Optimization of signal-to-noise ratio for efficient microarray probe design

Olga V Matveeva; Yury D Nechipurenko; Evgeniy Riabenko; Chikako Ragan; Nafisa N Nazipova; Aleksey Y Ogurtsov; Svetlana A Shabalina

doi:10.1093/bioinformatics/btw451

Optimization of signal-to-noise ratio for efficient microarray probe design

Bioinformatics. 2016 Sep 1;32(17):i552-i558. doi: 10.1093/bioinformatics/btw451.

Authors

Olga V Matveeva¹, Yury D Nechipurenko², Evgeniy Riabenko³, Chikako Ragan⁴, Nafisa N Nazipova⁵, Aleksey Y Ogurtsov⁶, Svetlana A Shabalina⁶

Affiliations

¹ Biopolymer Design LLC, Acton, MA 01721, USA Engelhardt Institute of Molecular Biology, Moscow 119991, Russia.
² Engelhardt Institute of Molecular Biology, Moscow 119991, Russia.
³ Moscow Institute of Physics and Technology, Dolgoprudny, Moscow Region, 141701, Russia.
⁴ Queensland Brain Institute, University of Queensland, Brisbane, QLD 4072 Australia.
⁵ Institute of Mathematical Problems of Biology, Pushchino, Moscow Region, 142290, Russia.
⁶ National Center for Biotechnology Information, National Library of Medicine, National Institutes of Health, Bethesda, MD 20894, USA.

Abstract

Motivation: Target-specific hybridization depends on oligo-probe characteristics that improve hybridization specificity and minimize genome-wide cross-hybridization. Interplay between specific hybridization and genome-wide cross-hybridization has been insufficiently studied, despite its crucial role in efficient probe design and in data analysis.

Results: In this study, we defined hybridization specificity as a ratio between oligo target-specific hybridization and oligo genome-wide cross-hybridization. A microarray database, derived from the Genomic Comparison Hybridization (GCH) experiment and performed using the Affymetrix platform, contains two different types of probes. The first type of oligo-probes does not have a specific target on the genome and their hybridization signals are derived from genome-wide cross-hybridization alone. The second type includes oligonucleotides that have a specific target on the genomic DNA and their signals are derived from specific and cross-hybridization components combined together in a total signal. A comparative analysis of hybridization specificity of oligo-probes, as well as their nucleotide sequences and thermodynamic features was performed on the database. The comparison has revealed that hybridization specificity was negatively affected by low stability of the fully-paired oligo-target duplex, stable probe self-folding, G-rich content, including GGG motifs, low sequence complexity and nucleotide composition symmetry.

Conclusion: Filtering out the probes with defined 'negative' characteristics significantly increases specific hybridization and dramatically decreasing genome-wide cross-hybridization. Selected oligo-probes have two times higher hybridization specificity on average, compared to the probes that were filtered from the analysis by applying suggested cutoff thresholds to the described parameters. A new approach for efficient oligo-probe design is described in our study.

Contact: shabalin@ncbi.nlm.nih.gov or olga.matveeva@gmail.com

Supplementary information: Supplementary data are available at Bioinformatics online.

MeSH terms

DNA Probes
Gene Expression Profiling
Genome*
Genomics
Nucleic Acid Hybridization*
Oligonucleotide Array Sequence Analysis*
Oligonucleotides
Sensitivity and Specificity
Signal-To-Noise Ratio*

Substances

DNA Probes
Oligonucleotides