Abstract
Epidermal keratinocytes achieve sequential differentiation from basal to granular layers, and undergo a specific programmed cell death, cornification, to form an indispensable barrier of the body. Although elevation of the cytoplasmic calcium ion concentration ([Ca2+]i) is one of the factors predicted to regulate cornification, the dynamics of [Ca2+]i in epidermal keratinocytes is largely unknown. Here using intravital imaging, we captured the dynamics of [Ca2+]i in mouse skin. [Ca2+]i was elevated in basal cells on the second time scale in three spatiotemporally distinct patterns. The transient elevation of [Ca2+]i also occurred at the most apical granular layer at a single cell level, and lasted for approximately 40 min. The transient elevation of [Ca2+]i at the granular layer was followed by cornification, which was completed within 10 min. This study demonstrates the tightly regulated elevation of [Ca2+]i preceding the cornification of epidermal keratinocytes, providing possible clues to the mechanisms of cornification.
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Introduction
The body surface of mammalians is covered with skin, which protects them against infection, dehydration, chemicals, and mechanical stress. This barrier function is mainly provided by the stratified squamous epithelium of the skin, the epidermis. The epithelial cells (epidermal keratinocytes) proliferate at the lowest layer of the epidermis and then commence differentiation and upward migration, which takes 40–56 or 8–10 days in humans and mice, respectively1. During this differentiation, the morphology of epidermal keratinocytes changes markedly. On the basis of its morphological characteristics, the epidermis can be subdivided into four layers: basal, spinous, granular, and cornified layers. The granular layer is further subdivided into three layers designated as SG1, SG2, and SG3 from the apical to the basal side2.
At the border of the granular and cornified layers, epidermal keratinocytes (SG1 cells) undergo a programmed cell death called cornification, which is characterized by a rapid loss of cell volume3. Although apoptosis and cornification share similarities, such as the loss of an intact nucleus and other organelles, the dead cell corpses of epidermal keratinocytes are not removed; instead, they are maintained to fulfill a barrier function4. The regulatory mechanisms of cornification remain elusive, and their clarification is important to furthering our understanding of skin homeostasis.
The concentration of cytoplasmic calcium ions ([Ca2+]i) is one of the factors predicted to regulate cornification for several reasons5,6. First, it is known that the various forms of cell death (necrosis, apoptosis, and autophagic programmed cell death) share molecular effectors and signaling routes, and the elevation of [Ca2+]i is involved in the process of apoptosis, which is assumed to have many similarities to cornification4,7. Second, in cultured keratinocytes, [Ca2+]i elevation following stimulation for differentiation has been identified8. Third, in both the human and murine epidermis, a number of experimental and theoretical analyses have shown the preferential distribution of calcium ions in the granular layer, which are indicated to localize to intracellular compartments9,10,11,12,13,14. Therefore, it has been suspected that the transient elevation of [Ca2+]i occurs during the process of differentiation and/or cornification. However, the spatio-temporal dynamics of [Ca2+]i in the sequential differentiation of epidermal keratinocytes remains largely unknown because of technical limitations.
In this study, using a two-photon microscope that enables morphological and physiological analyses in vivo at subcellular resolution15,16,17, we analyzed the in vivo dynamics of [Ca2+]i in epidermal keratinocytes. We identified the transient elevation of [Ca2+]i in SG1 cells preceding the morphological changes during the process of cornification.
Results
[Ca2+]i is elevated in epidermal keratinocytes in two layers in a steady state
To visualize [Ca2+]i, we used mice systemically expressing a genetically encoded Ca2+ indicator (GCaMP3)18. GCaMP3 is a modified green fluorescent protein (GFP) that increases its fluorescence in proportion to the level of [Ca2+]i19.
In ear skin in a steady state, cells with an increased fluorescence of GCaMP3 (GCaMP3high cells) were identified in a subset of epidermal keratinocytes in two layers: the lowest layer of the epidermis (basal layer) and the upper epidermis (granular layer) (Fig. 1a–c). The elevated fluorescence of GCaMP3 was detected in the cytoplasm in the basal layer (Fig. 1d), whereas it was detected in both the nucleus and the cytoplasm in the granular layer (Fig. 1e).
Physiological state of [Ca2+]i in the epidermis. Representative two-photon images of the ear skin of mice systemically expressing GCaMP3 (GCaMP3 mice). (a) Three-dimensional view, (b) Vertical view showing cells with elevated fluorescence of GCaMP3 (GCaMP3high cells). Arrow and arrowhead: GCaMP3high cells in the basal and granular layers, respectively. Green: GCaMP3; red: autofluorescence; blue: second-harmonic generation from dermal collagen. Dashed line in (b): dermo-epidermal junction. (c) Hematoxylin and eosin staining of the ear skin section. Double-headed arrows: epithelial layers. (d) Horizontal view of the basal layer. Arrows: GCaMP3high basal cells. (e) Maximum intensity view of the granular layer. Arrowhead: a GCaMP3high granular cell. Arrow: nucleus. Scale bars: 50 μm (a–d) and 10 μm (e). [Ca2+]i: concentration of calcium ions in the cytoplasm. Results are representative of at least three independent experiments.
To dissect whether this difference in the localization of elevated GCaMP3 fluorescence between basal and granular cells actually reflects the difference of [Ca2+]i elevation or derives from uneven subcellular distribution of GCaMP3 protein, we immunostained GCaMP3 protein with anti-GFP antibody using sections of fingertip skin of GCaMP3 mice. In the basal cells, the protein of GCaMP3 distributed preferentially in the cytoplasm, whereas it was hardly detected in the nucleus (Supplemental Fig. 1). In contrast, in the granular cells, the protein of GCaMP3 was detected in both the cytoplasm and nucleus (Supplemental Fig. 1). Therefore, the lack of elevated fluorescence of GCaMP3 in the nucleus of basal cells might be due to the low concentration of the GCaMP3 protein.
A Ca2+ spike in the basal layer occurs on the second time scale in three distinct patterns
Next, we evaluated temporal changes in the basal layer of the ear skin. The appearance of GCaMP3high cells had three spatiotemporally different patterns (Fig. 2a–c).
Three patterns of transient [Ca2+]i elevation in the basal layer. (a) Representative time-lapse images of the basal layer of the ear skin of GCaMP3 mice. Upper panel: Ca2+ spike in a single cell unit. Middle panel: clustered Ca2+ spike. Lower panel: radially spreading Ca2+ spike. Arrow: hair shaft. Green: GCaMP3; red: autofluorescence; blue: second-harmonic generation from dermal collagen. (b) Relationship between the duration and the proportion of Ca2+ spikes in a single cell unit (n = 416 events). (c) Relationship between the number of times and the proportion of Ca2+ spikes in a single cell unit (n = 310 cells) in 10 min. ND: not detected. Scale bars: 50 μm. Results are representative of at least three independent experiments.
The most common pattern was a Ca2+ spike in a single cell unit. The fluorescence of GCaMP3 elevated sporadically as single cells (Fig. 2a, upper panel, and Supplemental Movie 1). This occurred at both follicular and intrafollicular epithelia, and lasted for approximately 4 s (median value, Fig. 2b). Although most of the basal cells exhibited a Ca2+ spike only once during the observation period, some of the cells exhibited a Ca2+ spike several times in 10 min (Fig. 2c).
The second pattern was a clustered Ca2+ spike. GCaMP3high cells appeared sporadically as clustered cells less frequently than a Ca2+ spike in a single cell unit (Fig. 2a, middle panel). The duration of this pattern was also on the second time scale (Supplemental Movie 2). A clustered Ca2+ spike occurred around an oval GCaMP3high cell that was larger than basal keratinocytes, although this observation was quite rare (Supplemental Movie 3). The frequency of both a Ca2+ spike in a single cell unit and a clustered Ca2+ spike pattern was much lower in the hind paw skin (Supplemental Movie 4) than in the ear skin, suggesting that the fundamental level of [Ca2+]i in basal keratinocytes might differ significantly depending on the skin site.
The third pattern was a radially spreading Ca2+ spike. The elevation of the fluorescence of GCaMP3 sometimes originated from a few cells and radially propagated in the basal layer of the epidermis (Fig. 2a, lower panel, and Supplemental Movie 5). The mean duration and the radius of this pattern were 89.4 ± 5.5 s and 86.7 ± 6.9 μm (n = 19 events), respectively. The speed of radial propagation was 0.95 ± 0.04 μm/s or approximately 6.1 basal cells/min (n = 19 events). This pattern occurred several times at intervals of 139.8 ± 13.3 s (n = 10 sequential events), and the origin was always located around the hair follicles (Fig. 2a, lower panel). A radially spreading Ca2+ spike was not observed in hind paw skin that lacks hair follicles (Supplemental Movie 4).
The frequency of these three patterns of Ca2+ spikes did not linearly correlate with the strength of the excitation laser (Supplemental Fig. 2), indicating that these were not dependent on artifacts of laser stimulation but were physiological phenomena in a steady state.
[Ca2+]i in the granular layer is elevated transiently for approximately 40 min
Next, we addressed the dynamics of elevation of [Ca2+]i in the granular layer.
Time-lapse imaging showed that the elevation of the fluorescence of GCaMP3 was transient (Fig. 3a,b, Supplemental Movie 6). The mean duration of elevated fluorescence was approximately 40 min in both ear and fingertip skin (Fig. 3c). The frequency of GCaMP3high cells was much higher in the fingertip skin than in the ear skin (Fig. 3d). The estimated times within which the elevation of [Ca2+]i took place in the entire observational area were 23.4 h and 4.7 h in the ear and fingertip skin, respectively. GCaMP3high cells in the granular layer appeared at a single cell level and did not spread to adjacent cells (Fig. 3a). Furthermore, GCaMP3high cells rarely overlapped at the same horizontal position within the observational period (Fig. 3e,f).
Dynamics of [Ca2+]i elevation in the granular layer. (a) Schematic (far left) and representative time-lapse images of the granular layer of the ear skin of GCaMP3 mice. Green: GCaMP3; red: autofluorescence; blue: second-harmonic generation from dermal collagen. (b) Heat map showing the relative intensity of the fluorescence of GCaMP3 in each granular cell. Note that each cell exhibits a transient elevation of fluorescence only once in the observation period. (c) Duration of transient [Ca2+]i elevation in the granular cells in ear skin (n = 10 cells) and fingertip skin (n = 17 cells). (d) Percentage of area with elevated fluorescence of GCaMP3 in an observation field in the ear and fingertip skin. Overall, 13 and 25 time points were analyzed in the ear and fingertip skin, respectively. (e) Representative two-photon image of the fingertip skin of mice systemically expressing GCaMP3 and tandem dimer Tomato (GCaMP3/tdTomato mice). Arrow: intra-epidermal sweat duct. Green: GCaMP3, red: tdTomato. (f) Time-projection image showing the order of transient [Ca2+]i elevation in the fingertip skin. Bright green: newly appearing cells with transient [Ca2+]i elevation; dark green: areas that showed transient [Ca2+]i elevation previously; magenta: area that showed overlap of transient [Ca2+]i elevation. Error bars: standard error of the mean. Scale bars: 50 μm. Results are representative of at least three independent experiments.
Taken together, these results suggest that the order and the duration of [Ca2+]i elevation were tightly regulated in each granular cell that eventually achieved cornification.
[Ca2+]i is elevated in a subset of SG1 cells
Next, we investigated the precise location of GCaMP3high cells in the granular layer. The granular layer is subdivided into three layers, and granular cells in the middle layer (SG2 cells) form a tight junction barrier2,20. Subsequently, granular cells in the most apical layer (SG1 cells) finally achieve cornification, and then become integrated into the cornified layer.
To visualize the SG2 layer, we utilized mice systemically expressing ZO-1 EGFP, and crossbred them with GCaMP3 mice21 (ZO-1 EGFP/GCaMP3 mice). In ZO-1 EGFP mice, zonula occludens-1 (ZO-1), a constituent molecule of tight junctions, is fused with enhanced green fluorescent protein (eGFP). Using these mice, we can visualize the SG2 layer by exciting eGFP. In the ear and hind paw skin of ZO-1 EGFP/GCaMP3 mice, GCaMP3high cells were located above the tight-junction signal (Fig. 4)20, indicating that the transient elevation of [Ca2+]i occurs in SG1 cells.
Location of GCaMP3high cells and tight junctions in the granular layer. (a-c) Representative two-photon images of the hind paw skin of mice systemically expressing both GCaMP3 and ZO-1 EGFP. The intensity of green fluorescence from both GCaMP3 and ZO-1 EGFP is represented in gray scale. (a) Vertical view. (b,c) Horizontal view. Arrows: fluorescence from ZO-1 EGFP that corresponds to tight-junctions. Arrowheads: a granular cell showing transient [Ca2+]i elevation. (d) Schematic of the location of [Ca2+]i-high granular cells and tight junctions. SG1 and SG2: The most apical and middle layers of the granular layer, respectively. Scale bars: 20 μm.
To further confirm this observation, we next used tandem dimer Tomato (tdTomato) mice. Tdtomato is one of the red fluorescent proteins, which was specifically designed for low aggregation22. In this strain, the morphology of epidermal keratinocytes (the nuclei and intracellular granules in the granular layer) was well visualized with the red fluorescence of tdTomato. In addition, the border of the granular and cornified layers was visualized by contrast with fluorescence intensity (Fig. 5a), which may have been be due to the condensation of fluorescent protein arising from the reduction of cell volume during cornification. We crossbred tdTomato mice with GCaMP3 mice (tdTomato/GCaMP3 mice) and observed their ear and hind paw skin. Consistent with the results in ZO-1 EGFP/GCaMP3 mice, GCaMP3high cells were located immediately beneath the cornified layer (Fig. 5a). During the transient elevation of the fluorescence of GCaMP3, these cells sustained the typical morphology of granular cells: intact nuclear structure and intracellular granules (Fig. 5c).
Temporal relationship between transient [Ca2+]i elevation and cornification. (a,b) Representative images of two-photon microscope of the fingertip skin of GCaMP3/tdTomato mice. (a) Vertical view. Note that cornified cells exhibit intensified fluorescence of tdTomato. Arrows: granular cells with transient [Ca2+]i elevation. White line: the surface of the skin. Cyan lines: upper and lower borders of the granular layer. Dashed white line: dermo-epidermal junction. (b) Horizontal view showing the granular layer at different depths. Note that nuclei and cytoplasmic granules are visualized with the fluorescence of tdTomato. (c) Representative plot of the relative fluorescence intensity of GCaMP3 (green line) and tdTomato (red line) in the process of transient [Ca2+]i elevation and cornification. (d) Time-lapse imaging of the most apical granular cell. A white arrow indicates the start of [Ca2+]i elevation, and a yellow arrow indicates the end of [Ca2+]i elevation. Cyan arrow: cytoplasmic granules. White arrowhead: abrupt elevation of the fluorescence of tdTomato in the nucleus. Cyan arrowhead: disappearance of cytoplasmic granules. Yellow arrowhead: cornified cell that becomes indistinguishable from the neighboring cell. Green: GCaMP3, red: tdTomato, blue: second-harmonic generation from dermal collagen. Scale bars: 20 μm. Results are representative of at least three independent experiments.
Taken together, these results demonstrate that a subset of SG1 cells residing immediately beneath the cornified layer showed the transient elevation of [Ca2+]i.
Morphological changes of keratinocytes from the granular layer to the cornified layer begin seconds after the transient elevation of [Ca2+]i
Next, we investigated the association between the transient elevation of [Ca2+]i and the transition from granular to cornified cells using tdTomato/GCaMP3 mice.
Seconds after the end of the decrease in the fluorescence of GCaMP3, the fluorescence intensity of tdTomato began to increase (Fig. 5c). Then, within 3 min of the decrease in the fluorescence of GCaMP3, the nucleus exhibited transformation, followed by the disappearance of intracellular granules (Fig. 5d, Supplemental Movie 7). Subsequently, the nuclear and cytoplasmic signals of tdTomato became homogeneous, and these cells became indistinguishable from adjacent cornified cells (Fig. 5d, Supplemental Movie 7), which occurred within 10 min in both ear and fingertip skin. Morphological changes and the transient elevation of the fluorescence of GCaMP3 were paired in all cells examined (Table 1).
To further characterize the nuclear changes in the transition from granular to cornified cells, we used Fucci mice and crossbred them with GCaMP3 mice (Fucci/GCaMP3 mice). In Fucci mice, the nucleus is labeled with green and red fluorescent protein, and the ratio of these proteins indicates the cell cycle. The nuclear signal disappeared immediately after the decrease in the fluorescence of GCaMP3 (Fig. 6a), indicating that some cell death other than apoptosis had occurred, because apoptotic cells exhibit fragmented nuclei but do not lose the fluorescent label23.
Temporal relationship between the transient [Ca2+]i elevation and changes in the nucleus. (a) Time-lapse imaging of the most apical granular cell in the hind paw of mice systemically expressing Fucci and GCaMP3. Arrow: nuclear signal of red fluorescent protein of Fucci system. Note that the nuclear signal disappeared along with the decrease in the fluorescence of GCaMP3. (b) Time-lapse imaging of the granular and cornified layers of the hind paw skin of GCaMP3 mice injected with Hoechst 33342. Yellow arrowheads: granular cells with elevated fluorescence of GCaMP3. White arrows: intensified fluorescence of Hoechst 33342. Green: GCaMP3; red: mKO2-hCdt1 (a), Hoechst 33342 (b). Scale bars: 20 μm. Results are representative of at least two independent experiments.
We next assessed temporal changes in the DNA of the nucleus by labeling it with Hoechst 3334224,25. The fluorescence of Hoechst 33342 gradually increased over 100 min after the decrease in GCaMP3 fluorescence (Fig. 6b) and then disappeared (Supplemental Fig. 2). These results suggest that the condensation of DNA, possibly because of the reduction in cell volume by cornification, occurred after the decrease of [Ca2+]i, which is followed by the degradation of DNA in the process of cell death (Supplemental Fig. 2).
Taken together, these results indicate that the transition from SG1 cells to cornified cells occurs within a short time after the transient elevation of [Ca2+]i.
[Ca2+]i-high cells are observed in the upper layer of various types of cornifying stratified epithelia
To evaluate whether the transient elevation of [Ca2+]i is a common feature of epithelia that undergo cornification, we carried out the in vivo and ex vivo observations of various stratified squamous epithelia. Stratified squamous epithelia with cornified layers are classified into two types: cornification with enucleation (orthokeratosis) and cornification without enucleation (parakeratosis). Most parts of the skin exhibit orthokeratosis, whereas some parts of the skin and most of the mucous epithelia with cornified layers exhibit parakeratosis.
We examined the tail skin in vivo; at this site, both orthokeratosis and parakeratosis coexist under physiological conditions26. Elevated fluorescence of GCaMP3 was observed in the cytoplasm and the nucleus in a subset of SG1 cells in both orthokeratotic and parakeratotic areas (Fig. 7a). In addition, in the parakeratotic area, residual nuclei in the cornified layer showed intense fluorescence of GCaMP3 (Fig. 7a). Next, we examined the parakeratotic area of the oral mucosa (hard palate) or vagina by ex vivo observation and identified GCaMP3high cells beneath the cornified layer (Fig. 7b,c). These results suggest that the transient elevation of [Ca2+]i in SG1 cells is general in cornifying epithelia, regardless of enucleation.
Physiological state of [Ca2+]i in the parakeratotic epidermis and mucous epithelia. Representative two-photon images of GCaMP3 mice (a,b) or GCaMP3/tdTomato (c), in a vertical view. (a) In vivo observation of the tail skin. (b,c) Ex vivo observation of the mucous epithelia of the (b) vagina and (c) oral cavity. The contrast in the fluorescence of GCaMP3 was corrected using the fluorescence signal of tdTomato, which reflects the concentration of fluorescent proteins in the cytoplasm. Arrowheads: cells with elevated fluorescence of GCaMP3 beneath the cornified layer. Dashed lines: dermo-epidermal junction or lower edge of the mucous epithelia. Green: GCaMP3; red: autofluorescence (a); blue: second-harmonic generation from dermal collagen. Double-headed arrows: epithelial layers. Scale bars: 50 μm. Results are representative of at least three independent experiments.
Discussion
Here, we elucidated the physiological dynamics of [Ca2+]i in epidermal keratinocytes. We identified three patterns of Ca2+ spikes in the basal layer, and the transient elevation of [Ca2+]i in SG1 cells preceding the morphological changes of cornification.
To the best of our knowledge, spontaneous Ca2+ spikes in the basal layer of the epidermis have never been documented. A Ca2+ spike in a single cell unit might be a feature shared among epithelial cells because a similar phenomenon was observed in the intestinal epithelium27. A clustered Ca2+ spike was very occasionally observed to occur frequently in the vicinity of uncharacterized large oval GCaMP3high cells. This suggests that a clustered Ca2+ spike might reflect the stimulation of basal keratinocytes by dermal cells. A radially spreading Ca2+ spike might be related to hair follicles. In addition, this pattern might be transmitted via gap junctions, because Ca2+ propagation through gap junctions has been detected in the basal layer of ex vivo human skin28. Importantly, all patterns of Ca2+ spikes were sporadic and occurred several times in the same cells. Furthermore, it was shown that the level of [Ca2+]i oscillation regulates the activity of stem cells in the intestine of Drosophila29. Therefore, we speculated that these events might be correlated with the proliferation or early differentiation of epidermal keratinocytes rather than cornification.
Our study revealed that the transient elevation of [Ca2+]i occurred at a single cell level in SG1 cells, which has not been identified by previous studies showing a high concentration of calcium ions in the granular layer9,10,11. This result fits with the recent in vivo studies showing the terminal differentiation of keratinocytes in an apparently sporadic manner2,30. Because the transient elevation of [Ca2+]i rarely occurred at the same horizontal position within the observational period, the order of this event is unlikely to be completely stochastic; rather, it is probably regulated by some unknown mechanisms. The frequency of the elevation of [Ca2+]i in SG1 cells might reflect the speed of turnover of the epidermal keratinocytes, which depend on the site of skin31.
The transient elevation of [Ca2+]i in SG1 cells was coupled with and occurred just before the morphological changes associated with cornification. Although the causal relationship between the elevation of [Ca2+]i and cornification was not evaluated in this study, our data strongly suggest that the transient elevation of [Ca2+]i is involved in the mechanisms of cornification. Indeed, previous studies demonstrated rapid increase in the number of transitional cells after elevation of [Ca2+]i by an inhibition of sarco/endoplasmic reticulum Ca2+ ATPase (SERCA)12,32. Furthermore, it is known that Ca2+ is required to activate the transglutaminases that assemble the cornified envelope, a protective barrier structure inside the plasma membrane33. In addition, Ca2+ influx induces the formation of the cornified envelope in cultured keratinocytes34,35. Therefore, it is possible that elevated [Ca2+]i activates transglutaminases in SG1 cells before the transformation to cornified cells.
GCaMP3-protein was distributed exclusively in the cytoplasm in the basal cells, but distributed to both the nucleus and cytoplasm in the granular cells. This observation raises a hypothesis that GCaMP3 protein in the cytosol re-distributed to nucleus due to increased permeability of nuclear envelope in the process of cell death36. In this scenario, the initiation of cell death precedes the transient elevation of [Ca2+]i. Because the elevated fluorescence of GCaMP3 disappears in skin sections for immunohistochemistry, establishment of an in vivo evaluation system to detect GCaMP3 fluorescence and keratinocyte differentiation markers or cell death markers would be necessary to clarify this issue.
Gene mutations related to Ca2+ homeostasis result in skin lesions, including aberrantly promoted cornification in congenital diseases such as keratitis-ichthyosis-deafness (KID) syndrome and Darier’s disease37,38. This implies a possible link between Ca2+ homeostasis and cornification. In KID syndrome, mutated connexin proteins were recently shown to form hyperactive hemi channels, connecting the inside and outside of the cells39,40. Therefore, Ca2+ influx through hyperactive hemi channels in the granular layer might promote cornification in the skin of patients with KID syndrome. Whereas, Darier’s disease is caused by a mutation in ATP2A2 coding type 2 isoform of SERCA (SERCA2)38. Because calcium ions in the granular layer are suggested to localize to intracellular compartments including endoplasmic reticulum (ER), it is possible that the source of calcium ions in the transient elevation of [Ca2+]i in SG1 cells are intracellular compartments13,14. Generally, the high concentration of calcium ions in these compartments is sustained by calcium pumps or channels including SERCA2. Therefore, mutated SERCA2 proteins might affect the concentration of calcium ions in ER and the dynamics of [Ca2+]i in SG1 cells, eventually resulting in aberrant cornification in the granular layer in Darier’s disease.
In conclusion, we identified the transient elevation of [Ca2+]i in SG1 cells preceding cornification. This finding significantly deepens our understanding of the mechanisms of cornification in epidermal keratinocytes and may lead to the development of specific treatment for skin diseases affecting the cornified layer.
Materials and Methods
Mice
R26-CAG-LoxP-GCaMP3 mice18 (RBRC05163; RIKEN BRC, Ibaraki, Japan) and R26-CAG-tdTomato mice (007908; Jackson Laboratory, Bar Harbor, Maine, USA) were crossbred with EIIa-cre mice (Jackson Laboratory) to generate mice systemically expressing fluorescent proteins. These mice were further crossbred with R26-ZO1-EGFP21 or R26p-Fucci241 mice (CDB0256K and CDB0203T; RIKEN CLST[http://www2.clst.riken.jp/arg/reporter_mice.html], Kobe, Japan). Both male and female mice were applied for experiments at their age of 8–24 weeks. All experimental protocols were approved by the Animal Experimentation Committee of Kyoto University and all animal experimental procedures were performed according to the Animal Protection Guidelines of Kyoto University.
Two-photon microscope
In vivo two-photon imaging of the skin was performed as previously described16. In brief, mice were anesthetized with isoflurane and positioned on the heating plate on the stage of a two-photon microscope (IX-81; Olympus, Tokyo, Japan). The earlobes, feet, and tails were fixed with a single drop of immersion oil. We checked the correlations between the intensity of excitation laser and the frequency of Ca2+ spikes in the basal layer (Supplemental Fig. 2), and determined the observation settings that do not evoke artifacts by heat or laser stimulation (Supplemental Table). In certain experiments, Hoechst 33342 (Invitrogen, Carlsbad, CA, USA) was injected into the hind paw at a concentration of 1 mg/mL, 1 day before observation. After confirming that the fluorescence pattern of GCaMP3 at the granular layer did not change within 5 min after skin excision, we performed ex vivo imaging of the mucous epithelia within 5 min after the excision of each organ.
Immunostaining
Freshly excised fingertip skin was immersed with 4% paraformaldehyde, 20% sucrose overnight, respectively. Samples were then embedded in the OCT compound (Sakura, Tokyo, Japan) and was frozen in liquid nitrogen. Sections of 5 μm thickness were stained with anti-GFP antibody (A11122; Molecular Probes, Carlsbad, CA, USA) and anti-rabbit IgG antibody (A21207; Invitrogen, Carlsbad, CA, USA). Fluorescence images were obtained using a fluorescence microscope (BZ-9000; Keyence, Osaka, Japan).
Image analysis
Images were processed using ImageJ version 1.45 s (NIH, Bethesda, USA) and Imaris software version 7.2.1 (Bitplane, Zurich, Switzerland). The elevation of the fluorescence of GCaMP3 was determined in time series images, with a threshold of a 50% increase relative to the mean fluorescence intensity of each cell.
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Acknowledgements
We thank I. Imayoshi (Kyoto University) for the R26-CAG-LoxP-GCaMP3 mice and T. Furuyashiki (Kyoto University) for the EIIa-cre mice. This study was supported by JSPS KAKENHI (JP26–5153). JSPS KAKENHI (JP26–5153) and Agency for Medical Research and Development (16he0902003h0002).
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T.M., T.H. and K.K. designed this study and wrote the manuscript. T.M. performed the experiments. G.E., Y.Y., R.I., F.T. and T.D. provided technical support and intellectual guidance. All authors reviewed the manuscript.
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Supplemental Movie 3: Clustered Ca2+ spike frequently observed around a continuously fluorescent cell in the basal layer
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Murata, T., Honda, T., Egawa, G. et al. Transient elevation of cytoplasmic calcium ion concentration at a single cell level precedes morphological changes of epidermal keratinocytes during cornification. Sci Rep 8, 6610 (2018). https://doi.org/10.1038/s41598-018-24899-7
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DOI: https://doi.org/10.1038/s41598-018-24899-7
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