4.7 Article

BRET-Based method for detection of specific RNA species

Journal

BIOCONJUGATE CHEMISTRY
Volume 19, Issue 1, Pages 178-184

Publisher

AMER CHEMICAL SOC
DOI: 10.1021/bc700278n

Keywords

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Funding

  1. NATIONAL CANCER INSTITUTE [P50CA114747, R01CA082214] Funding Source: NIH RePORTER
  2. NCI NIH HHS [5R01 CA82214, P50CA114747] Funding Source: Medline

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RNA detection and quantitation is a common necessity in modern molecular biology research. Most methods, however, are complex and/or, time-intensive. Presented here is a BRET (bioluminescene resonance energy transfer)based method. that can accomplish the task of RNA identification quickly and easily. By conjugating BRET enzymes to two different oligonucleotides that are complementary to the same target sequence, probes were developed that could detect RNA using a solution-based assay. This assay was optimized for spacer length between the binding sites (found to be 10 nucleotides), and sensitivity was determined to be 1 mu g for a specific species of RNA within a mixed population. Specificity of the assay was assessed using in vitro transcribed cRNA and found to be statistically siginificant (p = 3.11 X 10(-6), ANOVA, multiple range test). This assay represents a possibility for a less technically demanding, streamlined alternative to canonical RNA assays.

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