Optimization of the Omni-ATAC protocol to chromatin accessibility profiling in snap-frozen rat adipose and muscle tissues

Venugopalan D. Nair; Mital Vasoya; Vishnu Nair; Gregory R. Smith; Hanna Pincas; Yongchao Ge; Collin M. Douglas; Karyn A. Esser; Stuart C. Sealfon

doi:10.1016/j.mex.2022.101681

Optimization of the Omni-ATAC protocol to chromatin accessibility profiling in snap-frozen rat adipose and muscle tissues

Venugopalan D. Nair, Mital Vasoya, Vishnu Nair, Gregory R. Smith, Hanna Pincas, Yongchao Ge, Collin M. Douglas, Karyn A. Esser, Stuart C. Sealfon

Research output: Contribution to journal › Article › peer-review

Abstract

ATAC-seq is a fast and sensitive method for the epigenomic profiling of open chromatin and for mapping of transcription factor binding sites [1]. Despite the development of the Omni-ATAC protocol for the profiling of chromatin accessibility in frozen tissues [2], studies in adipose tissue have been restricted due to technical challenges including the high lipid content of adipocytes and reproducibility issues between replicates. Here, we provide a modified Omni-ATAC protocol that achieves high data reproducibility in various tissue types from rat, including adipose and muscle tissues [3]. • This protocol describes a methodology that enables chromatin accessibility profiling from snap-frozen rat adipose and muscle tissues. • The technique comprises an optimized bead-based tissue homogenization process that substitutes to Dounce homogenization, reduces variability in the experimental procedure, and is adaptable to various tissue types. • In comparison with the Omni-ATAC protocol, the method described here results in improved ATAC-seq data quality that complies with ENCODE quality standards.

Original language	English
Article number	101681
Journal	MethodsX
Volume	9
DOIs	https://doi.org/10.1016/j.mex.2022.101681
State	Published - Jan 2022

Keywords

ATAC-seq
Bead-based tissue homogenization
ENCODE quality standards
Ruptor-ATAC
Snap-frozen adipose and muscle tissue

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title = "Optimization of the Omni-ATAC protocol to chromatin accessibility profiling in snap-frozen rat adipose and muscle tissues",

abstract = "ATAC-seq is a fast and sensitive method for the epigenomic profiling of open chromatin and for mapping of transcription factor binding sites [1]. Despite the development of the Omni-ATAC protocol for the profiling of chromatin accessibility in frozen tissues [2], studies in adipose tissue have been restricted due to technical challenges including the high lipid content of adipocytes and reproducibility issues between replicates. Here, we provide a modified Omni-ATAC protocol that achieves high data reproducibility in various tissue types from rat, including adipose and muscle tissues [3]. • This protocol describes a methodology that enables chromatin accessibility profiling from snap-frozen rat adipose and muscle tissues. • The technique comprises an optimized bead-based tissue homogenization process that substitutes to Dounce homogenization, reduces variability in the experimental procedure, and is adaptable to various tissue types. • In comparison with the Omni-ATAC protocol, the method described here results in improved ATAC-seq data quality that complies with ENCODE quality standards.",

keywords = "ATAC-seq, Bead-based tissue homogenization, ENCODE quality standards, Ruptor-ATAC, Snap-frozen adipose and muscle tissue",

author = "Nair, {Venugopalan D.} and Mital Vasoya and Vishnu Nair and Smith, {Gregory R.} and Hanna Pincas and Yongchao Ge and Douglas, {Collin M.} and Esser, {Karyn A.} and Sealfon, {Stuart C.}",

note = "Funding Information: This work was funded by NYSTAR and the Icahn School of Medicine at Mount Sinai. We thank Mary Anne Amper and Nitish Seenarine for outstanding technical assistance. We also express gratitude to the reviewers for providing valuable feedback to our submission. Publisher Copyright: {\textcopyright} 2022 The Author(s)",

year = "2022",

month = jan,

doi = "10.1016/j.mex.2022.101681",

language = "English",

volume = "9",

journal = "MethodsX",

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AU - Nair, Venugopalan D.

AU - Vasoya, Mital

AU - Nair, Vishnu

AU - Smith, Gregory R.

AU - Pincas, Hanna

AU - Ge, Yongchao

AU - Douglas, Collin M.

AU - Esser, Karyn A.

AU - Sealfon, Stuart C.

N1 - Funding Information: This work was funded by NYSTAR and the Icahn School of Medicine at Mount Sinai. We thank Mary Anne Amper and Nitish Seenarine for outstanding technical assistance. We also express gratitude to the reviewers for providing valuable feedback to our submission. Publisher Copyright: © 2022 The Author(s)

PY - 2022/1

Y1 - 2022/1

N2 - ATAC-seq is a fast and sensitive method for the epigenomic profiling of open chromatin and for mapping of transcription factor binding sites [1]. Despite the development of the Omni-ATAC protocol for the profiling of chromatin accessibility in frozen tissues [2], studies in adipose tissue have been restricted due to technical challenges including the high lipid content of adipocytes and reproducibility issues between replicates. Here, we provide a modified Omni-ATAC protocol that achieves high data reproducibility in various tissue types from rat, including adipose and muscle tissues [3]. • This protocol describes a methodology that enables chromatin accessibility profiling from snap-frozen rat adipose and muscle tissues. • The technique comprises an optimized bead-based tissue homogenization process that substitutes to Dounce homogenization, reduces variability in the experimental procedure, and is adaptable to various tissue types. • In comparison with the Omni-ATAC protocol, the method described here results in improved ATAC-seq data quality that complies with ENCODE quality standards.

AB - ATAC-seq is a fast and sensitive method for the epigenomic profiling of open chromatin and for mapping of transcription factor binding sites [1]. Despite the development of the Omni-ATAC protocol for the profiling of chromatin accessibility in frozen tissues [2], studies in adipose tissue have been restricted due to technical challenges including the high lipid content of adipocytes and reproducibility issues between replicates. Here, we provide a modified Omni-ATAC protocol that achieves high data reproducibility in various tissue types from rat, including adipose and muscle tissues [3]. • This protocol describes a methodology that enables chromatin accessibility profiling from snap-frozen rat adipose and muscle tissues. • The technique comprises an optimized bead-based tissue homogenization process that substitutes to Dounce homogenization, reduces variability in the experimental procedure, and is adaptable to various tissue types. • In comparison with the Omni-ATAC protocol, the method described here results in improved ATAC-seq data quality that complies with ENCODE quality standards.

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Optimization of the Omni-ATAC protocol to chromatin accessibility profiling in snap-frozen rat adipose and muscle tissues

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Keywords

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