Selective nucleic acid removal via exclusion (SNARE): Capturing mRNA and DNA from a single sample

Lindsay Strotman, Rachel O'Connell, Benjamin P. Casavant, Scott M. Berry, Jamie M. Sperger, Joshua M. Lang, David J. Beebe

Research output: Contribution to journalArticlepeer-review

40 Scopus citations

Abstract

The path from gene (DNA) to gene product (RNA or protein) is the foundation of genotype giving rise to phenotype. Comparison of genomic analyses (DNA) with paired transcriptomic studies (mRNA) is critical to evaluating the pathogenic processes that give rise to human disease. The ability to analyze both DNA and mRNA from the same sample is not only important for biologic interrogation but also to minimize variance (e.g., sample loss) unrelated to the biology. Existing methods for RNA and DNA purification from a single sample are typically time-consuming and labor intensive or require large sample sizes to split for separate RNA and DNA extraction procedures. Thus, there is a need for more efficient and cost-effective methods to purify both RNA and DNA from a single sample. To address this need, we have developed a technique, termed SNARE (Selective Nucleic Acid Removal via Exclusion), that uses pinned oil interfaces to simultaneous purify mRNA and DNA from a single sample. A unique advantage of SNARE is the elimination of dilutive wash and centrifugation processes that are fundamental to conventional methods where sample is typically discarded. This minimizes loss and maximizes recovery by allowing nondilutive reinterrogation of the sample. We demonstrate that SNARE is more sensitive than commercially available kits, robustly and repeatably achieving mRNA and DNA purification from extremely low numbers of cells for downstream analyses. In addition to sensitivity, SNARE is fast, easy to use, and cost-effective and requires no laboratory infrastructure or hazardous chemicals. We demonstrate the clinical utility of the SNARE with prostate cancer circulating tumor cells to demonstrate its ability to perform both genomic and transcriptomic interrogation on rare cell populations that would be difficult to achieve with any current method.

Original languageEnglish
Pages (from-to)9764-9770
Number of pages7
JournalAnalytical Chemistry
Volume85
Issue number20
DOIs
StatePublished - Oct 15 2013

Funding

FundersFunder number
National Institutes of Health (NIH)5R33CA137673
National Science Foundation (NSF)GRFP DGE-0718123
U.S. Department of DefenseW81XWH-12-1-0052
National Childhood Cancer Registry – National Cancer InstituteP30CA014520

    ASJC Scopus subject areas

    • Analytical Chemistry

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