4.4 Article

DNA self-polymers as microarray probes improve assay sensitivity

Journal

JOURNAL OF NEUROSCIENCE METHODS
Volume 151, Issue 2, Pages 216-223

Publisher

ELSEVIER SCIENCE BV
DOI: 10.1016/j.jneumeth.2005.07.006

Keywords

transcriptome profiling; DNA microarray; hybridization; resonance light scattering; DNA polymerisation; self-ligation; low abundance transcripts

Funding

  1. NIMH NIH HHS [K02 MH070786, MH45156, R21 MH62760] Funding Source: Medline

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DNA microarrays provide a method for determining the expression levels of thousands of genes simultaneously. However, the phenotypic complexity of brain tissue and cross-dilution of transcripts from different sources make it difficult to detect many of the low abundance RNA species. Furthermore, these experiments require significant amounts of starting material, which must often be amplified by one or two rounds of T7 amplification. We have developed a novel microarray probe with increased sensitivity. In this approach, PCR-generated microarray probes are end-ligated into redundant polymers and printed on standard arraying surfaces. These DNA polymer probes result in greatly improved sensitivity over classical monomer probes. Furthermore, polymer microarray sensitivity can be even further improved by incorporation of a biotin adapter into the first strand cDNA during reverse transcription and attachment of a gold particle (Genicon RLS, Invitrogen, CA) in a secondary reaction. This approach allowed us to reliably assess: expression of genes from < 5 mu g of total RNA starting material without sample amplification. Finally, the resonance light scattering-labeled microarrays can be archived without fading, allowing re-scanning at a later time. (c) 2005 Elsevier B.V. All rights reserved.

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