Meiotic resetting of the cellular Sod1 pool is driven by protein aggregation, degradation, and transient LUTI-mediated repression

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Abstract

ABSTRACT Gametogenesis requires packaging of the cellular components needed for the next generation. In budding yeast, this process includes degradation of many mitotically stable proteins, followed by their resynthesis. Here, we show that one such case—Superoxide dismutase 1 (Sod1), a protein that commonly aggregates in human ALS patients—is regulated by an integrated set of events, beginning with the formation of pre-meiotic Sod1 aggregates. This is followed by degradation of a subset of the prior Sod1 pool and clearance of Sod1 aggregates. As degradation progresses, Sod1 protein production is transiently blocked during mid-meiotic stages by transcription of an extended and poorly translated SOD1 mRNA isoform, SOD1 LUTI . Expression of SOD1 LUTI is induced by the Unfolded Protein Response, and it acts to repress canonical SOD1 mRNA expression. SOD1 LUTI is no longer expressed following the meiotic divisions, enabling a resurgence of canonical mRNA and synthesis of new Sod1 protein such that gametes inherit a full complement of this important enzyme that is essential for gamete viability. Altogether, this work reveals meiosis to be an unusual cellular context in which Sod1 levels are tightly regulated. Our findings also suggest that further investigation of Sod1 during yeast gametogenesis could shed light on conserved aspects of its aggregation and degradation that could have implications for our understanding of human disease.

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last seen: 2026-05-19T01:45:01.086888+00:00