4.6 Review

Caged oligonucleotides for studying biological systems

Journal

JOURNAL OF INORGANIC BIOCHEMISTRY
Volume 150, Issue -, Pages 182-188

Publisher

ELSEVIER SCIENCE INC
DOI: 10.1016/j.jinorgbio.2015.03.010

Keywords

Light-activated oligonucleotides; Caging chemistry; Ruthenium photolinkers; Transcriptome In Vivo Analysis

Funding

  1. NIH [R-01 GM083030]
  2. Camille and Henry Dreyfus Teacher-Scholar Award
  3. McKnight Technological Innovations in Neuroscience Award

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Light-activated (caged) compounds have been widely employed for studying biological processes with high spatial and temporal control. In the past decade, several new approaches for caging the structure and function of DNA and RNA oligonucleotides have been developed. This review focuses on caged oligonucleotides that incorporate site-specifically one or two photocleavable linkers, whose photolysis yields oligonucleotides with dramatic structural and functional changes. This technique has been employed by our laboratory and others to photoregulate gene expression in cells and living organisms, typically using near UV-activated organic chromophores. To improve capabilities for in vivo studies, we harnessed the rich inorganic photochemistry of ruthenium bipyridyl complexes to synthesize Ru-caged morpholino antisense oligonucleotides that remain inactive in zebrafish embryos until uncaged with visible light. Expanding into new caged oligonucleotide applications, our lab has developed Transcriptome In Vivo Analysis (TIVA) technology, which provides the first noninvasive, unbiased method for isolating mRNA from single neurons in brain tissues. TIVA-isolated mRNA can be amplified and then analyzed using next-generation sequencing (RNA-seq). (C) 2015 Elsevier Inc. All rights reserved.

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