Pyrrolo-C as a molecular probe for monitoring conformations of the tRNA 3′ end

Zhang, Chunmei; Liu, Cuiping; Christian, Tom; Gamper, Howard; Rozenski, Jef; Pan, Dongli; Randolph, John B.; Wickstrom, Eric; Cooperman, Barry S.; Hou, Ya‐Ming

doi:10.1261/rna.1158508

Cited by 18 publications

(11 citation statements)

References 45 publications

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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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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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“…For tRNAs esterified with aromatic or other highly hydrophobic side chains, aa-tRNAs and non-aa-tRNAs can be directly separated using RP-HPLC, based on their difference in hydrophobicity (Cayama, Yepez, Rotondo, Bandeira, Ferreras et al, 2000; Zhang, Liu, Christian, Gamper, Rozenski et al, 2008). For tRNAs esterified with other amino acids, in particular those with small or polar side chains (e.g., glycine, alanine), chromatographic methods are generally unable to achieve satisfactory separation.…”

Section: Methodsmentioning

confidence: 99%

A Flexible, Scalable Method for Preparation of Homogeneous Aminoacylated tRNAs

Zhang¹,

Ferré-D′Amaré²

2014

Methods in Enzymology

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Transfer RNAs (tRNAs) are cellular courier molecules that decipher the genetic code in messenger RNAs and enable the transfer of appropriate esterified amino acids to the growing peptide chain. The preparation of biophysical quantities of homogeneous aminoacylated tRNAs has remained a significant technical challenge. This is primarily due to the difficulty in removing contaminating non-aminoacylated tRNAs that are have very similar properties overall, as well as the hydrolytic instability of the aminoacyl linkage. We describe a flexible, scalable method to prepare homogeneous aminoacylated tRNAs that is also broadly compatible with mutant, misacylated or otherwise aberrant tRNAs and other RNAs. This method combines ribozyme-mediated aminoacylation with reversible N-pentenoylation of the esterified amino acid, which not only protects against spontaneous deacylation but also provides a hydrophobic purification handle. This protocol makes it straightforward to produce biophysical quantities of natural and unnatural aminoacylated tRNAs, and has proven essential for mechanistic investigations of the T-box riboswitches.

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“…The penultimate base of the appropriate tRNALeu (UAA) isoacceptor was labelled with a pyrrolo-cytidine fluorophore. To achieve labelling, E. coli tRNA nucleotidyl transferase enzyme was incubated with a truncated in vitro tRNA transcript and pyrrolo-CTP (Trilink Biotechnologies) and ATP as outlined previously 32 . Fluorescence experiments were performed in buffer containing 50 mM HEPES (pH 7.4), 20 mM KCl, 10 mM MgCl 2 and 10 mM b-ME at 28 1C.…”

Section: Methodsmentioning

confidence: 99%

“…3c). This approach was used to monitor the conformation of the CCA 3 0 -end of tRNA Cys interacting with cysteinyl-tRNA synthetase 32 . By monitoring the fluorescence from this probe, we expected to see a significant change in the spectrum when the LeuRS Á tRNApyr Leu complex was bound to TM84 or not.…”

Section: Tm84 Is a Tight-binding Inhibitor Of Trna Leu Aminoacylationmentioning

confidence: 99%

Plant tumour biocontrol agent employs a tRNA-dependent mechanism to inhibit leucyl-tRNA synthetase

et al. 2013

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Leucyl-tRNA synthetases (LeuRSs) have an essential role in translation and are promising targets for antibiotic development. Agrocin 84 is a LeuRS inhibitor produced by the biocontrol agent Agrobacterium radiobacter K84 that targets pathogenic strains of A. tumefaciens, the causative agent of plant tumours. Agrocin 84 acts as a molecular Trojan horse and is processed inside the pathogen into a toxic moiety (TM84). Here we show using crystal structure, thermodynamic and kinetic analyses, that this natural antibiotic employs a unique and previously undescribed mechanism to inhibit LeuRS. TM84 requires tRNA Leu for tight binding to the LeuRS synthetic active site, unlike any previously reported inhibitors. TM84 traps the enzyme-tRNA complex in a novel 'aminoacylation-like' conformation, forming novel interactions with the KMSKS loop and the tRNA 3 0 -end. Our findings reveal an intriguing tRNAdependent inhibition mechanism that may confer a distinct evolutionary advantage in vivo and inform future rational antibiotic design.

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Pyrrolo-C as a molecular probe for monitoring conformations of the tRNA 3′ end

Cited by 18 publications

References 45 publications

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

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

A Flexible, Scalable Method for Preparation of Homogeneous Aminoacylated tRNAs

Plant tumour biocontrol agent employs a tRNA-dependent mechanism to inhibit leucyl-tRNA synthetase

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