Abstract
An assay for transposase-accessible chromatin with high-throughput sequencing (ATAC-seq) has become an increasingly popular method to assess genome-wide chromatin accessibility in isolated nuclei from fresh tissues. However, many biobanks contain only snap-frozen tissue samples. While ATAC-seq has been applied to frozen brain tissues in human, its applicability in a wide variety of tissues in horse remains unclear. The Functional Annotation of Animal Genome (FAANG) project is an international collaboration aimed to provide high quality functional annotation of animal genomes. The equine FAANG initiative has generated a biobank of over 80 tissues from two reference female animals and experiments to begin to characterize tissue specificity of genome function for prioritized tissues have been performed. Due to the logistics of tissue collection and storage, extracting nuclei from a large number of tissues for ATAC-seq at the time of collection is not always practical. To assess the feasibility of using stored frozen tissues for ATAC-seq and to provide a guideline for the equine FAANG project, we compared ATAC-seq results from nuclei isolated from frozen tissue to cryopreserved nuclei (CN) isolated at the time of tissue harvest in liver, a highly cellular homogenous tissue, and lamina, a relatively acellular tissue unique to the horse. We identified 20,000–33,000 accessible chromatin regions in lamina and 22–61,000 in liver, with consistently more peaks identified using CN isolated at time of tissue collection. Our results suggest that frozen tissues are an acceptable substitute when CN are not available. For more challenging tissues such as lamina, nuclei extraction at the time of tissue collection is still preferred for optimal results. Therefore, tissue type and accessibility to intact nuclei should be considered when designing ATAC-seq experiments.
Highlights
The completion of the equine genome assembly (Wade et al, 2009; Kalbfleisch et al, 2018) has enabled research leading to novel discoveries concerning the health and reproduction of horses (Finno and Bannasch, 2014; Ghosh et al, 2018; Raudsepp et al, 2019)
The Functional Annotation of Animal Genome (FAANG) initiative (The FAANG Consortium et al, 2015) is an international collaboration aimed to bridge this gap between genotype and phenotype
Libraries prepared by two laboratories (L1 and L2) using nuclei isolated from snap-frozen tissues (FTDN) or cryopreserved from tissues at time of collection (CN) from liver and lamina of two animals (AH1 and AH2, Thoroughbred adult mares) were sequenced at PE75 on an Illumina HiSeq 4000 (L1) or PE42 on an Illumina NextSeq 500 (L2)
Summary
The completion of the equine genome assembly (Wade et al, 2009; Kalbfleisch et al, 2018) has enabled research leading to novel discoveries concerning the health and reproduction of horses (Finno and Bannasch, 2014; Ghosh et al, 2018; Raudsepp et al, 2019). Despite having the same genomic sequence, differential regulation of gene expression leads to tissue-specific profiles. A lack of understanding of gene regulation has largely stalled research of complex traits in horses. The Encyclopedia of DNA Elements (ENCODE) project has provided an abundance of data for understanding gene regulation and its role in complex diseases and traits (Qu and Fang, 2013). The Functional Annotation of Animal Genome (FAANG) initiative (The FAANG Consortium et al, 2015) is an international collaboration aimed to bridge this gap between genotype and phenotype. The equine FAANG project has successfully generated a biobank of over 80 tissues and bodily fluids of two reference animals (Burns et al, 2018). Additional projects are underway to identify tissue specific chromatin states to integrate all of these datasets and build a robust tissue specific functional annotation atlas in the horse (Giuffra et al, 2019)
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