4.8 Article

Direct Fluorescence Detection of RNA on Microarrays by Surface-Initiated Enzymatic Polymerization

Journal

ANALYTICAL CHEMISTRY
Volume 85, Issue 1, Pages 426-433

Publisher

AMER CHEMICAL SOC
DOI: 10.1021/ac303132j

Keywords

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Funding

  1. Coulter Foundation
  2. DARPA [N66001-09-C-2082]
  3. NSF [CBET-1033621]
  4. Duke University
  5. Div Of Chem, Bioeng, Env, & Transp Sys
  6. Directorate For Engineering [1033621] Funding Source: National Science Foundation

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We report the first demonstration of surface-initiated enzymatic polymerization (SIEP) for the direct detection of RNA in a fluorescence microarray format. This new method incorporates multiple fluorophores into an RNA strand using the two-step sequential and complementary reactions catalyzed by yeast poly(A) polymerase (PaP) to incorporate deoxyadenosine triphosphate (dATP) at the 3'-OH of an RNA molecule, followed by terminal deoxynucleotidyl transferase (TdT) to catalyze the sequential addition of a mixture of natural and fluorescent deoxynucleotides (dNTPs) at the 3'-OH of an RNA-DNA hybrid. We found that the 3'-end of RNA can be efficiently converted into DNA (similar to 50% conversion) by polymerization of dATP using yeast PaP, and the short DNA strand appended to the end of the RNA by PaP acts as the initiator for the TdT-catalyzed polymerization of longer DNA strands from a mixture of natural and fluorescent dNTPs that contain up to similar to 45 Cy3 fluorophores per 1 kb DNA. We obtained an similar to 2 pM limit of detection (LOD) and a 3 log-linear dynamic range for hybridization of a short 21 base-long RNA target to an immobilized peptide nucleic acid probe, while fragmented mRNA targets from three different full length mRNA transcripts yielded a similar to 10 pM LOD with a similar dynamic range in a microarray format.

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