Elaboration of a novel technique for purification of plasma membranes from <i>Xenopus laevis</i> oocytes

Leduc‐Nadeau, Alexandre; Lahjouji, Karim; Bissonnette, Pierre; Lapointe, Jean‐Yves; Bichet, Daniel G.

doi:10.1152/ajpcell.00136.2006

Cited by 37 publications

(40 citation statements)

References 22 publications

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“…To this end we used Jacobson's pellicle method [46]. Intact cells (oocytes or CHO) were treated with cationic silica to coat the exterior of the plasma membranes [47,48]. The colloidal silica particles were then crosslinked by polyacrylic acid.…”

Section: Discussionmentioning

confidence: 99%

The monomeric state of the proton‐coupled folate transporter represents the functional unit in the plasma membrane

et al. 2013

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Folic acid is an essential vitamin required for de novo biosynthesis of nucleotides and amino acids. The proton-coupled folate transporter (PCFT; SLC46A1) has been identified as the major contributor for intestinal folate uptake. It is also involved in folate transport across the blood-brain barrier and into solid tumors. PCFT belongs to the major facilitator superfamily. Major facilitator superfamily members can exist in either monomeric or homo-oligomeric form. Here, we utilized blue native polyacrylamide gel electrophoresis (BN/PAGE) and crosslinking with bi-functional chemicals to investigate the quaternary structure of human PCFT after heterologous expression in Xenopus laevis oocytes and CHO cells. PCFT was expressed in the plasma membrane in both expression systems. The functionality of the utilized PCFT construct was confirmed in oocytes by folic acid induced currents at acidic pH. For both the oocyte and CHO expression system [ 3 H]folic acid uptake studies indicated that PCFT was functional. To analyze the oligomeric state of PCFT in the plasma membrane, plasma membranes were isolated by polymerization with colloidal silica and polyacrylic acid and subsequent centrifugation. The digitoninsolubilized non-denatured PCFT migrated during BN/PAGE as a monomer, as judged by comparison with a membrane protein (5-HT 3A receptor) of known pentameric assembly that was used to create a molecular sizing ladder. The chemical crosslinkers glutaraldehyde and dimethyl adipimidate were not able to covalently link potential higher order PCFT structures to form oligomers that were stable following SDS treatment. Together, our results demonstrate that plasma-membrane PCFT functions as a monomeric protein.

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Section: Discussionmentioning

confidence: 99%

The monomeric state of the proton‐coupled folate transporter represents the functional unit in the plasma membrane

et al. 2013

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“…Oocyte membranes were purified using a modification of a technique described by Leduc-Nadeau et al (18). In brief, for the preparation of total membranes, five oocytes were homogenized in 1 ml buffer (HbAϩ: 5 mM MgCl2, 5 mM NaH2PO4, 1 mM EDTA, 80 mM sucrose, 20 mM Tris, pH 7.48, and 8 M leupeptin, and 0.4 mM Pefabloc).…”

Section: Methodsmentioning

confidence: 99%

Role of multiple phosphorylation sites in the COOH-terminal tail of aquaporin-2 for water transport: evidence against channel gating

Moeller¹,

MacAulay²,

Knepper³

et al. 2009

American Journal of Physiology-Renal Physiology

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Moeller HB, MacAulay N, Knepper MA, Fenton RA. Role of multiple phosphorylation sites in the COOH-terminal tail of aquaporin-2 for water transport: evidence against channel gating. Am J Physiol Renal Physiol 296: F649 -F657, 2009. First published January 14, 2009 doi:10.1152/ajprenal.90682.2008.-Arginine vasopressin (AVP)-regulated phosphorylation of the water channel aquaporin-2 (AQP2) at serine 256 (S256) is essential for its accumulation in the apical plasma membrane of collecting duct principal cells. In this study, we examined the role of additional AVP-regulated phosphorylation sites in the COOH-terminal tail of AQP2 on protein function. When expressed in Xenopus laevis oocytes, prevention of AQP2 phosphorylation at S256A (S256A-AQP2) reduced osmotic water permeability threefold compared with wild-type (WT) AQP2-injected oocytes. In contrast, prevention of AQP2 single phosphorylation at S261 (S261A), S264 (S264A), and S269 (S269A), or all three sites in combination had no significant effect on water permeability. Similarly, oocytes expressing S264D-AQP2 and S269D-AQP2, mimicking AQP2 phosphorylated at these residues, had similar water permeabilities to WT-AQP2-expressing oocytes. The use of high-resolution confocal laser-scanning microscopy, as well as biochemical analysis demonstrated that all AQP2 mutants, with the exception of S256A-AQP2, had equal abundance in the oocyte plasma membrane. Correlation of osmotic water permeability relative to plasma membrane abundance demonstrated that lack of phosphorylation at S256, S261, S264, or S269 had no effect on AQP2 unit water transport. Similarly, no effect on AQP2 unit water transport was observed for the 264D and 269D forms, indicating that phosphorylation of the COOH-terminal tail of AQP2 is not involved in gating of the channel. The use of phosphospecific antibodies demonstrated that AQP2 S256 phosphorylation is not dependent on any of the other phosphorylation sites, whereas S264 and S269 phosphorylation depend on prior phosphorylation of S256. In contrast, AQP2 S261 phosphorylation is independent of the phosphorylation status of S256. water channel; vasopressin; NDI; kidney AQUAPORIN-2 (AQP2) is a vasopressin-regulated water channel expressed in the principal cells of the kidney collecting duct. In the absence of vasopressin (AVP), AQP2-containing vesicles localize to subapical regions of the cell. Binding of AVP to the basolaterally localized type 2 vasopressin receptor initiates a signaling cascade resulting in increased intracellular cAMP, activation of PKA, phosphorylation of AQP2, and subsequent insertion of the water channel into the apical plasma membrane. This event, rendering the cell more permeable to water, is essential for water reabsorption by the collecting duct and thereby for concentrating the urine. Upon removal of AVP, AQP2 is retrieved from the membrane by endocytosis. Thus the abundance of AQP2 in the apical membrane is a regulated balance between exocytosis and endocytosis.Protein phosphorylation and dephosphorylation are common, re...

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“…Briefly, the coding region of HvPIP2;5 cDNAs was sub-cloned into pXbG-ev1, and corresponding cRNA was synthesized and injected into oocytes. Total membranes of oocytes expressing HvPIP2;5 protein were extracted according to Leduc-Nadeau et al (2007). All membrane protein corresponding to one oocyte was used as a sample and subjected to solubilization, SDS-PAGE and Western blotting as described previously (Katsuhara et al, 2002).…”

Section: Generation Of Antibodies Against Aqps Protein Expression Inmentioning

confidence: 99%

Exogenous application of abscisic acid (ABA) increases root and cell hydraulic conductivity and abundance of some aquaporin isoforms in the ABA-deficient barley mutant Az34

Sharipova

Веселов

Kudoyarova

et al. 2016

Ann Bot

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Background and Aims Regulation of water channel aquaporins (AQPs) provides another mechanism by which abscisic acid (ABA) may influence water flow through plants. To the best of our knowledge, no studies have addressed the changes in ABA levels, the abundance of AQPs and root cell hydraulic conductivity (Lp Cell ) in the same tissues. Thus, we followed the mechanisms by which ABA affects root hydraulics in an ABA-deficient barley mutant Az34 and its parental line 'Steptoe'. We compared the abundance of AQPs and ABA in cells to determine spatial correlations between AQP abundance and local ABA concentrations in different root tissues. In addition, abundance of AQPs and ABA in cortex cells was related to Lp Cell.Methods Root hydraulic conductivity (Lp Root ) was measured by means of root exudation analyses and Lp Cell using a cell pressure probe. The abundance of ABA and AQPs in root tissues was assessed through immunohistochemical analyses. Isoform-specific antibodies raised against HvPIP2;1, HvPIP2;2 and HvPIP2;5 were used.Key Results Immunolocalization revealed lower ABA levels in root tissues of Az34 compared with 'Steptoe'. Root hydraulic conductivity (Lp Root ) was lower in Az34, yet the abundance of HvPIPs in root tissues was similar in the two genotypes. Root hair formation occurred closer to the tip, while the length of the root hair zone was shorter in Az34 than in 'Steptoe'. Application of external ABA to the root medium of Az34 and 'Steptoe' increased the immunostaining of root cells for ABA and for HvPIP2;1 and HvPIP2;2 especially in root epidermal cells and the cortical cell layer located beneath, parallel to an increase in Lp Root and Lp Cell . Treatment of roots with Fenton reagent, which inhibits AQP activity, prevented the ABA-induced increase in root hydraulic conductivity.Conclusion Shortly after (<2 h) ABA application to the roots of ABA-deficient barley, increased tissue ABA concentrations and AQP abundance (especially the plasma-membrane localized isoforms HvPIP2;1 and HvPIP2;2) were spatially correlated in root epidermal cells and the cortical cell layer located beneath, in conjunction with increased Lp Cell of the cortical cells. In contrast, long-term ABA deficiency throughout seedling development affects root hydraulics through other mechanisms, in particular the developmental timing of the formation of root hairs closer to the root tip and the length of the root hair zone.

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Elaboration of a novel technique for purification of plasma membranes from Xenopus laevis oocytes

Cited by 37 publications

References 22 publications

The monomeric state of the proton‐coupled folate transporter represents the functional unit in the plasma membrane

The monomeric state of the proton‐coupled folate transporter represents the functional unit in the plasma membrane

Role of multiple phosphorylation sites in the COOH-terminal tail of aquaporin-2 for water transport: evidence against channel gating

Exogenous application of abscisic acid (ABA) increases root and cell hydraulic conductivity and abundance of some aquaporin isoforms in the ABA-deficient barley mutant Az34

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