Folding of the hammerhead ribozyme: Pyrrolo-cytosine fluorescence separates core folding from global folding and reveals a pH-dependent conformational change

Buskiewicz, Iwona; Burke, John M.

doi:10.1261/rna.030999.111

Cited by 12 publications

(10 citation statements)

References 69 publications

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“…The difficulty arises in trying to define often short-lived intermediates that are very difficult to identify and quantify. Previous attempts have utilized a range of time-resolved techniques such as footprinting (Sclavi et al 1998;Silverman et al 2000;Shcherbakova et al 2004), scattering (both X-ray and neutron) (Russell et al 2000;Das et al 2003;Perez-Salas et al 2004;Moghaddam et al 2009;Roh et al 2010;Pollack 2011), as well as fluorescence Haller et al 2011;Buskiewicz and Burke 2012;St-Pierre et al 2014;Frener and Micura 2016). Our experiments directly observe continuous changes in the orientations and stacking of the 2AP nucleobases (local events) as well as changes in the global conformational ensemble observed via SAXS during the transition from secondary structure to tertiary folds.…”

mentioning

confidence: 73%

Divalent ions tune the kinetics of a bacterial GTPase center rRNA folding transition from secondary to tertiary structure

Welty

Pabit

Katz

et al. 2018

RNA

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Folding of an RNA from secondary to tertiary structure often depends on divalent ions for efficient electrostatic charge screening (nonspecific association) or binding (specific association). To measure how different divalent cations modify folding kinetics of the 60 nucleotide E. coli rRNA GTPase center, we combined stopped-flow fluorescence in the presence of Mg 2+ , Ca 2+ , or Sr 2+ together with time-resolved small angle X-ray scattering (SAXS) in the presence of Mg 2+ to observe the folding process. Immediately upon addition of each divalent ion, the RNA undergoes a transition from an extended state with secondary structure to a more compact structure. Subsequently, specific divalent ions modulate populations of intermediates in conformational ensembles along the folding pathway with transition times longer than 10 msec. Rate constants for the five folding transitions act on timescales from submillisecond to tens of seconds. The sensitivity of RNA tertiary structure to divalent cation identity affects all but the fastest events in RNA folding, and allowed us to identify those states that prefer Mg 2+ . The GTPase center RNA appears to have optimized its folding trajectory to specifically utilize this most abundant intracellular divalent ion.

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mentioning

confidence: 73%

Divalent ions tune the kinetics of a bacterial GTPase center rRNA folding transition from secondary to tertiary structure

Welty

Pabit

Katz

et al. 2018

RNA

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“…To probe the structural context of C178 in the complex, we employed the fluorescent cytosine analog pyrrolocytosine (PyC). PyC forms a base pair with G that exhibits structural and thermodynamic properties of a normal G•C pair, and its fluorescence is sensitive to its environment (Buskiewicz and Burke, 2012; Tinsley and Walter, 2006; Zhang et al, 2008; Zhang and Wadkins, 2009). To introduce PyC at T-box position 178, we nicked the non-conserved loop of the antiterminator between positions 170 and 171, generating a two-piece variant of T-box 182 .…”

Section: Resultsmentioning

confidence: 99%

Direct Evaluation of tRNA Aminoacylation Status by the T-Box Riboswitch Using tRNA-mRNA Stacking and Steric Readout

Zhang

Ferré-D′Amaré

2014

Molecular Cell

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SUMMARY T-boxes are gene-regulatory mRNA elements with which Gram-positive bacteria sense amino acid availability. T-boxes have two functional domains. Stem I recognizes the overall shape and anticodon of tRNA, while a 3′ domain evaluates its aminoacylation status, overcoming an otherwise stable transcriptional terminator if the bound tRNA is uncharged. Although T-boxes are believed to evaluate tRNA charge status without using any proteins, this has not been demonstrated experimentally because of the instability of aminoacyl-tRNA. Using a novel, facile method to prepare homogeneous aminoacyl-tRNA, we show that the Bacillus subtilis GlyQS T-box functions independently of any tRNA-binding protein. Comparison of aminoacyl-tRNA analogs demonstrates that the T-box detects the molecular volume of tRNA 3′-substituents. Calorimetry and fluorescence lifetime analysis of labeled RNAs shows that the tRNA acceptor end coaxially stacks on a helix in the T-box 3′ domain. This intimate intermolecular association, selective for uncharged tRNA, stabilizes the antiterminator conformation of the T-box.

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“…It suggests that in vitro conditions (Tris/HCl buffer, pH 7.5) are insufficient for effective folding of TLR-extended ribozymes. It has been suggested that at least two-step folding, if inhibited, might become the rate-limiting step explaining low in vitro efficiency [31]. A similar observation was also made for other extended hammerhead ribozymes [28].…”

Section: Figure 8 Comparative In Silico Analysis Of Distances and Angmentioning

confidence: 55%

Prediction of hammerhead ribozyme intracellular activity with the catalytic core fingerprint

Gabryelska

Wyszko

Szymański

et al. 2013

Biochemical Journal

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Hammerhead ribozyme is a versatile tool for down-regulation of gene expression in vivo. Owing to its small size and high activity, it is used as a model for RNA structure-function relationship studies. In the present paper we describe a new extended hammerhead ribozyme HH-2 with a tertiary stabilizing motif constructed on the basis of the tetraloop receptor sequence. This ribozyme is very active in living cells, but shows low activity in vitro. To understand it, we analysed tertiary structure models of substrate-ribozyme complexes. We calculated six unique catalytic core geometry parameters as distances and angles between particular atoms that we call the ribozyme fingerprint. A flanking sequence and tertiary motif change the geometry of the general base, general acid, nucleophile and leaving group. We found almost complete correlation between these parameters and the decrease of target gene expression in the cells. The tertiary structure model calculations allow us to predict ribozyme intracellular activity. Our approach could be widely adapted to characterize catalytic properties of other RNAs.

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Folding of the hammerhead ribozyme: Pyrrolo-cytosine fluorescence separates core folding from global folding and reveals a pH-dependent conformational change

Cited by 12 publications

References 69 publications

Divalent ions tune the kinetics of a bacterial GTPase center rRNA folding transition from secondary to tertiary structure

Divalent ions tune the kinetics of a bacterial GTPase center rRNA folding transition from secondary to tertiary structure

Direct Evaluation of tRNA Aminoacylation Status by the T-Box Riboswitch Using tRNA-mRNA Stacking and Steric Readout

Prediction of hammerhead ribozyme intracellular activity with the catalytic core fingerprint

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