AI Article Synopsis

  • RNA ligation is essential for adding cross-linkers and nonnatural nucleotides into RNA, with the traditional method using DNA ligase facing efficiency issues.
  • A new method using T4 RNA ligase improves this process, allowing ligation to nearly complete in just 30 minutes.
  • This technique enables high-efficiency synthesis of RNA, paving the way for new research in RNA biology, including site-specific fluorescent labeling to study RNA structure and function.

Article Abstract

RNA ligation has been a powerful tool for incorporation of cross-linkers and nonnatural nucleotides into internal positions of RNA molecules. The most widely used method for template-directed RNA ligation uses DNA ligase and a DNA splint. While this method has been used successfully for many years, it suffers from a number of drawbacks, principally, slow and inefficient product formation and slow product release, resulting in a requirement for large quantities of enzyme. We describe an alternative technique catalyzed by T4 RNA ligase instead of DNA ligase. Using a splint design that allows the ligation junction to mimic the natural substrate of RNA ligase, we demonstrate several ligation reactions that appear to go nearly to completion. Furthermore, the reactions generally go to completion within 30 min. We present data evaluating the relative importance of various parameters in this reaction. Finally, we show the utility of this method by generating a 128-nucleotide pre-mRNA from three synthetic oligoribonucleotides. The ability to ligate synthetic or in vitro transcribed RNA with high efficiency has the potential to open up areas of RNA biology to new functional and biophysical investigation. In particular, we anticipate that site-specific incorporation of fluorescent dyes into large RNA molecules will yield a wealth of new information on RNA structure and function.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC1624903PMC
http://dx.doi.org/10.1261/rna.93506DOI Listing

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