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Raw Western blot images from Fig 8 [Dataset]

Authors: Ferré, Alba; Chauvigné, François; Zapater, Cinta; Finn, Roderick N.; Cerdà, Joan;

Raw Western blot images from Fig 8 [Dataset]

Abstract

Aquaporin-mediated oocyte hydration is a developmentally regulated adaptive mechanism that co-occurs with meiosis resumption in marine teleosts. It provides the early embryos with vital water until osmoregulatory systems develop, and in the majority of marine teleosts causes their eggs to float. Recent studies have shown that the subdomains of two water channels (Aqp1ab1 and Aqp1ab2) encoded in a teleost-specific aquaporin-1 cluster (TSA1C) co-evolved with duplicated Ywhaz-like (14-3-3ζ-like) binding proteins to differentially control their membrane trafficking for maximal egg hydration. Here, we report that in species that encode the full TSA1C, in-frame intronic splice variants of Aqp1ab1 result in truncated proteins that cause dominant-negative inhibition of the canonical channel trafficking to the plasma membrane. The inhibition likely occurs through hetero-oligomerization and retention in the endoplasmic reticulum (ER) and ultimate degradation. Conversely, in species that only encode the Aqp1ab2 channel we found an in-frame intronic splice variant that results in an intact protein with an extended extracellular loop E, and an out-of frame intronic splice variant with exon readthrough that results in a truncated protein. Both isoforms cause dominant-negative enhancement of the degradation pathway. However, the extended and truncated Aqp1ab2-type variants can also partially escape from the ER to reach the oocyte plasma membrane, where they dominantly-negatively inhibit water flux. The ovarian follicular expression ratios of the Aqp1ab2 isoforms in relation to the canonical channel are lowest during oocyte hydration, but subsequently highest when the canonical channel is recycled, thus leaving the eggs endowed with >90% water. These findings suggest that the expression of inhibitory isoforms of Aqp1ab1 and Aqp1ab2 may represent a new regulatory mechanism through which the cell-surface expression and the activity of the canonical channels can be physiologically modulated during oocyte hydration in marine teleosts.

With the institutional support of the ‘Severo Ochoa Centre of Excellence’ accreditation (CEX2019-000928-S).

Peer reviewed

Keywords

Truncated proteins, aqp1ab2 isoforms, Marine teleosts, Aqp1ab2 may represent, Maximal egg hydration, Osmoregulatory systems develop, Inhibition likely occurs, Membrane trafficking, Truncated aqp1ab2, Canonical channels, Thus leaving, Vital water, 1 cluster, Negative inhibition, Ultimate degradation, Oocyte hydration, Also partially escape, Canonical channel trafficking, Canonical channel, Duplicated ywhaz, Truncated protein, Meiosis resumption, Differentially control, Binding proteins, Cause dominant, Specific aquaporin, New regulatory mechanism, Inhibitory isoforms, Findings suggest, Type variants, Isoforms cause dominant, Intact protein, Degradation pathway, Exon readthrough, Marine teleosts causes, Two water channels, Mediated oocyte hydration, Physiologically modulated, Oocyte plasma membrane, Negative enhancement, aqp1ab2 channel, Recent studies, Xink "> aquaporin, Endoplasmic reticulum, Plasma membrane, Subsequently highest, Early embryos

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This is an alternative to the "Influence" indicator, which also reflects the overall/total impact of an article in the research community at large, based on the underlying citation network (diachronically).
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popularity
This indicator reflects the "current" impact/attention (the "hype") of an article in the research community at large, based on the underlying citation network.
BIP!Popularity provided by BIP!
influence
This indicator reflects the overall/total impact of an article in the research community at large, based on the underlying citation network (diachronically).
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impulse
This indicator reflects the initial momentum of an article directly after its publication, based on the underlying citation network.
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