Development of a Single-Step Subtraction Method for Eukaryotic 18S and 28S Ribonucleic Acids

Abstract

The abundance of mammalian 18S and 28S ribosomal RNA can decrease the detection sensitivity of bacterial or viral targets in complex host-pathogen mixtures. A method to capture human RNA in a single step was developed and characterized to address this issue. For this purpose, capture probes were covalently attached to magnetic microbeads using a dendrimer linker and the solid phase was tested using rat thymus RNA (mammalian components) with Escherichia coli RNA (bacterial target) as a model system. Our results indicated that random capture probes demonstrated better performance than specific ones presumably by increasing the number of possible binding sites, and the use of a tetrame-thylammonium-chloride (TMA-Cl-) based buffer for the hybridization showed a beneficial effect in the selectivity. The subtraction efficiency determined through real-time RT-PCR revealed capture-efficiencies comparable with commercially available enrichment kits. The performance of the solid phase can be further fine tuned by modifying the annealing time and temperature.

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Document Details

Document Type
Technical Report
Publication Date
Jan 01, 2011
Accession Number
ADA544576

Entities

People

  • Baochuan Lin
  • Marie J. Archer

Organizations

  • United States Naval Research Laboratory

Tags

DTIC Thesaurus Topics

  • Acids
  • Albumins
  • Annealing
  • Biotechnology
  • Chemistry
  • Dendrimers
  • Deoxyribonucleic Acids
  • Detection
  • Efficiency
  • Escherichia
  • Escherichia Coli
  • Hybridization
  • Materials
  • Nucleic Acids
  • Phase
  • Ribonucleic Acids
  • Solid Phases

Fields of Study

  • Biology

Readers

  • Molecular Genetics
  • Nanocomposite Materials Science