Ligand Response of Guanidine-IV riboswitch at Single-molecule Level

  1. Lingzhi Gao
  2. Dian Chen
  3. Yu Liu

  • Curated by eLife

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    eLife assessment

    This is an important study on the biochemical and biophysical analysis of a transcriptional riboswitch, detailing how Mg2+ and guanidine regulate RNA conformations. The study provides compelling evidence, developing Position-specific labeling of RNA (PLOR) and single-molecule FRET (smFRET) microscopy that are well suited to investigate the conformational dynamics of RNA structure formation. The study would have been strengthened by using a bacterial instead of phage protein to better recapitulate the physiology of the process. The work is of broad interest to those interested in RNA functional architecture and regulation.

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Abstract

Riboswitches represent a class of non-coding RNA that possess the unique ability to specifically bind ligands and, in response, regulate gene expression. A recent report unveiled a type of riboswitch, known as the guanidine-IV riboswitch, which responds to guanidine levels to regulate downstream genetic transcription. However, the precise molecular mechanism through which the riboswitch senses its target ligand and undergoes conformational changes remain elusive. This gap in understanding has impeded the potential applications of this riboswitch. To bridge this knowledge gap, our study investigated the conformational dynamics of the guanidine-IV riboswitch RNA upon ligand binding. We employed single-molecule fluorescence resonance energy transfer (smFRET) to dissect the behaviors of the aptamer, terminator, and full-length riboswitch. Our findings indicated that the aptamer portion exhibited higher sensitivity to guanidine compared to the terminator and full-length constructs. Additionally, we utilized Position-specific Labelling of RNA (PLOR) combined with smFRET to observe, at the single-nucleotide and single-molecule level, the structural transitions experienced by the guanidine-IV riboswitch during transcription. Notably, we discovered that the influence of guanidine on the riboswitch RNA’s conformations was significantly reduced after the transcription of 88 nucleotides. Furthermore, we proposed a folding model for the guanidine-IV riboswitch in the absence and presence of guanidine, thereby providing insights into its ligand-response mechanism.

Impact statement

The aptamer domain of the guanidine-IV riboswitch exhibits a greater sensitivity to guanidine, surpassing that observed in both the terminator and full-length riboswitch. A finely-tuned transcriptional window of the guanidine-IV riboswitch was detected to be responsive to ligand binding. Furthermore, a folding-function model for the guanidine-IV riboswitch under both guanidine-free and guanidine-present conditions offers valuable insights into its regulatory mechanism.

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  1. Version published to 10.1101/2023.12.05.570130v2 on bioRxiv
  2. Version published to 10.7554/elife.94706 on eLife
  3. Version published to 10.7554/elife.94706.1 on eLife
  4. eLife

    eLife assessment

    This is an important study on the biochemical and biophysical analysis of a transcriptional riboswitch, detailing how Mg2+ and guanidine regulate RNA conformations. The study provides compelling evidence, developing Position-specific labeling of RNA (PLOR) and single-molecule FRET (smFRET) microscopy that are well suited to investigate the conformational dynamics of RNA structure formation. The study would have been strengthened by using a bacterial instead of phage protein to better recapitulate the physiology of the process. The work is of broad interest to those interested in RNA functional architecture and regulation.

  5. eLife

    Reviewer #1 (Public Review):

    Summary:

    This work presents an in-depth characterization of the factors that influence the structural dynamics of the Clostridium botulinum guanidine-IV riboswitch (riboG). Using a single-molecule FRET, the authors demonstrate that riboG undergoes ligand and Mg2+ dependent conformational changes consistent with the dynamic formation of a kissing loop (KL) in the aptamer domain. Formation of the KL is attenuated by Mg2+ and Gua+ ligand at physiological concentrations as well as the length of the RNA. Interestingly, the KL is most stable in the context of just the aptamer domain compared to longer RNAs capable of forming the terminator stem. To attenuate transcription, binding of Gua+ and formation of the KL must occur rapidly after transcription of the aptamer domain but before transcription of the rest of the terminator stem.

    Strengths:

    (1) Single-molecule FRET microscopy is well suited to unveil the conformational dynamics of KL formation and the authors provide a wealth of data to examine the effect of the ligand and ions on riboswitch dynamics. The addition of complementary transcriptional readthrough assays provides further support for the author's proposed model of how the riboswitch dynamics contribute to function.

    (2) The single-molecule data strongly support that the effect of Gua+ ligand and Mg2+ influence the RNA structure differently for varying lengths of the RNA. The authors also demonstrate that this is specific for Mg2+ as Na+ and K+ ions have little effect.

    (3) The PLOR method utilized is clever and well adapted for both dual labeling of RNAs and examining RNA at various lengths to mimic co-transcriptional folding. Using PLOR, they demonstrate that a change in the structural dynamics and ligand binding can occur after the extension of the RNA transcript by a single nucleotide. Such a tight window of regulation has intriguing implications for kinetically controlled riboswitches.

    Weaknesses:

    (1) The authors use only one mutant to confirm that their FRET signal indicates the formation of the KL. Importantly, this mutation does not involve the nucleotides that are part of the KL interaction. It would be more convincing if the authors used mutations in both strands of the KL and performed compensatory mutations that restore base pairing. Experiments like this would solidify the structural interpretation of the work, particularly in the context of the full-length riboG RNA or in the co-transcriptional mimic experiments, which appear to have more conformational heterogeneity.

    (2) The existence of the pre-folded state (intermediate FRET ~0.5) is not well supported in their data and could be explained by an acquisition artifact. The dwell times are very short often only a single frame indicating that there could be a very fast transition (< 0.1s) from low to high FRET that averages to a FRET efficiency of 0.5. To firmly demonstrate that this intermediate FRET state is metastable and not an artifact, the authors need to perform measurements with a faster frame rate and demonstrate that the state is still present.

    (3) The PLOR method employs a non-biologically relevant polymerase (T7 RNAP) to mimic transcription elongation and folding near the elongation complex. T7 RNAP has a shorter exit channel than bacterial RNAPs and therefore, folding in the exit channel may be different between different RNAPs. Additionally, the nascent RNA may interact with bacterial RNAP differently. For these reasons, it is not clear how well the dynamics observed in the T7 ECs recapitulate riboswitch folding dynamics in bacterial ECs where they would occur in nature.

  6. eLife

    Reviewer #2 (Public Review):

    Summary:

    Gao et al. used single-molecule FRET and step-wise transcription methods to study the conformations of the recently reported guanidine-IV class of bacterial riboswitches that upregulate transcription in the presence of elevated guanidine. Using three riboswitch lengths, the authors analyzed the distributions and transitions between different conformers in response to different Mg2+ and guanidine concentrations. These data led to a three-state kinetic model for the structural switching of this novel class of riboswitches whose structures remain unavailable. Using the PLOR method that the authors previously invented, they further examined the conformations, ligand responses, and gene-regulatory outcomes at discrete transcript lengths along the path of vectorial transcription. These analyses uncover that the riboswitch exhibits differential sensitivity to ligand-induced conformational switching at different steps of transcription, and identify a short window where the regulatory outcome is most sensitive to ligand binding.

    Strengths:

    Dual internal labeling of long RNA transcripts remains technically very challenging but essential for smFRET analyses of RNA conformations. The authors should be commended for achieving very high quality and purity in their labelled RNA samples. The data are extensive, robust, thorough, and meticulously controlled. The interpretations are logical and conservative. The writing is reasonably clear and the illustrations are of high quality. The findings are significant because the paradigm uncovered here for this relatively simple riboswitch class is likely also employed in numerous other kinetically regulated riboswitches. The ability to quantitatively assess RNA conformations and ligand responses at multiple discrete points along the path towards the full transcript provides a rare and powerful glimpse into co-transcriptional RNA folding, ligand-binding, and conformational switching.

    Weaknesses:

    The use of T7 RNA polymerase instead of a near-cognate bacterial RNA polymerase in the termination/antitermination assays is a significant caveat. It is understandable as T7 RNA polymerase is much more robust than its bacterial counterparts, which probably will not survive the extensive washes required by the PLOR method. The major conclusions should still hold, as the RNA conformations are probed by smFRET at static, halted complexes instead of on the fly. However, potential effects of the cognate RNA polymerase cannot be discerned here, including transcriptional rates, pausing, and interactions between the nascent transcript and the RNA exit channel, if any. The authors should refrain from discussing potential effects from the DNA template or the T7 RNA polymerase, as these elements are not cognate with the riboswitch under study.

  7. eLife

    Reviewer #3 (Public Review):

    Summary:

    In this article, Gao et. al. uses single-molecule FRET (smFRET) and position-specific labelling of RNA (PLOR) to dissect the folding and behavioral ligand sensing of the Guanidine-IV riboswitch in the presence and absence of the ligand guanidine and the cation Mg2+. The results provided valuable information on the mechanistic aspects of the riboswitch, including the confirmation of the kissing loop present in the structure as essential for folding and riboswitch activity. Co-transcriptional investigations of the system provided key information on the ligand-sensing behavior and ligand-binding window of the riboswitch. A plausible folding model of the Guanidine-IV riboswitch was proposed as a final result. The evidence presented here sheds additional light on the mode of action of transcriptional riboswitches.

    Strengths:

    The investigations were very thorough, providing data that supports the conclusions. The use of smFRET and PLOR to investigate RNA folding has been shown to be a valuable tool for the understanding of folding and behavior properties of these structured RNA molecules. The co-transcriptional analysis brought important information on how the riboswitch works, including the ligand-sensing and the binding window that promotes the structural switch. The fact that investigations were done with the aptamer domain, aptamer domain + terminator/anti-terminator region, and the full-length riboswitch were essential to inform how each domain contributes to the final structural state if in the presence of the ligand and Mg2+.

    Weaknesses:

    The system has its own flaws when compared to physiological conditions. The RNA polymerase used (the study uses T7 RNA polymerase) is different from the bacterial RNA polymerase, not only in complexity, but also in transcriptional speed, which can directly interfere with folding and ligand-sensing. Additionally, rNTPs concentrations were much lower than physiological concentrations during transcription, likely causing a change in the polymerase transcriptional speed. These important aspects and how they could interfere with results are important to be addressed to the broad audience. Another point of consideration to be aware of is that the bulky fluorophores attached to the nucleotides can interfere with folding to some extent.

  8. Version published to 10.1101/2023.12.05.570130v1 on bioRxiv