First published online August 3, 2006
Journal of Experimental Biology 209, 3199-3208 (2006)
Published by The Company of Biologists 2006
doi: 10.1242/jeb.02351
Molecular and cellular characterization of a new aquaporin, AQP-x5, specifically expressed in the small granular glands of Xenopus skin
Makoto Kubota,
Takahiro Hasegawa,
Takashi Nakakura,
Haruna Tanii,
Masakazu Suzuki and
Shigeyasu Tanaka*
Department of Biology, Faculty of Science, Shizuoka University, Ohya
836, Shizuoka 422-8529, Japan
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Fig. 1. (A) Nucleotide and deduced amino acid sequence of Xenopus AQP-x5
cDNA. The predicted amino acid is shown below the nucleotide sequence. The
asterisk indicates the terminal codon. NPA motifs and polyadenylation signal
regions are outlined. The square, diamonds, and open triangles indicate
phosphorylation sites for protein kinase A, protein kinase C and
mercurial-inhibition sites, respectively. (B) Kyte-Doolittle hydropathy
profile (window 11) of the deduced AQP-x5 amino acid sequence.
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Fig. 2. RT-PCR of Xenopus tissue extracts. RT-PCR products using primers
as described in the Materials and methods were separated on a 2% agarose gel
and stained with ethidium bromide. +, mRNA present; -, mRNA absent.
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Fig. 3. Expression of AQP-x5 in Xenopus oocytes. (A) Osmotic water
permeability (Pf) was calculated from the initial rate of oocyte swelling.
Oocytes were microinjected with water or cRNA encoding AQP-x5. A portion of
the AQP-x5-injected oocytes was incubated with 0.3 mmol l-1
HgCl2. All data shown are given as the mean ± s.e.m. of
measurements from 8-11 oocytes (as indicated above the bars) in each
experimental group. *P<0.001 vs water,
**P<0.001 vs AQP-x5. (B) Immunofluorescence
images of AQP-x5 protein in AQP-x5-injected oocytes. (1) After completion of
the swelling experiments, immunoreactive AQP-x5 substances are visible,
predominantly in the plasma membrane. (2) The corresponding Nomarski
differential interference image. (3) In the absorption test, positive
immunoreactive substances obtained with anti-AQP-x5 are nearly eliminated at
background levels in AQP-x5-injected oocyte. (4) As in 3, only background
levels are seen in the water-injected oocyte with anti-AQP-x5. Arrowheads
indicate plasma membrane. Scale bar, 50 µm.
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Fig. 4. Characterization of anti-AQP-x5 serum by western blot analysis. (A)
Immunoreactive bands are seen at 29.0 kDa in an extract of AQP-x5
cRNA-injected oocytes. (B) The membrane was immunostained with the antiserum
preabsorbed with the antigen peptide (10 µg ml-1).
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Fig. 5. Mallory's triple staining of Xenopus skin. In sections treated
with Mallory's triple stain the skin glands can be classified into three
types: the granular gland (g), the mucous gland (m), and the small granular
gland (sg). Scale bar, 50 µm.
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Fig. 6. Immunofluorescence localization of AQP-x5 in the skin glands. (A,C,D)
Fluorescence images of AQP-x5 and (B) the corresponding Nomarski differential
interference contrast image. (A,B) The labels (green; arrows) are clearly
visible in the apical plasma membrane of granular cells in the small granular
glands (sg). Weak positive reaction is visible in the apical plasma membrane
of glandular cells located in upper sides of the mucous glands (arrowheads).
No labeling is seen in the mucous (m) and granular (g) glands. The asterisk in
B indicates red blood cells, displaying a nonspecific label for AQP-x5. (C) No
labeling is detected in any of the cells of the skins when anti-AQP-x5 is
preabsorbed with the corresponding antigen peptide. (D) Double-labeling for
AQP-x5 (green) and V-ATPase E-subunit (red); V-ATPase-expressing cells are
observed among the glandular cells (arrowheads). Nuclei are counterstained
with DAPI (blue); l, lumen. Scale bars, 50 µm (A-C); 10 µm (D).
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Fig. 7. Localization of AQP-x5 by immunofluorescent staining in Hyla
japonica (A,B), Rana japonica (C,D) and Bufo marinus
(E,F). Fluorescence images (A,C,E) for AQP-x5 and the corresponding Nomarski
differential interference contrast images (B,D,F) are shown. AQP-x5 (green;
arrows); V-ATPase E-subunit (red; arrowheads) are clearly visible. l, lumen.
Scale bars, 10 µm (A-D); 50 µm (E,F).
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Fig. 8. A conventional electron micrograph showing secretory cells (sc) and a
mitochondria-rich cell (mrc) in the small granular gland. The secretory cell
has many secretory granules (sg), whereas the cytoplasm in the
mitochondria-rich cell is filled with mitochondria, and microvilli-like
structures (arrows) develop throughout the region of the plasma membrane.
Scale bar, 1 µm.
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Fig. 9. (A) An immunoelectron micrograph showing the small granular gland
immunolabeled for AQP-x5. Labels are visible in the apical plasma membrane of
the secretory cells (sc) in the small granular gland. (B) An immunoelectron
micrograph showing secretory and mitochondria-rich cells labeled with the
antibody preabsorbed with the antigen. Immunogold particles were seen at
background levels, especially in mitochondria-rich cell (arrowheads). l,
lumen; mrc, mitochondria-rich cell; m, mitochondria; asterisks, secretory
granule. Scale bar, 1 µm.
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© The Company of Biologists Ltd 2006
