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Self-Splicing and Cyclization of Anabaena pre-tRNA

April 14, 2026
in Medicine
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In a groundbreaking study that promises to reshape our understanding of RNA splicing and circularization, researchers have unveiled the first detailed structural insights into the full-length Anabaena pre-tRNA group I intron system. Using cutting-edge cryo-electron microscopy, they captured multiple conformational states of this catalytic RNA, illuminating a rare natural mechanism where RNA not only self-splices but also circularizes with no sequence loss. This work not only addresses long-standing questions about the structural basis of group I intron catalysis but also opens new avenues for RNA-based biotechnology, including synthetic circular RNA engineering.

Group I introns, known as ribozymes capable of self-splicing, have fascinated molecular biologists since their discovery due to their intrinsic catalytic activity devoid of protein enzymes. Despite extensive biochemical and genetic studies, full-length ribozyme structures that encompass entire exon sequences remain elusive. This limitation has impeded a comprehensive understanding of how these introns transition through splicing states and achieve efficient circularization – a process increasingly recognized for its role in RNA metabolism and regulatory functions. The present study dramatically advances this field by resolving a series of high-resolution structures representing critical intermediates of splicing and subsequent RNA cyclization.

The subject of this exploration lies within the tRNA(Leu) precursor from the cyanobacterium Anabaena, a model organism harboring group I introns with unique mechanistic features. Initially, the researchers observed the apo state of the pre-tRNA, revealing that the exons preassemble into a tRNA-like fold even prior to splicing. This pre-formed architecture serves as a scaffold that promotes the formation of the P1 helix, a key helix implicated in defining splice sites. Such exon prestructuring challenges previous assumptions that exon regions remain flexible and unstructured before intron excision, suggesting instead a direct role for exon folding in guiding catalytic efficiency.

As the RNA transitions through its splicing trajectory, substantial conformational rearrangements materialize, emphasizing the dynamic nature of intron catalysis. These rearrangements are not mere structural curiosities but represent essential molecular motions allowing precise active site assembly. The analyses show how the interplay between intron folding and exon positioning orchestrates the chemical steps of self-splicing, from the first transesterification event to intron release. Importantly, these observations detail an intricate choreography of RNA elements that achieves both sequence specificity and catalytic precision.

Unlike many group I introns, the Anabaena intron showcases a remarkable ability to circularize the intron RNA without any nucleotide loss, a process facilitated by its guanosine binding site acting as the catalytic center. This circularization, previously theorized but not structurally defined, involves a novel mechanism wherein the site of circularization is precisely positioned by intricate RNA motifs. The study highlights the essential role of a guanosine at position 37 (G37) whose strategic reorientation is pivotal in catalyzing the intron’s circularization. This finding substantially diverges from canonical group I introns and underlines a unique molecular adaptation for circular RNA formation.

Further examination revealed that a conserved wobble receptor motif plays a critical role synergizing with G37 to stabilize the circularization site. Mutational analyses confirm that alterations in these motifs drastically reduce cyclization efficiency, pinpointing these elements as indispensable components of the catalytic apparatus. These molecular insights not only explain biological circular RNA production but also suggest design principles for synthetic biology, where precise RNA cyclization is desirable for enhancing RNA stability and function.

One of the most exciting aspects of the research lies in its translational potential. By leveraging the structural blueprint uncovered, the team tested engineered Permuted Intron-Exon (PIE) systems, demonstrating that the identified catalytic principles can be harnessed to improve synthetic RNA circularization. Such engineered systems benefit from the innate catalytic potency and fidelity inherent to the Anabaena intron, enabling efficient generation of circular RNA constructs that hold promise for therapeutic and biotechnological applications, including RNA vaccines and gene regulation tools.

The high-resolution cryo-EM data shed light on the complexity and elegance of RNA catalysis, illustrating how nature employs RNA folding landscapes and nucleotide interactions to orchestrate a cascade of chemical transformations. By resolving the conformational intermediates along the splicing path, the study provides a rare window into dynamic RNA enzymology rarely achievable by conventional methods such as X-ray crystallography, especially when capturing entire exon-intron assemblies in their near-native states.

This investigation also challenges the dogma that RNA catalysis is dominated by protein enzymes, highlighting the versatility of RNA molecules as autonomous catalysts. The findings reinforce the concept that RNA’s structural plasticity and specificity are sufficient to drive complex biochemical reactions, supporting hypotheses that envision such RNA molecules as evolutionary precursors to protein enzymes. The revelation of self-splicing coupled with intron circularization without nucleotide loss adds a new dimension to our understanding of RNA processing and molecular evolution.

Moreover, the structural snapshots reveal how intron-exon interactions sculpt the RNA architecture to ensure splicing accuracy and subsequent circular RNA formation. The pre-tRNA structural assembly observed promotes not only efficient catalysis but potentially coordinates downstream RNA maturation events. Such precise RNA folding mechanisms might reflect an evolutionary advantage, ensuring rapid and error-free processing in cellular contexts where RNA quality control is paramount.

The study’s implications extend to RNA therapeutic strategies, where circular RNAs are gaining recognition for their enhanced stability and translational potential compared to linear RNAs. By elucidating the molecular determinants governing natural RNA circularization, this research lays a foundation for engineering robust circular RNA platforms. These can be tailored to resist exonuclease degradation, facilitate sustained protein expression, or modulate gene networks, thereby transforming RNA-based therapeutics toward clinical realization.

In summary, the elucidation of full-length Anabaena pre-tRNA group I intron structures offers an unprecedented view of RNA self-splicing and cyclization mechanisms. The combined application of cryo-electron microscopy and mutational analyses unravels a rare catalytic paradigm in which RNA reorientation and conserved motifs collaborate to forge RNA circles without sequence loss. This paradigm not only enriches fundamental RNA biology but also propels forward the design of next-generation RNA biotechnologies, capitalizing on nature’s own catalytic brilliance.

As researchers continue to explore the vast repertoire of catalytic RNA activities, the Anabaena intron’s unique features serve as a compass directing future efforts to harness and manipulate RNA structure-function relationships. The structural insights gained here underscore the pivotal role of RNA architecture in dictating enzymatic outcomes and set a new standard for comprehensive molecular characterization of RNA catalysts. This study marks a significant milestone in our quest to understand and exploit the RNA world.

Ultimately, the integration of structural biology, molecular genetics, and biochemical experimentation exemplified by this research embodies the multidisciplinary approach necessary for modern life sciences innovation. The revelation of self-splicing and circularization mechanisms at this atomic level offers transformative potential not only for molecular biology but also for diverse fields such as synthetic biology, RNA therapeutics, and evolutionary biology. The Anabaena pre-tRNA group I intron now stands as a model system illuminating the hidden capabilities encoded within RNA sequences.


Subject of Research: Self-splicing and cyclization of full-length Anabaena pre-tRNA group I introns.

Article Title: Self-splicing and cyclization mechanisms of the full-length Anabaena pre-tRNA.

Article References:
Zhang, X., An, L., Yang, W. et al. Self-splicing and cyclization mechanisms of the full-length Anabaena pre-tRNA. Nat Chem Biol (2026). https://doi.org/10.1038/s41589-026-02205-1

Image Credits: AI Generated

DOI: https://doi.org/10.1038/s41589-026-02205-1

Tags: Anabaena pre-tRNA group I introncatalytic RNA conformational statescryo-electron microscopy RNA structurecyanobacterial tRNA intron systemfull-length ribozyme structural insightsgroup I intron ribozyme catalysisRNA circularization without sequence lossRNA metabolism and regulationRNA self-splicing mechanismRNA-based biotechnology applicationssynthetic circular RNA engineeringtRNA precursor splicing dynamics
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