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First published online May 2, 2008
Journal of Experimental Biology 211, 1690-1695 (2008)
Published by The Company of Biologists 2008
doi: 10.1242/jeb.017186
Cutaneous water loss and sphingolipids covalently bound to corneocytes in the stratum corneum of house sparrows Passer domesticus
1 Department of Evolution, Ecology and Organismal Biology, 318 W. 12th Avenue,
Aronoff Laboratory, Ohio State University, Columbus, OH 43210, USA
2 Applied Biosystems, 500 Old Connecticut Path, Framingham, MA 01710, USA
Author for correspondence (e-mail: address:
munoz-garcia.1{at}osu.edu)
Accepted 25 March 2008
 |
Summary |
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 TOP Summary INTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONReferences |
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-hydroxyceramides attached to the outer surface of
corneocytes. Evidence suggests that covalently bound lipids in the SC might be
crucial for the establishment of a competent permeability barrier. In this
study we assessed the composition of covalently bound lipids of the avian SC
and their relationship to cutaneous water loss (CWL) in two populations of
house sparrows, one living in the deserts of Saudi Arabia and the other in
mesic Ohio. Previously, we showed that CWL of adult desert sparrows was 25%
lower than that of mesic birds. In the present study we characterize
covalently bound lipids of the SC using thin layer chromatography and high
performance liquid chromatography coupled with atmospheric pressure
Photospray® ionization mass spectrometry. Our study is the first to
demonstrate the existence of sphingolipids covalently bound to corneocytes in
the SC of birds. Although -hydroxyceramides occurred in the lipid
envelope surrounding corneocytes, the major constituent of the covalently
bound lipid envelope in house sparrows was -hydroxycerebrosides,
ceramides with a hexose molecule attached. Sparrows from Saudi Arabia had more
covalently bound cerebrosides, fewer covalently bound ceramides and a lower
ceramide to cerebroside ratio than sparrows living in Ohio; these differences
were associated with CWL.
Key words: covalently bound lipid, house sparrows, desert, cutaneous water loss
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INTRODUCTION |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONReferences |
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). Given that
cutaneous water loss (CWL) is 50–70% of total evaporative water loss at
moderate air temperatures (Tieleman and
Williams, 2002), it becomes apparent that the role played by skin
as a barrier to water vapor diffusion is important. In both birds and mammals,
resistance to CWL is conferred by lipid molecules arranged in an extracellular
matrix located in the stratum corneum (SC), the outer layer of the epidermis
(Menon et al., 1986;
Wertz, 2000;
Bouwstra et al., 2003;
Coderch et al., 2003;
Lillywhite, 2006). The SC is
composed of flattened dead cells, called corneocytes, and two compartments of
lipids; one fills the intercellular spaces of the SC and the other consists of
covalently bound lipids to corneocytes, called the lipid envelope. In mammals,
intercellular lipids of the SC consist of nearly equimolar proportions of
ceramides, cholesterol and free fatty acids
(Bouwstra et al., 2003;
Madison, 2003). These lipid
molecules are structured in bilayers called lamellae
(Swartzendruber et al., 1989;
Bouwstra et al., 2003; Hill and
Wertz, 2006). In the SC of birds, these same three classes of extracellular
lipids occur with the addition of cerebrosides, which are ceramide molecules
with an attached hexose (Wertz et al.,
1986; Muñoz-Garcia and
Williams, 2005).
Corneocytes of the SC are encapsulated by several structural proteins,
notably involucrin and loricrin (Downing,
1992; Marekov and Steinert,
1998). In electron micrographs of SC from which all intercellular
lipids have been extracted, one can observe on the exterior surface of
corneocytes a translucent layer of lipids, which were shown to be
-hydroxyceramides covalently bound to the protein envelope
(Wertz and Downing, 1987;
Wertz et al., 1989;
Downing, 1992;
Stewart and Downing, 2001). An
important protein involved in the formation of covalent bonds with lipids is
involucrin, a protein structured as a beta-sheet along the surface of the
corneocyte (Downing, 1992;
Marekov and Steinert, 1998).
Non-polar amino acids face the surface of the corneocyte, whereas polar amino
acids with negative charges, such as glutamate, are positioned on the external
surface of the cell. Lipids covalently bound to corneocytes are thought to be
ester-linked to glutamate residues of involucrin molecules and can be
liberated only after mild alkaline hydrolysis
(Wertz and Downing, 1987;
Downing, 1992;
Madison, 2003). Hydroxyl
groups of glutamate form ester bonds with the terminal hydroxyl group of the
fatty acid moiety of ceramides and the sphingosine head interacts with
lamellae of lipid in the extracellular spaces
(Wertz et al., 1989;
Downing, 1992;
Stewart and Downing, 2001).
Covalently bound lipids are thought to serve as a cohesive force binding
corneocytes together at their end plates and to act as a template that
orchestrates the lamellar organization of the intercellular lipids of the SC.
Therefore, in mammals, these lipids appear to play a fundamental role in the
formation of a barrier to water vapor diffusion
(Wertz et al., 1989;
Madison, 2003;
Farwanah et al., 2007).
The chemical structures of the avian protein and the covalently bound lipid
of the SC have received less attention than their counterparts in mammalian
skin. Recent studies on corneocytes of avian SC hint that they are composed of
proteins similar to those of mammals
(Alibardi and Toni, 2004).
Whether corneocytes in the skin of birds also have covalently bound lipids
attached to them, and if they do, what the nature of these lipids might be,
remains unknown. In this report we test the idea that corneocytes of avian SC
have covalently bound -hydroxyceramides, as found in the SC of mammals.
Further, we explore the idea that birds from two radically different
environments have different lipids attached to their corneocytes, which might
lead to a different organization of lipids in the extracellular spaces. Our
results indicate that corneocytes of house sparrows have
-hydroxyceramides and -hydroxycerebrosides attached to their
corneocytes in the SC. This is the first time that cerebrosides have been
found as lipid components covalently attached to corneocytes of a
vertebrate.
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MATERIALS AND METHODS |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONReferences |
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We measured cutaneous water loss (CWL) using an open flow mask respirometry
system (Tieleman and Williams,
2002). Data for CWL of desert and mesic house sparrows are
reported elsewhere (see
Muñoz-Garcia and Williams,
2005).
Extraction of covalently bound lipids
After measuring CWL, we sacrificed birds, and removed their skin. We then
isolated the stratum corneum (SC) and extracted intercellular lipids following
published procedures (Haugen et al.,
2003; Muñoz-Garcia and
Williams, 2005). The SC was stored in glass test tubes at
–20°C under an atmosphere of nitrogen.
To confirm that all extracellular lipids had been extracted, we soaked the SC for each bird for 2 h in chloroform:methanol 1:2 (v/v). We then examined extracts for lipids using thin layer chromatography (TLC). No lipid bands were detected in our plates, indicating that all the intercellular lipids had been removed.
Next we searched for covalently bound lipids (CBL) on corneocytes by
immersing the SC in 2 ml of 1 mol l–1 NaOH in 90% methanol at
60°C for 2 h (Wertz and Downing,
1987). This mild alkaline hydrolysis breaks the ester bonds of
lipids attached by an ester linkage to proteins
(Wertz and Downing, 1987). We
then adjusted the to pH 6 by adding 3 mol l–1 HCl, and added
2.5 ml of chloroform. The solution was then passed through a sintered glass
filter, and centrifuged at 3000 g for 15 min. After a few
minutes, the solution separated into two layers, an aqueous layer and an
organic layer that contained any lipids. The organic phase was washed twice
with distilled water to remove contaminants. The aqueous phase was mixed with
1 ml of chloroform to extract any lipids that might be in this phase, and
recentrifuged at 3000 g for 10 min. We combined the organic
fractions, and removed any remaining small particles by passing the solution
through a PTFE filter, 0.45 µm pore size (Millex, Millipore Corp., Bedford,
MA, USA). We dried the filtrates with a stream of nitrogen and stored them at
–20°C. Prior to analysis of lipids, the extracts were re-constituted
in 50 µl of chloroform:methanol (2:1, v/v) containing 50 mg
l–1 of the antioxidant butylate hydroxytoluene, BHT.
Identification and quantitation of covalently bound lipids
We tested for CBL in the stratum corneum by using analytical thin layer
chromatography (TLC) on 20 cm x 20 cm glass plates covered with silicic
acid (0.25 mm thick, Adsorbosil-Plus 1, Alltech, Deerfield, IL, USA). Plates
were prepared by developing them with chloroform:methanol (2:1, v/v) to the
top, air drying them, and activating them for 30 min at 110°C. Then, we
divided each plate in 10 mm wide lanes. We prepared standards with known
concentrations of nonhydroxy fatty acid ceramides, galactocerebrosides,
cholesterol and a mixture of free fatty acids, all purchased from Sigma (St
Louis, MO, USA). The concentration of the standards varied from 0.3 to 10
µgµl–1, a range that spanned the concentration of
lipids in our extracts. We loaded 5 µl of both standards and samples on to
plates, both in duplicate, with a Teflon tipped Hamilton syringe. More polar
lipids, such as ceramides and cerebrosides, were separated using a development
of chloroform:methanol:water (40:10:1, v/v/v) to 8 cm from the bottom,
followed by two developments with chloroform:methanol:acetic acid (190:9:1,
v/v/v) to the top, and a final development with hexane:diethyl ether:acetic
acid (70:30:1, v/v/v) to a half. For neutral lipids, such as free fatty acids,
we developed plates with hexane to the top, followed by a development with
toluene to the top, and a final development with hexane:diethyl ether:acetic
acid (70:30:1, v/v/v) to half. After development, we sprayed plates with a
solution of 3% cupric acetate in 8% phosphoric acid, placed them on aluminum
hotplates and slowly raised the temperature to 160°C over a period of 30
min. The procedure charred the lipids, allowing their visualization.
Some of the lipids in our extracts migrated on TLC plates at a rate
consistent with cerebroside standards. To confirm that these lipids were
cerebrosides, we tested these bands for the presence of sugars by spraying
plates with a mixture of 100 g of 2,4-dinitrophenylhydrazine in 100 ml
phosphoric acid/ethanol (1:1, v/v). Then, we heated the plate at 110°C for
10 min. In the presence of sugars, 2,4-dinitrophenylhydrazine yields an orange
color (Wall, 2005).
We also used high performance thin layer chromatography (HPTLC) to search for classes of covalently bound cerebrosides in the SC because this method may provide greater resolution of cerebroside classes. For this procedure we used 10x20 cm plates coated with a 0.20 mm thick layer of silica gel (Si 60, Merck, Darmstadt, Germany). We used the same protocol as for analytical TLC, except that we loaded 3 µl of lipid extract and standards on plates. Plates were developed with chloroform:methanol:water (40:10:1, v/v/v) to the top of the plate and bands of lipid visualized as above.
To quantify the concentrations of the CBL classes, we scanned carbonized
plates with a Hewlett Packard scanner, and measured lipid amounts with the
software TN Image (Nelson,
2003). Validation of our methods indicates that we can routinely
measure lipid amounts within ±2%
(Muñoz-Garcia and Williams,
2005).
|
To isolate classes of lipids on preparative plates without changing their chemical structure, we sprayed plates with 0.2% 2,7-dichlorofluorescein in 95% ethanol and visualized bands under UV light. Comparing bands of standards with unknown bands allowed us to designate unknown bands as ceramides or cerebrosides. We marked their location under UV light, and scraped the silica gel from that area. Cerebrosides were recovered from the silica gel by extraction with chloroform:methanol:water (50:50:1, v/v/v), and filtration through a sintered glass filter. Fluorescein was precipitated from this mixture by washing with 2.5% potassium carbonate. Samples were dried in a stream of nitrogen gas and stored in an atmosphere of N2 at –20°C until analyses with HPLC-APPI-MS.
Confirmation of covalently bound cerebrosides using HPLC coupled to atmospheric pressure photo ionization mass spectrometry (APPI-MS)
Because cerebrosides covalently bonded to corneocytes have not previously
been found to be in SC of any vertebrate, we wanted to confirm our
identification of these lipids. Extracts of putative cerebrosides from
preparative TLC were re-dissolved in chloroform:methanol 2:1. We injected 10
µl of this sample onto a HPLC column (Phenomenex Luna C18, spherical 5
µm particle size, 150x2.0 mm i.d., 100 Å pore size, Phenomenex,
Torrance, CA, USA), thermostatically controlled at 48°C, and eluted lipids
using a reverse phase solvent system
(Muñoz-Garcia et al.,
2006). We used a gradient solvent system with methanol:water 95:5
(v/v) as the initial solvent, changed in steps to 100% ethyl acetate, with
flow rate programmed from 180 µl min–1 to 350 µl
min–1 over 30 min.
After passing through our HPLC system, sphingolipids were routed into an Applied Biosystems Q TRAP® hybrid triple quadrupole linear ion trap SCIEX mass spectrometer equipped with a PhotoSpray® ion source (Applied Biosystems, Ontario, Canada) operated in positive ion mode. Toluene, a dopant for our system, was delivered at a flow rate of 20 µl min–1.
Parameters used on the Q TRAP were: collision gas set to High, curtain gas to 27, Ion Transfer voltage set at 2000 V, nebulizer temperature of 460°C, declustering potential set at 40 V and interface heater on.
Using Enhanced MS with signals collected by dynamic fill time, we surveyed lipid molecules between 450 and 1450 amu (±0.4 amu) at a scan rate of 4000 amu s–1. We confirmed the presence of cerebroside molecules by MS/MS by searching for a hexose fragment.
|
Statistics
All statistical tests were performed with SPSS 14.0
(SPSS, 2007) with the null
hypothesis being rejected when P<0.05. Values are reported as
means ± s.d. We tested for significant differences between means using
two-tailed t-test for independent samples.
|
RESULTS |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONReferences |
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To explore differences that might occur in covalently bound lipids between sparrows that inhabit markedly different environments, we compared bound lipids in the SC of sparrows from Saudi Arabia with those in the SC of sparrows from Ohio. We found that sparrows from Saudi Arabia had significantly less ceramides and more cerebrosides covalently bound to their corneocytes than did sparrows from Ohio (t=2.48, P<0.03; t=2.10, P<0.05, respectively) (Table 1). The ceramide:cerebroside ratio was 0.21 in desert sparrows and 0.41 in Ohio birds, a difference that was significant (t=5.95, P<0.001).
|
Identification of covalently bound cerebroside molecules by photospray ionization mass spectrometry
Using HPLC-APPI-MS we confirmed the presence of cerebroside molecules
covalently bound to corneocytes in SC of sparrows from Ohio. A representative
spectrum of one of the cerebrosides in our extract is shown in
Fig. 2A. The molecular ion
[M+H+–2H2O] had a mass of 1016.9, which is
consistent with a cerebroside having a hydroxyl group at the omega position
(Fig. 2B). Hydroxyl ions in
sphingolipids are typically lost as water in the photospray ionization
process. The ion 836.9 is consistent with [M+H+–Hexose] and
indicated that the molecular ion contained a sugar moiety. The fragment at
604.6 further supports the view that the molecule had a terminal hydroxyl
group. The fragment at 264.3 indicates the presence of sphingosine
(Muñoz-Garcia et al.,
2006).
|
|
)]. Sparrows from Ohio had a lower total content of covalently
bound lipids, a higher concentration of covalently bound ceramides, a lower
content of covalently bound cerebrosides than desert sparrows, and a higher
ratio of ceramides to cerebrosides than did desert sparrows. |
DISCUSSION |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONReferences |
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; Munoz-Garcia et al.,
2008), a finding that is consistent for over 20 species of birds
(J.R., A.M.-G., J.C.B. and J.B.W., unpublished data). Thus, cerebrosides seem
to constitute a major lipid class in the avian SC, in both the intercellular
compartment and among lipids covalently bound to corneocytes. Because other
lipid classes found in the SC are the same for birds and mammals, we suspect
that the presence of cerebrosides in the SC is associated with differences in
CWL rates between these taxa. However, the specific role of cerebrosides on
the formation of the avian permeability barrier is not well understood.
Previously we showed that rates of CWL for adult sparrows from deserts in
Saudi Arabia were 25% lower than for their mesic counterparts
(Munoz-Garcia and Williams,
2005). When we compared the composition of the lipid envelope of
the SC of desert and mesic house sparrows, we found that desert sparrows had a
lower concentration of ceramides and a higher concentration of cerebrosides
covalently bound to the corneocytes. Hence lower CWL was associated with
increase in cerebrosides covalently bound to the corneocytes. This result is
in contradistinction to what we expected because glycosylceramides have an
array of hydroxyl groups attached that we thought should interact with water
and therefore increase water permeation.
This finding has prompted us to consider how covalently bound lipids might
be organized on the surface of the corneocytes. We identified sphingolipids of
the lipid envelope of house sparrows as -hydroxyceramides and
-hydroxycerebrosides. Thus, covalently bound sphingolipids of house
sparrows had a hydroxyl group at the omega position of the fatty acid residue,
the same molecular structure as found in mammals
(Wertz and Downing, 1987;
Farwanah et al., 2007). If
hydroxyl groups of the acyl chains of the sphingolipids are covalently
attached to the proteins of the protein envelope
(Stewart and Downing, 2001),
the hexose moiety of the cerebrosides and the sphingosine heads of the
ceramides will face the outer surface of the corneocyte. Why an increase in
cerebrosides covalently bound to corneocytes reduced water vapor diffusion
remains an enigma. We envision two models to stimulate thinking about the
organization of these lipids in the SC of birds. Both models assume that
ceramides align along the outer surface of the intercellular lamellae
(Bouwstra et al., 2003;
Muñoz-Garcia et al.,
2008) and that adjacent corneocytes are bound together by
interactions of covalently bound ceramides.
The `water shell' model suggests that hexose moieties from cerebrosides will form hydrogen bonds with molecules of water forming a water shell around each corneocyte (Fig. 4A). In this model, strong interactions between water molecules and hydroxyl groups of sugar residues reduce water vapor diffusion through the skin. Desert birds had a high concentration of cerebrosides in the lipid envelope, which binds with higher amounts of water, resulting in lower rates of CWL. If this model is correct, we predict that the level of hydration of SC from desert sparrows, from which all intercellular lipids have been removed, would be higher than that of SC from sparrows from Ohio treated in the same manner.
The `hexose link' model, envisions that the hexose moiety of covalently linked cerebrosides forms molecular interactions with sphingosine heads of the intercellular ceramides. In this model, covalently bound cerebrosides of desert sparrows form tighter chemical linkages with the intercellular lipids making water permeation slower. Desert sparrows had more cerebrosides in the layer of covalently bound lipids, implying that a higher number of sugar molecules will interact with intercellular lipid layers. These molecular interactions will promote the formation of a more ordered structure leading to lower rates of CWL.
The picture that has emerged from studies on mammals and now birds is that
lipids of the SC are synthesized in the Golgi apparatus of the basal cells of
the epidermis (Landmann, 1980).
As these cells progress towards the exterior of the epidermis, the Golgi
apparatus transforms into multigranular bodies
(Landmann, 1980): some lipids
in these organelles, mainly glycolipids and phospholipids, are stacked in
lamellae, whereas others are thought to be bound to the membrane. When
multigranular bodies fuse with the cell membrane of the corneocytes, lipids
are extruded to the exterior. Some form intercellular lamellae while others
covalently bind to proteins of the outer surface of the corneocytes, creating
a monolayer of lipids that coats the cell
(Wertz, 2000). In mammals, the
sugar moiety of covalently bound cerebrosides is cleaved enzymatically to
produce ceramides, the major component of the mammalian lipid envelope
(Wertz and Downing, 1987).
Apparently, this enzymatic transformation occurs only partially in avian SC
because we have found ceramides and cerebrosides covalently bound to
corneocytes. With their protruding sugar molecules, cerebrosides bound to
corneocytes would have a profound effect on the formation of incipient lipid
lamellae of the intercellular spaces in the SC. Hence covalently bound lipids
affect the organization of the intercellular lipids of the SC, which in turn
influences rates of CWL.
LIST OF ABBREVIATIONS
|
Acknowledgments |
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Footnotes |
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