Extremely sensitive, background-free gene detection using binary probes and beta replicase

  1. S Tyagi,
  2. U Landegren,
  3. M Tazi,
  4. P M Lizardi, and
  5. F R Kramer
  1. Department of Molecular Genetics, Public Health Research Institute, New York, NY 10016, USA.

Abstract

We have developed a specific and sensitive nucleic acid amplification assay that is suitable for routine gene detection. The assay is based on a novel molecular genetic strategy in which two different RNA probes are hybridized to adjacent positions on a target nucleic acid and then ligated to form an amplifiable reporter RNA. The reporter RNA is then replicated up to a hundred billion-fold in a 30-min isothermal reaction that signals the presence of the target. The assay can detect fewer than 100 nucleic acid molecules; it provides quantitative results over a wide range of target concentrations and it employs a universal format that can detect any infectious agent.

« Previous | Next Article »Table of Contents

This Article

  1. PNAS May 28, 1996 vol. 93 no. 11 5395-5400
  1. » Abstract
  2. Full Text (PDF)

Classifications

About Our New Site Design >>
Link: Advanced Search

This Week's Issue

  1. November 18, 2008, 105 (46)
  1. Current Issue
  1. Alert me to new issues of PNAS

Most