Literature DB >> 29052679

Oligonucleotide modifications enhance probe stability for single cell transcriptome in vivo analysis (TIVA).

S B Yeldell1, B K Ruble, I J Dmochowski.   

Abstract

Single cell transcriptomics provides a powerful discovery tool for identifying new cell types and functions as well as a means to probe molecular features of the etiology and treatment of human diseases, including cancer. However, such analyses are limited by the difficulty of isolating mRNA from single cells within biological samples. We recently introduced a photochemical method for isolating mRNA from single living cells, Transcriptome In Vivo Analysis (TIVA). The TIVA probe is a "caged" polyU : polyA oligonucleotide hairpin designed to enter live tissue, where site-specific activation with 405 nm laser reveals the polyU-biotin strand to bind mRNA in a target cell, enabling subsequent mRNA isolation and sequencing. The TIVA method is well suited for analysis of living cells in resected tissue, but has not yet been applied to living cells in whole organisms. Adapting TIVA to this more challenging environment requires a probe with higher thermal stability, more robust caging, and greater nuclease resistance. In this paper we present modifications to the original TIVA probe with multiple aspects of enhanced stability. These newer probes utilize an extended 22mer polyU capture strand with two 9mer polyA blocking strands ("22/9/9") for higher thermal stability pre-photolysis and improved mRNA capture affinity post-photolysis. The "22/9/9 GC" probe features a terminal GC pair to reduce pre-photolysis interactions with mRNA by more than half. The "PS-22/9/9" probe features a phosphorothioated backbone, which extends serum stability from <1 h to at least 48 h, and also mediates uptake into cultured human fibroblasts.

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Year:  2017        PMID: 29052679      PMCID: PMC5718921          DOI: 10.1039/c7ob02353g

Source DB:  PubMed          Journal:  Org Biomol Chem        ISSN: 1477-0520            Impact factor:   3.876


  29 in total

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4.  Single-cell analyses of transcriptional heterogeneity during drug tolerance transition in cancer cells by RNA sequencing.

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7.  Duplex stabilities of phosphorothioate, methylphosphonate, and RNA analogs of two DNA 14-mers.

Authors:  L Kibler-Herzog; G Zon; B Uznanski; G Whittier; W D Wilson
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8.  Sequence-Dependent Fluorescence of Cy3- and Cy5-Labeled Double-Stranded DNA.

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10.  Nanoscale imaging of RNA with expansion microscopy.

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  6 in total

1.  Oligonucleotide Probe for Transcriptome in Vivo Analysis (TIVA) of Single Neurons with Minimal Background.

Authors:  Sean B Yeldell; Linlin Yang; Jaehee Lee; James H Eberwine; Ivan J Dmochowski
Journal:  ACS Chem Biol       Date:  2020-09-23       Impact factor: 5.100

2.  Photoactivatable Circular Caged Oligonucleotides for Transcriptome In Vivo Analysis (TIVA).

Authors:  Linlin Yang; Dora von Trentini; HyunBum Kim; Jai-Yoon Sul; James H Eberwine; Ivan J Dmochowski
Journal:  ChemPhotoChem       Date:  2021-06-23

3.  Efficient Synthesis of Light-Triggered Circular Antisense Oligonucleotides Targeting Cellular Protein Expression.

Authors:  Linlin Yang; Hyun Bum Kim; Jai-Yoon Sul; Sean B Yeldell; James H Eberwine; Ivan J Dmochowski
Journal:  Chembiochem       Date:  2018-04-17       Impact factor: 3.164

4.  Caspase-Activated Oligonucleotide Probe.

Authors:  Linlin Yang; James H Eberwine; Ivan J Dmochowski
Journal:  Bioconjug Chem       Date:  2020-08-24       Impact factor: 4.774

5.  A red-shifted two-photon-only caging group for three-dimensional photorelease.

Authors:  Yvonne Becker; Erik Unger; Manuela A H Fichte; Daniel A Gacek; Andreas Dreuw; Josef Wachtveitl; Peter J Walla; Alexander Heckel
Journal:  Chem Sci       Date:  2018-02-09       Impact factor: 9.825

Review 6.  Conditionally Activated ("Caged") Oligonucleotides.

Authors:  Linlin Yang; Ivan J Dmochowski
Journal:  Molecules       Date:  2021-03-09       Impact factor: 4.411

  6 in total

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