BaseSpace
Correlation Engine 2.0
Import Your Data
Literature

FAQ

More FAQs

Back to top
Clear Search sequence regions
(e.g. Heart, Alcohol, Rosiglitazone, rs2300478, NEUROG3, Apoptosis, Pseudomonas infection)
Bookmark Forward

QuASAR-MPRA: accurate allele-specific analysis for massively parallel reporter assays.

Cynthia A Kalita, Gregory A Moyerbrailean, Christopher Brown, Xiaoquan Wen, Francesca Luca, Roger Pique-Regi

Bioinformatics (Oxford, England) 2018 Mar 01


filter terms:
  • alleles (1)
  • data analysis (2)
  • elements (1)
  • gene (4)
  • human (3)
  • meta analysis (1)
  • nucleic acid (1)
  • parallel (6)
  • plasmid (1)
  • signals (1)
    • Sizes of these terms reflect their relevance to your search.

    The majority of the human genome is composed of non-coding regions containing regulatory elements such as enhancers, which are crucial for controlling gene expression. Many variants associated with complex traits are in these regions, and may disrupt gene regulatory sequences. Consequently, it is important to not only identify true enhancers but also to test if a variant within an enhancer affects gene regulation. Recently, allele-specific analysis in high-throughput reporter assays, such as massively parallel reporter assays (MPRAs), have been used to functionally validate non-coding variants. However, we are still missing high-quality and robust data analysis tools for these datasets. We have further developed our method for allele-specific analysis QuASAR (quantitative allele-specific analysis of reads) to analyze allele-specific signals in barcoded read counts data from MPRA. Using this approach, we can take into account the uncertainty on the original plasmid proportions, over-dispersion, and sequencing errors. The provided allelic skew estimate and its standard error also simplifies meta-analysis of replicate experiments. Additionally, we show that a beta-binomial distribution better models the variability present in the allelic imbalance of these synthetic reporters and results in a test that is statistically well calibrated under the null. Applying this approach to the MPRA data, we found 602 SNPs with significant (false discovery rate 10%) allele-specific regulatory function in LCLs. We also show that we can combine MPRA with QuASAR estimates to validate existing experimental and computational annotations of regulatory variants. Our study shows that with appropriate data analysis tools, we can improve the power to detect allelic effects in high-throughput reporter assays. http://github.com/piquelab/QuASAR/tree/master/mpra. fluca@wayne.edu or rpique@wayne.edu. Supplementary data are available online at Bioinformatics. © The Author (2017). Published by Oxford University Press. All rights reserved. For Permissions, please email: journals.permissions@oup.com

    Citation

    Cynthia A Kalita, Gregory A Moyerbrailean, Christopher Brown, Xiaoquan Wen, Francesca Luca, Roger Pique-Regi. QuASAR-MPRA: accurate allele-specific analysis for massively parallel reporter assays. Bioinformatics (Oxford, England). 2018 Mar 01;34(5):787-794

    Expand section icon Mesh Tags


    PMID: 29028988

    View Full Text
    • Copyright © 2024 Illumina Inc. All rights reserved.