A uridine-rich sequence required for translation of prokaryotic mRNA.

Zhang, Jiren; Deutscher, Murray P.

doi:10.1073/pnas.89.7.2605

Cited by 69 publications

(51 citation statements)

References 20 publications

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“…Both constructs differ in their overall activity, because in RS10-10-10, the ribosomal binding site is located immediately downstream of the riboswitch U-stretch that has a strong positive impact on translation efficiency. 12,27 Accordingly, gene expression is reduced in the shifted counterpart. In this tridem, a further increase of the activation ratio compared to the tandem is not possible, as the theophylline-independent activity is already close to zero in RS10-10shift.…”

Section: Increasing the Activation Ratio By Tandem And Tridem Constructsmentioning

confidence: 99%

“…Furthermore, as the close proximity of the terminator U stretch and the downstream Shine-Dalgarno sequence leads to a strong theophylline-independent activity of the reporter gene due to an enhanced translation rate (see ref. 27 ), we additionally designed serial RS constructs based on a modified riboswitch RS10shift. 12 In these constructs, a 19 nt insertion increases the distance between riboswitches and Shine-Dalgarno sequence, leading to a dramatic reduction of activity without theophylline (Fig.…”

Section: Tandem Arrangement Allows Fast and Easy Enhancement Of Activmentioning

confidence: 99%

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Design criteria for synthetic riboswitches acting on transcription

et al. 2015

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Riboswitches are RNA-based regulators of gene expression composed of a ligand-sensing aptamer domain followed by an overlapping expression platform. The regulation occurs at either the level of transcription (by formation of terminator or antiterminator structures) or translation (by presentation or sequestering of the ribosomal binding site). Due to a modular composition, these elements can be manipulated by combining different aptamers and expression platforms and therefore represent useful tools to regulate gene expression in synthetic biology. Using computationally designed theophylline-dependent riboswitches we show that 2 parameters, terminator hairpin stability and folding traps, have a major impact on the functionality of the designed constructs. These have to be considered very carefully during design phase. Furthermore, a combination of several copies of individual riboswitches leads to a much improved activation ratio between induced and uninduced gene activity and to a linear dose-dependent increase in reporter gene expression. Such serial arrangements of synthetic riboswitches closely resemble their natural counterparts and may form the basis for simple quantitative read out systems for the detection of specific target molecules in the cell.

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Section: Increasing the Activation Ratio By Tandem And Tridem Constructsmentioning

confidence: 99%

Section: Tandem Arrangement Allows Fast and Easy Enhancement Of Activmentioning

confidence: 99%

Design criteria for synthetic riboswitches acting on transcription

et al. 2015

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“…The RBS of conventionally leadered Escherichia coli mRNA extends approximately Ϯ 15 nucleotides relative to the start codon (Steitz, 1969;Steitz and Jakes, 1975;Steitz and Steege, 1977), contains non-random sequence using statistical analysis (Scherer et al, 1980;Stormo et al, 1982), and is responsible for establishing a 1000-fold range of translational efficiencies (Ray and Pearson, 1974;. Highly efficient initiation regions include some or all of the following mRNA elements: a polypyrimidine tract for ribosomal protein S1 interaction (Boni et al, 1990;Zhang and Deutscher, 1991;Tzareva et al, 1994); a Shine-Dalgarno (SD) sequence with basepairing complementarity to the anti-SD (ASD) of the 16S rRNA (Shine and Dalgarno, 1974;Hui and de Boer, 1987;Jacob et al, 1987); a cognate start codon for initiator fMet-tRNA anticodon interaction (Ringquist et al, 1992;Vollenoweth and Rabinowitz, 1992); and base-specific enhancer sequences upstream (Olins and Rangwala, 1989) or downstream (Sprengart et al, 1990; of the start codon. The relative importance and interdependence of these mRNA elements as well as the temporal order of their recognition by initiating ribosomes is less well understood.…”

Section: Introductionmentioning

confidence: 99%

An AUG initiation codon, not codon–anticodon complementarity, is required for the translation of unleadered mRNA in Escherichia coli

Etten

Janssen

1998

Molecular Microbiology

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SummaryWe determined the in vivo translational efficiency of 'unleadered' lacZ compared with a conventionally leadered lacZ with and without a Shine-Dalgarno (SD) sequence in Escherichia coli and found that changing the SD sequence of leadered lacZ from the consensus 5Ј-AGGA-3Ј to 5Ј-UUUU-3Ј results in a 15-fold reduction in translational efficiency; however, removing the leader altogether results in only a twofold reduction. An increase in translation coincident with the removal of the leader lacking a SD sequence suggests the existence of stronger or novel translational signals within the coding sequence in the absence of the leader. We examined, therefore, a change in the translational signals provided by altering the AUG initiation codon to other naturally occurring initiation codons (GUG, UUG, CUG) in the presence and absence of a leader and find that mRNAs lacking leader sequences are dependent upon an AUG initiation codon, whereas leadered mRNAs are not. This suggests that mRNAs lacking leader sequences are either more dependent on perfect codon-anticodon complementarity or require an AUG initiation codon in a sequence-specific manner to form productive initiation complexes. A mutant initiator tRNA with compensating anticodon mutations restored expression of leadered, but not unleadered, mRNAs with UAG start codons, indicating that codon-anticodon complementarity was insufficient for the translation of mRNA lacking leader sequences. These data suggest that a cognate AUG initiation codon specifically serves as a stronger and different translational signal in the absence of an untranslated leader.

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“…This behavior is explained by Hfq's preference to bind to AU-rich regions close to RBSs (Franze de Fernandez et al 1972;Senear and Steitz 1976), which are known to act as translational enhancers (Zhang and Deutscher 1992;Hook-Barnard et al 2007). In addition, Hfq is involved in RNA processing, as it regulates polyadenylation-dependent mRNA decay (Hajnsdorf and Regnier 2000;Mohanty et al 2004).…”

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confidence: 99%

Noncanonical repression of translation initiation through small RNA recruitment of the RNA chaperone Hfq

Desnoyers¹,

Massé²

2012

Genes Dev.

122

136

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The RNA chaperone Hfq is mostly known to help small regulatory RNAs (sRNAs) interact with target mRNAs to block initiating ribosomes. In this model, whereas the sRNA is directly competing with initiating 30S ribosomal subunits, Hfq plays only an indirect role, allowing optimal sRNA-mRNA pairing. Here we report that Hfq is recruited by a sRNA, Spot42, to bind to a precise AU-rich region in the vicinity of the translation initiation region (TIR) of sdhC mRNA and competes directly with 30S ribosomal subunits. We show that the sRNA Spot42 binds sdhC too far upstream of the TIR to directly repress translation initiation in vitro and in vivo. Contrary to the canonical model of sRNA regulation, this suggests a new mechanism where Hfq is directly involved in the translational repression of the target mRNA and where the sRNA acts only as a recruitment factor.

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A uridine-rich sequence required for translation of prokaryotic mRNA.

Cited by 69 publications

References 20 publications

Design criteria for synthetic riboswitches acting on transcription

Design criteria for synthetic riboswitches acting on transcription

An AUG initiation codon, not codon–anticodon complementarity, is required for the translation of unleadered mRNA in Escherichia coli

Noncanonical repression of translation initiation through small RNA recruitment of the RNA chaperone Hfq

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