Functional characterization and cell immunolocalization of AQP-CD water channel in kidney collecting duct

Vasopressin-regulated water permeability of the kidney collecting duct is a key component of the urine concentration machinery. Recently, a cDNA for AQP-CD, the vasopressin-regulated water channel, initially reported as WCH-CD, has been isolated (K. Fushimi, S. Uchida, Y. Hara, Y. Hirata, F. Marumo, and S. Sasaki. Nature Lond. 361: 549-552, 1993). AQP-CD was expressed in oocyte membrane using a Xenopus expression vector, and functional characteristics of AQP-CD were examined. Osmotic water permeability (Pf) of oocytes expressing AQP-CD was 138 +/- 19 microns/s (mean +/- SE), 12 times greater than the control (11 +/- 3 microns/s), 90% inhibited by 0.3 mM HgCl2, and weakly temperature dependent (energy of activation for Pf was 4.0 kcal/mol). Urea influx measured from 15-min [14C]urea uptake by oocytes injected with AQP-CD/expression vector 1 cRNA was 86 +/- 17% of the control. Two-electrode voltage-clamp experiments revealed insignificant ion conductance of AQP-CD. Immunoblots of membranes from rat kidney medulla and oocytes expressing AQP-CD using anti-AQP-CD COOH-terminal antibody showed a 29-kDa protein and 35- to 50-kDa high-molecular-mass forms. Immunohistochemistry showed apical and subapical localization of AQP-CD in the collecting duct principal cells. Our results indicated that AQP-CD is a 29-kDa protein, a selective water channel, distinct from a urea channel, and localized to the membranes of vasopressin-sensitive components in kidney collecting duct principal cells.

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Expression, functional analysis, and in situ hybridization of a cloned rat kidney collecting duct water channel

AJP Cell Physiology ◽

10.1152/ajpcell.1994.266.1.c189 ◽

1994 ◽

Vol 266 (1) ◽

pp. C189-C197 ◽

Cited By ~ 45

Author(s):

T. Ma ◽

H. Hasegawa ◽

W. R. Skach ◽

A. Frigeri ◽

A. S. Verkman

Keyword(s):

Base Pair ◽

Collecting Duct ◽

Rat Kidney ◽

Water Channel ◽

Cloning And Expression ◽

Base Pairs ◽

Kidney Medulla ◽

Coding Sequence ◽

Kidney Collecting Duct ◽

Protein Size

The cloning and expression of an apical membrane water channel from rat kidney collecting duct (WCH-CD) homologous to a 28-kDa integral membrane protein (CHIP28) was reported recently (K. Fushimi, S. Uchida, Y. Hara, Y. Hirata, F. Marumo, and S. Sasaki. Nature Lond. 361: 549-552, 1993). We obtained an approximately 1.8-kilobase clone from a rat kidney lambda gt10 cDNA library by a polymerase chain reaction cloning method; whereas the coding sequence (814 base pairs, predicted protein size 29 kDa) was identical to that reported, we identified an in-frame ATG codon at base pair -123 predicting a protein size of 33 kDa. On Northern blots probed by cDNAs corresponding to the WCH-CD coding sequence (base pairs +1 to +814) or 5'-untranslated sequence (-403 to -16), a single band at 1.9 kilobases was observed in kidney medulla greater than in cortex but not in other tissues; mRNA expression was increased strongly by dehydration. Translation and oocyte expression studies were performed to identify the translation start site. The short (base pairs +1 to +814) and long (base pairs -123 to +814) cDNAs were subcloned in vector pSP64 containing the 5'-untranslated Xenopus globin sequence upstream to the ATGs; a 30-base pair c-myc sequence was engineered at the COOH- terminal for antibody recognition.(ABSTRACT TRUNCATED AT 250 WORDS)

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Endocytic vesicles from renal papilla which retrieve the vasopressin-sensitive water channel do not contain a functional H+ ATPase.

The Journal of Cell Biology ◽

10.1083/jcb.111.2.379 ◽

1990 ◽

Vol 111 (2) ◽

pp. 379-389 ◽

Cited By ~ 35

Author(s):

W I Lencer ◽

A S Verkman ◽

M A Arnaout ◽

D A Ausiello ◽

D Brown

Keyword(s):

Plasma Membrane ◽

Water Permeability ◽

Collecting Duct ◽

Water Channel ◽

Water Channels ◽

Proton Pumps ◽

Principal Cells ◽

Kidney Collecting Duct ◽

Fluorescence Imaging Microscopy ◽

Membrane Components

The water permeability of the kidney collecting duct epithelium is regulated by vasopressin (VP)-induced recycling of water channels between an intracellular vesicular compartment and the plasma membrane of principal cells. To test whether the water channels pass through an acidic endosomal compartment during the endocytic portion of this pathway, we measured ATP-dependent acidification of FITC-dextran-labeled endosomes in isolated microsomal fractions from different regions of Brattleboro rat kidneys. Both VP-deficient controls and rat treated with exogenous VP were examined. ATP-dependent acidification was not detectable in endosomes containing water channels from distal papilla (osmotic water permeability Pf = 0.038 +/- 0.004 cm/s). In contrast, the addition of ATP resulted in a strong acidification of renal cortical endosomes (pHmin = 5.8, initial rate = 0.18-0.25 pH U/s). Acidification of cortical endosomes was reversed with nigericin and strongly inhibited by N-ethyl-maleimide. Passive proton permeability was similar and low in both cortical and papillary endosomes from rats treated or not treated with VP. The fraction of labeled endosomes present in microsomal preparations was determined by fluorescence imaging microscopy of microsomes nonspecifically bound to poly-l-lysine-coated coverslips and was 25% in cortical preparations compared to 14% (+VP) and 9% (-VP) in papillary preparations. The fraction of cortical endosomes was enriched 1.5-fold by immunoabsorption to coverslips coated with mAbs against the bovine vacuolar proton pump. In contrast, the fraction of papillary endosomes was depleted more than twofold by immunoabsorption to identical coverslips. Finally, sections of distal papilla stained with antibodies against the lysosomal glycoprotein LGP120 showed that most of the entrapped FITC-dextran did not colocalize with this lysosomal protein. These results demonstrate that vesicles which internalize water channels in kidney collecting duct principal cells lack functional proton pumps, and do not deliver the bulk of their FITC-dextran content to lysosomes. The data suggest that the principal cell contains a specialized nonacidic apical endocytic compartment which functions primarily to recycle membrane components, including water channels, to the plasma membrane.

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Endocytosis of water channels in rat kidney: cell specificity and correlation with in vivo antidiuresis

AJP Cell Physiology ◽

10.1152/ajpcell.1990.259.6.c920 ◽

1990 ◽

Vol 259 (6) ◽

pp. C920-C932 ◽

Cited By ~ 24

Author(s):

W. I. Lencer ◽

D. Brown ◽

D. A. Ausiello ◽

A. S. Verkman

Keyword(s):

Water Permeability ◽

Collecting Duct ◽

Rat Kidney ◽

Water Channel ◽

Water Channels ◽

Intercalated Cells ◽

Principal Cells ◽

Osmotic Water ◽

Principal And Intercalated Cells

Vasopressin action in the renal collecting duct is believed to be mediated by the cycling of water channels in principal and, possibly, intercalated cells. We used 6-carboxyfluorescein (6-CF) or fluorescein-labeled dextran (FITC-dextran) to determine the location and water permeability of endocytic vesicles from papilla and inner stripe of Brattleboro rats in different states of diuresis. Fifteen minutes after FITC-dextran infusion, fluorescent vesicles were concentrated at the apical pole of principal and intercalated cells. The osmotic water permeability (Pf) of these endosomes was measured by fluorescence quenching. In papillary endosomes, Pf was high (0.04 +/- 0.004 cm/s) when rats were in physiological states of antidiuresis or after treatment with vasopressin, 1-desamino-8-D-arginine vasopressin (DDAVP), or oxytocin; endosomes isolated from these regions of untreated animals had a low Pf. The number of papillary endosomes with high Pf increased with increasing doses of DDAVP. Endosomes from the inner stripe also had a high Pf only after vasopressin treatment. Confocal microscopy of sections of papilla showed that vasopressin significantly increased endocytosis in principal cells but had no effect on intercalated cells. Our data demonstrate that the bulk of fluorescently labeled vesicles from the papilla originate from the apical membrane of principal cells and contain water channels in their limiting membrane only when the rats are in physiological states of antidiuresis. In contrast, the majority of endocytosis in intercalated cells is not involved in water channel recycling.

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Immunocytochemical localization of Na+ channels in rat kidney medulla

AJP Renal Physiology ◽

10.1152/ajprenal.1989.256.2.f366 ◽

1989 ◽

Vol 256 (2) ◽

pp. F366-F369 ◽

Cited By ~ 3

Author(s):

D. Brown ◽

E. J. Sorscher ◽

D. A. Ausiello ◽

D. J. Benos

Keyword(s):

Plasma Membrane ◽

Plasma Membranes ◽

Collecting Duct ◽

Rat Kidney ◽

Apical Plasma Membrane ◽

Na Channel ◽

Thick Ascending Limb ◽

Na Channels ◽

Kidney Medulla ◽

Principal Cells

Amiloride-sensitive Na+ channels were localized in semithin frozen sections of rat renal medullary collecting ducts, using polyclonal antibodies directed against purified bovine kidney Na+ channel protein. The apical plasma membrane of collecting duct principal cells was heavily stained by indirect immunofluorescence, whereas intercalated cells were negative. Basolateral plasma membranes of both cell types were unstained, as were subapical vesicles in the cytoplasm of these cells. In the thick ascending limb of Henle, some scattered granular fluorescence was seen in the cytoplasm and close to the apical pole of epithelial cells, suggesting the presence of antigenic sites associated with some membrane domains in these cells. No staining was detected in thin limbs of Henle, or in proximal tubules in the outer medulla. These results show that amiloride-sensitive sodium channels are located predominantly on the apical plasma membrane of medullary collecting duct principal cells, the cells that are involved in Na+ homeostasis in this region of the kidney.

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Immunolocalization and effect of dehydration on AQP3, a basolateral water channel of kidney collecting ducts

AJP Renal Physiology ◽

10.1152/ajprenal.1997.272.2.f235 ◽

1997 ◽

Vol 272 (2) ◽

pp. F235-F241 ◽

Cited By ~ 15

Author(s):

K. Ishibashi ◽

S. Sasaki ◽

K. Fushimi ◽

T. Yamamoto ◽

M. Kuwahara ◽

...

Keyword(s):

Xenopus Oocytes ◽

Collecting Duct ◽

Basolateral Membrane ◽

Broad Band ◽

Water Channel ◽

In Vitro Translation ◽

Mercury Chloride ◽

Channel Activity ◽

Kidney Medulla ◽

Principal Cells

Aquaporin-3 (AQP3) is unique in its structure (lowest homology with other aquaporins) and in its function (significantly conductive to both small nonelectrolytes and water). However, there is a controversy among researchers on its water transport and induction by dehydration. We examined its localization and the effect of dehydration on its expression in the kidney, as well as its water channel activity when expressed in Xenopus oocytes. In vitro translation using reticulocyte lysate revealed that the size of rat AQP3 was 26 kDa, and the band shifted to around 31 kDa with microsomal fraction, which was sensitive to the digestion with N-glycosidase F. In Western blot analysis of rat kidney medulla, AQP3 appeared as a sharp band at 27 kDa and a broad band at 34-40 kDa. In immunohistochemistry, AQP3 was localized to principal cells and absent in intercalated cells in outer medulla. In inner medulla, AQP3 was restricted to inner medullary collecting duct (IMCD) cells. AQP3 was confined to the basolateral membrane of these cells. Although dehydration of rats for 2 days did not change the distribution pattern of AQP3 in IMCD cells, the dehydration increased AQP3 mRNA by twofold with slight increase of its protein level in kidney medulla. Finally, we confirmed its water channel activity when expressed in Xenopus oocytes. The human AQP3 stimulated osmotic water permeability by eightfold, which was inhibited by 0.3 mM mercury chloride by 34% and reversed by beta-mercaptoethanol. Our results indicate that AQP3 is a glycosylated protein and a mercury-sensitive water channel localized at the basolateral membrane of principal cells and IMCD cells, and its expression is induced by dehydration at both protein and mRNA level.

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Localization of MIWC and GLIP water channel homologs in neuromuscular, epithelial and glandular tissues

Journal of Cell Science ◽

10.1242/jcs.108.9.2993 ◽

1995 ◽

Vol 108 (9) ◽

pp. 2993-3002 ◽

Cited By ~ 9

Author(s):

A. Frigeri ◽

M.A. Gropper ◽

F. Umenishi ◽

M. Kawashima ◽

D. Brown ◽

...

Keyword(s):

Electron Microscopy ◽

Urinary Bladder ◽

Collecting Duct ◽

Basolateral Membrane ◽

Water Channel ◽

Parietal Cells ◽

Immunogold Electron Microscopy ◽

Transitional Epithelium ◽

Principal Cells ◽

Kidney Collecting Duct

It was shown recently that water channel homologs MIWC (mercurial insensitive water channel) and GLIP (glycerol intrinsic protein) colocalized in basolateral membranes of kidney collecting duct, tracheal and colonic epithelia, and in brain pia mater. We report here an extensive immunolocalization study of MIWC and GLIP in non-epithelial and glandular epithelial tissues in rat. Immunogold electron microscopy confirmed colocalization of MIWC and GLIP in basolateral membrane of principal cells in kidney collecting duct. However, in other epithelia, MIWC but not GLIP was expressed in basolateral membrane of parietal cells in stomach, and in excretory tubules of salivary and lacrimal glands; GLIP but not MIWC was expressed in transitional epithelium of urinary bladder and skin epidermis. In the central nervous system, MIWC was strongly expressed in the ependymal layer lining the aqueductal system, and in astrocytes throughout the spinal cord and in selected regions of brain. MIWC was also expressed in a plasma membrane pattern in skeletal, but not smooth or cardiac muscle. Neither protein was expressed in small intestine, testis, liver, spleen and nerve. The tissue-specific expression of MIWC suggests a role in fluid transport and/or cell volume regulation in stomach and glandular epithelia. The functional role of MIWC expression in the neuromuscular system and of GLIP expression in skin and urinary bladder is uncertain. The specific cellular sites of MIWC expression (astrocytes, trachea, sarcolemma, gastric parietal cells and kidney principal cells) correspond exactly to sites where orthogonal arrays of particles (OAPs) have been visualized by freeze-fracture electron microscopy, suggesting that MIWC may be the OAP protein.

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Molecular and functional characterization of a vasotocin-sensitive aquaporin water channel in quail kidney

AJP Regulatory Integrative and Comparative Physiology ◽

10.1152/ajpregu.00589.2003 ◽

2004 ◽

Vol 287 (4) ◽

pp. R915-R924 ◽

Cited By ~ 10

Author(s):

Y. Yang ◽

Y. Cui ◽

W. Wang ◽

L. Zhang ◽

L. Bufford ◽

...

Keyword(s):

Water Permeability ◽

Early Stage ◽

Collecting Duct ◽

Functional Characterization ◽

Water Channel ◽

Arginine Vasotocin ◽

Mercury Chloride ◽

Xenopus Laevis Oocytes ◽

Mrna Levels ◽

Rt Pcr

Both mammals and birds can concentrate urine hyperosmotic to plasma via a countercurrent multiplier mechanism, although evolutionary lines leading to mammals and birds diverged at an early stage of tetrapod evolution. We reported earlier (Nishimura H, Koseki C, and Patel TB. Am J Physiol Regul Integr Comp Physiol 271: R1535–R1543, 1996) that arginine vasotocin (AVT; avian antidiuretic hormone) increases diffusional water permeability in the isolated, perfused medullary collecting duct (CD) of the quail kidney. In the present study, we have identified an aquaporin (AQP) 2 homolog water channel in the medullary cones of Japanese quail, Coturnix coturnix (qAQP2), by RT-PCR-based cloning techniques. A full-length cDNA contains an 822-bp open reading frame that encodes a 274-amino acid sequence with 75.5% identity to rat AQP2. The qAQP2 has six transmembrane domains, two asparagine-proline-alanine (NPA) sequences, and putative N-glycosylation (asparagine-124) and phosphorylation sites (serine-257) for cAMP-dependent protein kinase. qAQP2 is expressed in the membrane of Xenopus laevis oocytes and significantly increased its osmotic water permeability (Pf), inhibitable ( P < 0.01) by mercury chloride. qAQP2 mRNA (RT-PCR) was detected in the kidney; medullary mRNA levels were higher than cortical levels. qAQP2 protein that binds to rabbit anti-rat AQP2 antibody is present in the apical/subapical regions of both cortical and medullary CDs from normally hydrated quail, and the intensity of staining increased only in the medullary CDs after water deprivation or AVT treatment. The relative density of the ∼29-kDa protein band detected by immunoblot from the medullary cones was modestly higher in water-deprived/AVT-treated quail. The results suggest that 1) medullary CDs of quail kidneys express a mercury-sensitive functioning qAQP2 water channel, and 2) qAQP2 is at least partly regulated by an AVT-dependent mechanism. This is the first clear identification of AQP2 homolog in nonmammalian vertebrates.

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Cloning and expression of AQP3, a water channel from the medullary collecting duct of rat kidney.

Proceedings of the National Academy of Sciences ◽

10.1073/pnas.91.23.10997 ◽

1994 ◽

Vol 91 (23) ◽

pp. 10997-11001 ◽

Cited By ~ 193

Author(s):

M. Echevarria ◽

E. E. Windhager ◽

S. S. Tate ◽

G. Frindt

Keyword(s):

Collecting Duct ◽

Rat Kidney ◽

Water Channel ◽

Cloning And Expression ◽

Medullary Collecting Duct

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The Vasopressin Receptor 2 Mutant R137L Linked to the Nephrogenic Syndrome of Inappropriate Antidiuresis (NSIAD) Signals through an Alternative Pathway that Increases AQP2 Membrane Targeting Independently of S256 Phosphorylation

Cells ◽

10.3390/cells9061354 ◽

2020 ◽

Vol 9 (6) ◽

pp. 1354

Author(s):

Marianna Ranieri ◽

Maria Venneri ◽

Tommaso Pellegrino ◽

Mariangela Centrone ◽

Annarita Di Mise ◽

...

Keyword(s):

Water Permeability ◽

Collecting Duct ◽

Alternative Pathway ◽

Water Channel ◽

Rho Kinase ◽

Membrane Targeting ◽

Rock Inhibitor ◽

Activating Mutations ◽

Osmotic Water

NSIAD is a rare X-linked condition, caused by activating mutations in the AVPR2 gene coding for the vasopressin V2 receptor (V2R) associated with hyponatremia, despite undetectable plasma vasopressin levels. We have recently provided in vitro evidence that, compared to V2R-wt, expression of activating V2R mutations R137L, R137C and F229V cause a constitutive redistribution of the AQP2 water channel to the plasma membrane, higher basal water permeability and significantly higher basal levels of p256-AQP2 in the F229V mutant but not in R137L or R137C. In this study, V2R mutations were expressed in collecting duct principal cells and the associated signalling was dissected. V2R-R137L and R137C mutants had significantly higher basal pT269-AQP2 levels -independently of S256 and PKA-which were reduced to control by treatment with Rho kinase (ROCK) inhibitor. Interestingly, ROCK activity was found significantly higher in V2R-R137L along with activation of the Gα12/13–Rho–ROCK pathway. Of note, inhibition of ROCK reduced the basal elevated osmotic water permeability to control. To conclude, our data demonstrate for the first time that the gain-of-function mutation of the V2R, R137L causing NSIAD, signals through an alternative PKA-independent pathway that increases AQP2 membrane targeting through ROCK-induced phosphorylation at S/T269 independently of S256 of AQP2.

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Depletion of intercalated cells from collecting ducts of carbonic anhydrase II-deficient (CAR2 null) mice

AJP Renal Physiology ◽

10.1152/ajprenal.1995.269.6.f761 ◽

1995 ◽

Vol 269 (6) ◽

pp. F761-F774 ◽

Cited By ~ 27

Author(s):

S. Breton ◽

S. L. Alper ◽

S. L. Gluck ◽

W. S. Sly ◽

J. E. Barker ◽

...

Keyword(s):

Carbonic Anhydrase ◽

Collecting Duct ◽

Water Channel ◽

Immunofluorescent Staining ◽

Specific Marker ◽

Intercalated Cells ◽

Cortical Collecting Duct ◽

Principal Cells ◽

Collecting Tubules ◽

Deficient Mice

The kidneys of mice (CAR2-null mice) that are genetically devoid of carbonic anhydrase type II (CAII) were screened by immunocytochemistry with antibodies that distinguish intercalated and principal cells. Immunofluorescent localization of the anion exchanger AE1 and of the 56-kDa subunit of the vacuolar H(+)-adenosinetriphosphatase (H(+)-ATPase) was used to identify intercalated cells, while the AQP2 water channel was used as a specific marker for principal cells of the collecting duct. The CAII deficiency of the CAR2-null mice was first confirmed by the absence of immunofluorescent staining of kidney sections exposed to an anti-CAII antibody. Cells positive for AE1 and H(+)-ATPase were common in all collecting duct regions in normal mice but were virtually absent from the inner stripe of the outer medulla and the inner medulla of CAR2-null mice. The number of positive cells was also reduced threefold in the cortical collecting duct of CAR2-null animals compared with normal mice. In parallel, the percentage of AQP2-positive cells was correspondingly increased in the collecting tubules of CAII-deficient mice, whereas the total number of cells per tubule remained unchanged. These results suggest that intercalated cells are severely depleted and are replaced by principal cells in CAII-deficient mice. Quantitative analysis and double staining showed that, in the cortex, both type A and type B intercalated cells are equally affected. Elucidation of the mechanism(s) responsible for this phenotype will be of importance in understanding the origin and development of intercalated cells in the kidney.

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