Light-dependent Phosphorylation of the Drosophila Transient Receptor Potential Ion Channel

Voolstra, Olaf; Beck, Katherina; Oberegelsbacher, Claudia; Pfannstiel, Jens; Huber, Armin

doi:10.1074/jbc.m110.102053

Cited by 38 publications

(24 citation statements)

References 50 publications

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“…A third potential role for phosphorylation of the MSL10 N-terminal domain is in the regulation of its ion channel properties, as has been shown for TPK1 (Latz et al, 2007), TRP (Voolstra et al, 2010), CLH-3b (Yamada et al, 2013), and PIP2 (Prado et al, 2013). Mutations outside the membrane-spanning pore of bacterial MscS homologs alter channel conductance Cox et al, 2013) and gating properties (Nomura et al, 2008;Vásquez et al, 2008;Belyy et al, 2010;Koprowski et al, 2011).…”

Section: Preventing or Mimicking Phosphorylation Of The Msl10 N-termimentioning

confidence: 99%

Arabidopsis MSL10 Has a Regulated Cell Death Signaling Activity That Is Separable from Its Mechanosensitive Ion Channel Activity

et al. 2014

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Members of the MscS superfamily of mechanosensitive ion channels function as osmotic safety valves, releasing osmolytes under increased membrane tension. MscS homologs exhibit diverse topology and domain structure, and it has been proposed that the more complex members of the family might have novel regulatory mechanisms or molecular functions. Here, we present a study of MscS-Like (MSL)10 from Arabidopsis thaliana that supports these ideas. High-level expression of MSL10-GFP in Arabidopsis induced small stature, hydrogen peroxide accumulation, ectopic cell death, and reactive oxygen species-and cell death-associated gene expression. Phosphomimetic mutations in the MSL10 N-terminal domain prevented these phenotypes. The phosphorylation state of MSL10 also regulated its ability to induce cell death when transiently expressed in Nicotiana benthamiana leaves but did not affect subcellular localization, assembly, or channel behavior. Finally, the N-terminal domain of MSL10 was sufficient to induce cell death in tobacco, independent of phosphorylation state. We conclude that the plant-specific N-terminal domain of MSL10 is capable of inducing cell death, this activity is regulated by phosphorylation, and MSL10 has two separable activities-one as an ion channel and one as an inducer of cell death. These findings further our understanding of the evolution and significance of mechanosensitive ion channels.

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Section: Preventing or Mimicking Phosphorylation Of The Msl10 N-termimentioning

confidence: 99%

Arabidopsis MSL10 Has a Regulated Cell Death Signaling Activity That Is Separable from Its Mechanosensitive Ion Channel Activity

et al. 2014

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“…Mass Spectrometry-Mass spectrometry and data analysis was performed as described before (10), except that a longer gradient (90 min) was used for peptide elution from the HPLC column, survey spectra were recorded in the Orbitrap detector in the m/z range of 250 to 2000, and data-dependent tandem mass spectra were generated for the seven most abundant peptide precursors in the linear ion trap. Mascot 2.3 (Matrix Science) and Sequest (Thermo Fisher Scientific) search results were loaded into Proteome Discoverer 1.3 (Thermo Fisher Scientific) for verification.…”

Section: Methodsmentioning

confidence: 99%

“…Gel Electrophoresis and Immunoblot Analysis-Protein extracts were generated as described (10). 4 l of SDS extraction buffer was used per fly head, and extraction at room temperature was extended to 1 h. Immunoblot analysis was carried out as described (10) using anti-TRPL (12) and anti-␤-tubulin antibodies (Developmental Studies Hybridoma Bank, University of Iowa).…”

Section: Methodsmentioning

confidence: 99%

“…Immunoprecipitation of TRPL Channels-Protein extracts of 80 fly heads per sample for immunoprecipitation with ␣-GFP or 300 fly heads per sample for immunoprecipitation with ␣-TRPL were obtained as described (10). 2 l of extraction buffer was used per fly head.…”

Section: Methodsmentioning

confidence: 99%

“…The founding member of the TRP protein family, the Drosophila TRP channel, together with its homolog TRPL (TRP-like) is expressed in photoreceptor cells of the fly compound eye and generates the receptor potential in the visual transduction cascade (7)(8)(9). A mass spectrometry analysis of posttranslational TRP modifications identified 21 phosphorylation sites (10). One of the light-dependent phosphorylation sites of TRP, Ser-982, was shown to be critical for the proper deactivation of the photoresponse (11), whereas the physiological function of the other phosphorylation sites is still elusive.…”

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confidence: 99%

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Mutation of Light-dependent Phosphorylation Sites of the Drosophila Transient Receptor Potential-like (TRPL) Ion Channel Affects Its Subcellular Localization and Stability

Cerny

Oberacker

Pfannstiel

et al. 2013

Journal of Biological Chemistry

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Background: Drosophila TRPL is a cation channel of the phototransduction cascade that undergoes light-dependent subcellular translocation between cell compartments. Results: Drosophila TRPL exhibits a light-dependent phosphorylation pattern required for its stable localization in the rhabdomere of photoreceptor cells. Conclusion: Multiple phosphorylation sites control localization and stability of TRPL. Significance: A member of the TRP ion channel family displays a complex phosphorylation pattern with functional relevance.

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Solubility and subcellular localization of the three Drosophila RDGC phosphatase variants are determined by acylation

et al. 2018

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Protein phosphorylation is an abundant molecular switch that regulates a multitude of cellular processes. In contrast to other subfamilies of phosphoprotein phosphatases, the PPEF subfamily is only poorly investigated. Drosophila retinal degeneration C (RDGC) constitutes the founding member of the PPEF subfamily. RDGC dephosphorylates the visual pigment rhodopsin and the ion channel TRP.However, rdgC null mutant flies exhibit rhodopsin and TRP hyperphosphorylation, altered photoreceptor physiology, and retinal degeneration. Here, we report the identification of a third RDGC protein variant and show that the three RDGC isoforms harbor different N-termini that determine solubility and subcellular targeting due to fatty acylation. Taken together, solubility and subcellular targeting of RDGC splice variants are determined by their N-termini.

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Light-dependent Phosphorylation of the Drosophila Transient Receptor Potential Ion Channel

Cited by 38 publications

References 50 publications

Arabidopsis MSL10 Has a Regulated Cell Death Signaling Activity That Is Separable from Its Mechanosensitive Ion Channel Activity

Arabidopsis MSL10 Has a Regulated Cell Death Signaling Activity That Is Separable from Its Mechanosensitive Ion Channel Activity

Mutation of Light-dependent Phosphorylation Sites of the Drosophila Transient Receptor Potential-like (TRPL) Ion Channel Affects Its Subcellular Localization and Stability

Solubility and subcellular localization of the three Drosophila RDGC phosphatase variants are determined by acylation

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