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Sperm chromatin structure and reproductive fitness are altered by substitution of a single amino acid in mouse protamine 1

Lindsay Moritz, Samantha B. Schon, Mashiat Rabbani, Yi Sheng, Ritvija Agrawal, Juniper Glass-Klaiber, Caleb Sultan, Jeannie M. Camarillo, Jourdan Clements, Michael R. Baldwin, Adam G. Diehl, Alan P. Boyle, Patrick J. O'Brien, Kaushik Ragunathan, Yueh-Chiang Hu, Neil L. Kelleher, Jayakrishnan Nandakumar, Jun Z. Li, Kyle E. Orwig, Sy Redding, Saher Sue Hammoud

Nature structural & molecular biology(2023)

Cited 1|Views27
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Abstract
Conventional dogma presumes that protamine-mediated DNA compaction in sperm is achieved by electrostatic interactions between DNA and the arginine-rich core of protamines. Phylogenetic analysis reveals several non-arginine residues conserved within, but not across species. The significance of these residues and their post-translational modifications are poorly understood. Here, we investigated the role of K49, a rodent-specific lysine residue in protamine 1 (P1) that is acetylated early in spermiogenesis and retained in sperm. In sperm, alanine substitution (P1(K49A)) decreases sperm motility and male fertility-defects that are not rescued by arginine substitution (P1(K49R)). In zygotes, P1(K49A) leads to premature male pronuclear decompaction, altered DNA replication, and embryonic arrest. In vitro, P1(K49A) decreases protamine-DNA binding and alters DNA compaction and decompaction kinetics. Hence, a single amino acid substitution outside the P1 arginine core is sufficient to profoundly alter protein function and developmental outcomes, suggesting that protamine non-arginine residues are essential for reproductive fitness. Here, the authors show that a single substitution in mouse P1, outside of its arginine core and independently of its charge, suffices to alter sperm chromatin structure and associated developmental outcomes.
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