationally on the ribosome. During translation, a newly synthesized polypeptide chain enters the ribosomal exit tunnel and actively interacts with the ribosome elements -the r-proteins and rRNA that line the tunnel -prior to emerging into the cellular milieu. While understanding of the structure and function of the ribosome has advanced significantly, little is known about the process of folding of the emerging nascent chain (NC). Advances in cryoelectron microscopy are enabling visualization of NCs within the exit tunnel, allowing early glimpses of the interplay between the NC and the ribosome. Once it has emerged from the exit tunnel into the cytosol, the NC (still attached to its parent ribosome) can acquire a range of conformations, which can be characterized by NMR spectroscopy. Using experimental restraints within molecular-dynamics simulations, the ensemble of NC structures can be described. In order to delineate the process of co-translational protein folding, a hybrid structural biology approach is foreseeable, potentially offering a complete atomic description of protein folding as it occurs on the ribosome.

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“…As done in Belardinelli et al [21], we consider here that the 30S head rotations are monitored by S13-L33 FRET (30S head protein S13 labeled with the nonfluorescent acceptor and large 50S subunit protein L33 labeled with the fluorescence donor), the 30S subunit rotations are monitored by S6-L9 FRET (30S body protein S9 labeled with the nonfluorescent acceptor and 50S subunit protein L9 labeled with the fluorescence donor), the movement of mRNA is monitored with reporter Alx405 or Alx488 attached to the 3′ end of the mRNA, the deacylated tRNA dissociation is monitored by tRNA-L33 FRET, and the binding and dissociation of EF-G are monitored by L12-EF-G FRET.…”

Section: Resultsmentioning

confidence: 91%

“…The smFRET data revealed direct evidence of structurally distinct late intermediates during translocation such as exaggerated, reversible fluctuations of the 30S head [15]. The ensemble kinetic data revealed an early forward rotation or swiveling of the 30S head taking place while the 30S body rotating in the opposite, clockwise direction, and the backward swiveling of the 30S head starting upon tRNA translocation and continuing until the posttranslocation state is reached [21]. However, what similarities and differences are between the dynamic relations among different state transitions or processes in the translocation pathway exhibited in the smFRET data and those exhibited in the ensemble kinetic data are not clear.…”

Section: Introductionmentioning

confidence: 92%

“…To this end, both single molecule fluorescence resonance energy transfer (smFRET) and ensemble kinetic (or ensemble FRET) methods were recently employed to record simultaneously the FRET data between different pairs of multiple reporters placed on both ribosomal subunits, tRNA and EF-G [15, 21]. The smFRET data revealed direct evidence of structurally distinct late intermediates during translocation such as exaggerated, reversible fluctuations of the 30S head [15].…”

Section: Introductionmentioning

confidence: 99%

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Dynamic relationships between ribosomal conformational and RNA positional changes during ribosomal translocation

Xie

2016

Heliyon

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Ribosomal translocation catalyzed by EF-G hydrolyzing GTP entails multiple conformational changes of ribosome and positional changes of tRNAs and mRNA in the ribosome. However, the detailed dynamic relations among these changes and EF-G sampling are not clear. Here, based on our proposed pathway of ribosomal translocation, we study theoretically the dynamic relations among these changes exhibited in the single molecule data and those exhibited in the ensemble kinetic data. It is shown that the timing of these changes in the single molecule data and that in the ensemble kinetic data show very different. The theoretical results are in agreement with both the available ensemble kinetic experimental data and the single molecule experimental data.

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Choreography of molecular movements during ribosome progression along mRNA

Cited by 90 publications

References 46 publications

The ATPase Fap7 Tests the Ability to Carry Out Translocation-like Conformational Changes and Releases Dim1 during 40S Ribosome Maturation

The ATPase Fap7 Tests the Ability to Carry Out Translocation-like Conformational Changes and Releases Dim1 during 40S Ribosome Maturation

The ribosome and its role in protein folding: looking through a magnifying glass

Dynamic relationships between ribosomal conformational and RNA positional changes during ribosomal translocation

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