4. Modes of aquaporin regulation4.1

4. Modes of aquaporin regulation
4.1. Cotranslational and posttranslational modifications
Application over the last 10 years ofwell-developed proteomics and
mass spectrometry techniques have led to a comprehensive description
of cotranslational and posttranslational modifications of plant aquaporins
in their native membranes [54,59–61]. Combined with in vivo and
in vitro labeling studies, these approaches have indicated that PIP1s
and PIP2s from various species can be phosphorylated at multiple
sites on the N-terminal or C-terminal tail, respectively. In addition,
various environmental conditions such as drought, salinity or oxidative
stresses induce quantitative changes in PIP, TIP or NIP phosphorylation
[20,59,61–63]. However, knowledge of the protein kinases and protein
phosphatases determining reversible aquaporin phosphorylation is
still scarce [64,65]. Whereas aquaporin phosphorylation is very
common, glycosylation was identified in only a few homologs such as
soybean GmNOD26 and a TIP from Mesembryanthemum crystallinum
(ice plant) [66,67]. First evidence for methylation in aquaporins,
and even plant membrane proteins, was obtained with Arabidopsis
AtPIP2;1, Lys3 and Glu6 of which were di- and monomethylated,
respectively [68]. Altogether, these studies suggest that intricate
co- and post-translational regulation mechanisms regulate plant
aquaporins (Fig. 1). However, we are far from having a comprehensive view of how the numerous environmental or hormonal signals that
intervene during plant growth and development target, in time and
space, the multiple aquaporin isoforms expressed throughout the plant.