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Conditionally Activated (“Caged”) Oligonucleotides

by Dmochowski, Ivan J. , Yang, Linlin

in Adenosine / Animals / caged oligonucleotides / CRISPR / Cyclization - genetics / Deoxyribonucleic acid / DNA / enzyme activation / Enzyme Activation - genetics / Gene Expression - genetics / Gene Expression Profiling - methods / Gene Expression Regulation - genetics / Humans / Laboratories / Light / Medical research / Oligonucleotides - chemistry / Oligonucleotides - genetics / Oligonucleotides, Antisense - chemistry / Oligonucleotides, Antisense - genetics / Proteins / Review / RNA, Messenger - genetics / Synthetic Biology - methods / transcriptome in vivo analysis

2021

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Conditionally Activated (“Caged”) Oligonucleotides

by Dmochowski, Ivan J. , Yang, Linlin

2021

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Conditionally Activated (“Caged”) Oligonucleotides

by Dmochowski, Ivan J. , Yang, Linlin

2021

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Journal Article

Conditionally Activated (“Caged”) Oligonucleotides

Dmochowski, Ivan J.,

Yang, Linlin

2021

Overview

Conditionally activated (“caged”) oligonucleotides provide useful spatiotemporal control for studying dynamic biological processes, e.g., regulating in vivo gene expression or probing specific oligonucleotide targets. This review summarizes recent advances in caging strategies, which involve different stimuli in the activation step. Oligo cyclization is a particularly attractive caging strategy, which simplifies the probe design and affords oligo stabilization. Our laboratory developed an efficient synthesis for circular caged oligos, and a circular caged antisense DNA oligo was successfully applied in gene regulation. A second technology is Transcriptome In Vivo Analysis (TIVA), where caged oligos enable mRNA isolation from single cells in living tissue. We highlight our development of TIVA probes with improved caging stability. Finally, we illustrate the first protease-activated oligo probe, which was designed for caspase-3. This expands the toolkit for investigating the transcriptome under a specific physiologic condition (e.g., apoptosis), particularly in specimens where light activation is impractical.

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Publisher

MDPI AG,MDPI

Subject

Adenosine

/ Animals

/ caged oligonucleotides

/ CRISPR

/ Cyclization - genetics

/ Deoxyribonucleic acid

/ DNA