Efficient Enrichment of Synchronized Mouse Spermatocytes Suitable for Genome-Wide Analysis

Overview

Journal Methods Mol Biol

Specialty Molecular Biology

Date 2024 Aug 10

PMID 39126467

Authors

Agustin Carbajal

Irma Gryniuk

Rodrigo O de Castro

Roberto J Pezza

Affiliations

Soon will be listed here.

Abstract

Chromatin undergoes extensive remodeling during meiosis, leading to specific patterns of gene expression and chromosome organization, which ultimately controls fundamental meiotic processes such as recombination and homologous chromosome associations. Recent game-changing advances have been made by analysis of chromatin binding sites of meiotic specific proteins genome-wide in mouse spermatocytes. However, further progress is still highly dependent on the reliable isolation of sufficient quantities of spermatocytes at specific stages of prophase I. Here, we describe a combination of methodologies we adapted for rapid and reliable isolation of synchronized fixed mouse spermatocytes. We show that chromatin isolated from these cells can be used to study chromatin-binding sites by ChIP-seq. High-quality data we obtained from INO80 ChIP-seq in zygotene cells was used for functional analysis of chromatin-binding sites.

Citing Articles

INO80 regulates chromatin accessibility to facilitate suppression of sex-linked gene expression during mouse spermatogenesis.

Chakraborty P, Magnuson T PLoS Genet. 2024; 20(10):e1011431.

PMID: 39405305 PMC: 11508167. DOI: 10.1371/journal.pgen.1011431.

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