Cell Reports (Sep 2013)

Live-Cell Visualization of Pre-mRNA Splicing with Single-Molecule Sensitivity

  • Robert M. Martin,
  • José Rino,
  • Célia Carvalho,
  • Tomas Kirchhausen,
  • Maria Carmo-Fonseca

DOI
https://doi.org/10.1016/j.celrep.2013.08.013
Journal volume & issue
Vol. 4, no. 6
pp. 1144 – 1155

Abstract

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Removal of introns from pre-messenger RNAs (pre-mRNAs) via splicing provides a versatile means of genetic regulation that is often disrupted in human diseases. To decipher how splicing occurs in real time, we directly examined with single-molecule sensitivity the kinetics of intron excision from pre-mRNA in the nucleus of living human cells. By using two different RNA labeling methods, MS2 and λN, we show that β-globin introns are transcribed and excised in 20–30 s. Furthermore, we show that replacing the weak polypyrimidine (Py) tract in mouse immunoglobulin μ (IgM) pre-mRNA by a U-rich Py decreases the intron lifetime, thus providing direct evidence that splice-site strength influences splicing kinetics. We also found that RNA polymerase II transcribes at elongation rates ranging between 3 and 6 kb min−1 and that transcription can be rate limiting for splicing. These results have important implications for a mechanistic understanding of cotranscriptional splicing regulation in the live-cell context.