(Received for publication, April 18, 1997, and in revised form, June 5, 1997)
From the Departments of Medicine (Dermatology) and
¶ Cell Biology and Physiology, Washington University School of
Medicine, St. Louis, Missouri 63110
In all forms of cutaneous wounds, collagenase-1 (matrix metalloproteinase-1 (MMP-1)) is invariably expressed by basal keratinocytes migrating over the dermal matrix. We report that native type I collagen mediates induction of MMP-1 by primary human keratinocytes. Collagen-mediated induction of MMP-1 was rapid, being detected 2 h after plating, and was transcriptionally regulated. As demonstrated by in situ hybridization, only migrating keratinocytes expressed MMP-1, suggesting that contact with collagen is not sufficient to induce MMP-1 expression in keratinocytes; the cells must also be migrating. Upon denaturation, type I collagen lost its ability to induce MMP-1 expression but still supported cell adhesion. Other dermal or wound matrix proteins, such as type III collagen, fibrin, and fibronectin, and a mixture of basement membrane proteins did not induce MMP-1 production. In the presence of collagen, laminin-1 inhibited induction of MMP-1 but laminin-5 did not. Taken together, these observations suggest that as basal keratinocytes migrate from the basal lamina onto the dermal matrix contact with native type I collagen induces MMP-1 expression. In addition, our findings suggest that re-establishment of the basement membrane and, in particular, contact with laminin-1 provides a potent signal to down-regulate MMP-1 production as the epithelium is repaired.
Normal cutaneous wound healing, as well as healing in essentially all tissues, involves an orderly progression of events to re-establish the integrity of the injured tissue. The initial injury starts a programmed series of interdependent yet functionally separate responses, such as re-epithelialization and epithelial proliferation, inflammation, angiogenesis, fibroplasia, matrix accumulation, and eventually resolution. During each stage in this process, proteinases are needed to remove or remodel extracellular matrix components in both the epithelial and interstitial compartments to accommodate cell migration and tissue repair (1).
In a thorough examination of normally healing wounds and of a variety of chronic ulcers, we found that collagenase-1, a member of the matrix metalloproteinase (MMP)1 family with the ability to cleave fibrillar collagens type I, II, and III at a specific locus in their triple helical domain, is invariably expressed by basal keratinocytes at the edge of repairing tissue (2-4). In all, we have examined >100 different human skin specimens, representing a variety of chronic ulcers, blisters, and normally healing wounds, and in each sample with injury that breached the basement membrane, collagenase-1 was prominently and invariantly expressed by basal keratinocytes migrating over the dermal wound bed. The invariable expression of collagenase-1 in all forms of wounds and the confinement of its expression to periods of active re-epithelialization suggest that this enzyme plays a critical role in keratinocyte function during healing. Indeed, we recently demonstrated that keratinocyte migration on a native collagen matrix requires the catalytic activity of collagenase-1 (5). Thus, identifying the factors and events in a wound environment which control collagenase-1 expression will aid our understanding of fundamental processes of tissue repair.
The precise, spatially confined expression of collagenase-1 by migrating keratinocytes in vivo suggests that altered cell:matrix interactions, which are established as cells migrate off the basement membrane, induce enzyme expression. Indeed, collagenase-1 is only expressed by keratinocytes that are not in contact with an intact basement membrane (3, 4, 6, 7). Furthermore, expression of collagenase-1 is shut off once re-epithelialization is complete and the basement membrane is restored (3, 6). These in vivo findings suggest that altered cell:matrix interactions, which form as cells move from the basement membrane onto the dermal and provisional matrices and back onto the basement membrane at the completion of re-epithelialization, regulate the site-specific expression of collagenase-1 in keratinocytes.
In this report, we show that native fibrillar type I collagen is a principal, if not the main, stimulus initiating collagenase-1 production. Many other molecules that migrating keratinocytes could encounter in a wound setting, such as fibrin, fibronectin, or type III collagen, did not affect collagenase-1 production. In addition, we show that laminin-1 effectively inhibits collagen-mediated collagenase-1 expression, suggesting that renewed contact with this basement membrane component provides a signal to cease collagenase-1 expression and halt keratinocyte migration. Our findings support the idea that distinct cell:matrix interactions regulate keratinocyte behavior at different stages of repair.
Primary keratinocytes were isolated from full thickness skin obtained from reductive mammoplasty and lateral abdominoplasty and grown in high Ca2+ (1.8 mM) medium as described previously (8). Cell suspensions were plated on 3.8-cm2 tissue culture dishes precoated with a 100 µg/ml solution of bovine type I monomeric collagen (Vitrogen; Collagen Corp., Palo Alto, CA). Primary keratinocytes were also plated onto dishes precoated with 20 µg of fibrin (Sigma) or 20 µg of fibronectin (Sigma) or presaturated with a 100 µg/ml solution of laminin-1 (Upstate Biotechnology, Inc, Lake Placid, NY), laminin-5 (supplied by Dr. Robert E. Burgeson, Harvard University), Matrigel® (Becton Dickinson, Bedford, MA), type III collagen (R&D Systems), type IV collagen, vitronectin, rat or mouse type I collagen, or gelatin. Rat tail collagen was prepared by differential salt precipitation, and gelatin was generated by heating native type I collagen (bovine, rat, or mouse) for 10 min at 45 or 80 °C or by cleavage for 1 h at 37 °C with 14.5 µg/ml Clostridium collagenase (Worthington) that had been further purified by Sephacryl S-200 gel filtration (supplied by Dr. Edmond C. Crouch, Washington University, St. Louis, MO). The bacterial enzyme was inactivated by addition of serum. In experiments with two matrices, various amounts of laminin-1 or laminin-5 were combined with 100 µg/ml type I collagen, and dishes were coated with the resultant mixtures. Collagenase-1 accumulation in the medium was assessed 48 h later by competitive enzyme-linked immunosorbant assay (ELISA) and normalized to total cell protein (9).
Keratinocyte cell lines were grown under recommended conditions. The
HaCaT human keratinocyte cell line, provided by Dr. Norbert Fusenig,
German Cancer Research Center, was grown in DMEM containing 10%
heat-inactivated fetal calf serum, 1% Hepes, and antibiotics. KB,
SCC-4, and SSC-25 cell lines were obtained from the American Type
Culture Collection (ATCC, Rockville, MD; CRL-17, CRL-1624, and
CRL-1628, respectively). KB cells were grown in DMEM containing 10%
fetal calf serum, 2 mM L-glutamine, 100 units/ml penicillin, and 100 µg/ml streptomycin. The SSC cell lines
were grown in a 1:1 DMEM:Ham's F-12 medium supplemented with 10%
fetal calf serum, 100 units/ml penicillin, and 100 µg/ml
streptomycin. The JS.1 and JS.6 cell lines were provided by Dr. John C. Ansel (Oregon Health Sciences University) and grown in 3:1 keratinocyte
growth medium (Clonetics, San Diego, CA):DMEM medium supplemented with 10% fetal calf serum, 2.5 mM Hepes, pH 7.4, 100 units/ml
penicillin, and 100 µg/ml streptomycin. To determine if collagenase-1
was inducible in these cells lines, they were plated on plastic or type
I collagen and treated with 30 ng/ml epidermal growth factor (EGF;
Sigma) or 5 × 109 M
12-O-tetradecanoylphorbol 13-acetate (PMA) for 48 h.
Collagenase-1 mRNA was detected in formalin-fixed tissue samples and cultured cells by hybridization with 35S-labeled antisense RNA as described previously (10, 11). Keratinocytes were grown on collagen- or gelatin-coated Lab-Tek chamber slides (Nunc, Naperville, IL) for 48 h and were hybridized with 2.5 × 104 cpm/µl 35S-labeled antisense or sense RNA overnight at 57 °C. After hybridization, slides were washed under stringent conditions, including RNase A treatment, and were processed for autoradiography. After development of the photographic emulsion, slides were stained with hematoxylin-eosin. The specificity of the antisense RNA probe for collagenase-1 and the complete lack of reactivity with the sense probe has been demonstrated in previous studies (2, 3).
Protein SynthesisTotal protein synthesis was determined in cultured keratinocytes as described elsewhere (9). Cells were cultured under various conditions for 24 h and were then incubated for 1 h in leucine-free medium to deplete the intracellular pool of leucine, followed by a 3-h pulse in leucine-free medium containing 1 µCi/ml L-[3H]leucine (42 Ci/mmol). The medium and cell layer were collected, and macromolecules were precipitated with trichloroacetic acid and processed for scintillation spectrophotometry.
RNA AnalysisCollagenase-1 mRNA was detected by a
reverse transcription-polymerase chain reaction (RT-PCR) assay modified
from an established quantitative procedure (12). Total RNA was isolated
by phenol-chloroform extraction. To remove any contaminating DNA, RNA
was treated with RQ1 RNase-free DNase and RNasin (both from Promega,
Madison, WI) as described previously (12). DNase-treated RNA (10 ng)
was reverse transcribed with random hexamers using kit reagents and under the manufacturer's recommended conditions (GeneAmp RNA PCR kit,
Perkin Elmer Corp.). For each sample, a parallel reaction was run with
no reverse transcriptase. The 3-antisense primer was complementary to
bases 1496-1518 in the 3
-untranslated region (5
-GGACTCACACCATGTGTTTTCC-3
), and the 5
sense primer was defined by
bases 1114-1135 of the hemopexin-like domain
(5
-GGGCTGTTCAGGGACAGAATGT-3
) of human collagenase-1 (13). These
primers are to adjacent exons, and thus, the 405-base pair DNA produced
from collagenase-1 mRNA would be easily distinguished from products
amplified from contaminating DNA or preprocessed mRNA. In addition,
the resultant cDNA contains a single BamHI restriction
site, which, along with microsequencing, was used to verify product
identity. PCR was done for 25 cycles, and the resultant products were
detected by Southern hybridization using a human collagenase-1 cDNA
labeled by
-[32P]dCTP random priming.
Primary keratinocytes were plated on
type I collagen- or gelatin-coated tissue culture dishes (28.3 cm2) and were transfected and assayed for reporter activity
as described previously (9). Expression constructs contained the
chloramphenicol acetyltransferase (CAT) reporter gene with no promoter,
pSKCATS, or with a 2-kilobase pair genomic fragment of the human
collagenase-1 promoter, pCLCAT (provided by Dr. Steven Frisch, Burnham
Institute, La Jolla, CA). To assess transfection efficiency, cells were
co-transfected with a plasmid containing the luciferase gene driven by
a thymidine kinase promoter (provided by Dr. Douglas Dean, Washington
University, St. Louis, MO). Plasmids were purified by repeated CsCl
density centrifugation. Cells were transfected with 2 µg of CAT
plasmid DNA, 0.1 µg of the luciferase plasmid, and 10 µl of
LipofectAMINE (Life Technologies, Inc.). After 16 h, the medium
was replaced, and the cells were incubated for an additional 24 h
and harvested. To determine transfection frequency, parallel cultures
were transfected with a pCMV-
-galactosidase construct. Enzyme and
-galactosidase immunostaining assays were done as described
elsewhere (14).
The
spatial confinement of collagenase-1 expression to basal keratinocytes
at the wound edge is illustrated in pyogenic granulomas (Fig.
1), which are highly vascular lesions
containing a loose connective tissue stroma and, frequently, many small
ulcerations of the epidermis. As demonstrated by in situ
hybridization, collagenase-1 mRNA is prominently expressed by
keratinocytes at the migrating epithelial front (Fig. 1, upper
panels). Signal for collagenase-1 mRNA was confined to the
basal layer of the epidermis, diminished progressively away from the
wound edge, and was absent in intact epidermis. As we reported (3),
collagenase-1 is expressed only by basal keratinocytes not in contact
with an intact basement membrane. Expression of collagenase-1 only by
keratinocytes that have moved off of the basement membrane suggests
that alter cell-matrix interactions regulate production of this MMP
during wound healing.
Type I Collagen Promotes Keratinocyte Attachment and Induces Collagenase-1 Production
To identify which matrix components can regulate collagenase-1 expression, we isolated keratinocytes from normal adult human skin. Because primary keratinocytes do not adhere to tissue culture plastic (8), we precoated culture plates with native type I collagen or denatured collagen (gelatin). As assessed by in situ hybridization, collagenase-1 was induced in keratinocytes plated on native type I collagen (Fig. 1, Col) but not in cells plated on gelatin (Fig. 1, Gel).
Similar to wounded epidermis, cultured keratinocytes grown under high calcium (1.8 mM) conditions form subpopulations of migrating, proliferating, and differentiated cells (8). When viewed from above, differentiating keratinocytes are seen as blurred foci (asterisks, Fig. 1, bottom panels) and are surrounded by a monolayer apron of hyperproliferative cells. Bordering the hyperproliferative cells, and often detached from them, are migrating keratinocytes (Fig. 1, bottom panels). Reflecting the phenotype of basal cells involved in re-epithelialization in vivo, collagenase-1 mRNA was prominently expressed only in keratinocytes migrating from the colonies of proliferating and differentiated cells (Fig. 1, Col). As demonstrated in other studies, collagenase-1-positive keratinocytes are migrating and express keratin-14, a basal cell marker (5, 15). Thus, our primary human keratinocyte model duplicates the confinement of collagenase-1 expression by migrating basal keratinocytes seen in vivo. Primary keratinocytes grown in high calcium medium and plated on denatured type I collagen (gelatin) formed these same subpopulations but, as stated, did not express collagenase-1 (Fig. 1, Gel).
To assess if other interstitial proteins or if components of the provisional matrix or basement membrane induce or stimulate collagenase-1 expression, we plated primary keratinocytes on various purified connective tissue proteins and assessed the ability of the cells to attach, spread, and produce collagenase-1 (Table I). Attachment was scored as zero if less than 5% of the keratinocytes adhered to a substratum after the dishes were rinsed and refed 18 h after plating. Spreading was scored as zero if less than 5% of attached cells formed a cytoplasmic apron typical of primary keratinocytes. In all cases, either most keratinocytes (>80%) attached to or spread on a matrix protein or, as for fibronectin and fibrin (Table I), they did not.
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Primary keratinocytes did not attach to uncoated tissue culture plastic or to dishes coated with fibrin or fibronectin, components of the provisional wound matrix (Table I). In contrast, keratinocytes adhered to and spread on the basement membrane proteins, laminin-1 and laminin-5, and on Engelbreth-Holm-Swarm tumor matrix (Matrigel®), which contains laminin-1, type IV collagen, entactin/nidogen, and heparin sulfate proteoglycan, and on type III collagen, a dermal matrix component. None of these matrices, however, induced or stimulated collagenase-1 production as assessed by ELISA (Table I).
Consistent with the in situ hybridization data (Fig. 1),
gelatin supported cell adhesion and spreading but did not induce collagenase-1 production. In contrast, native type I collagen supported
keratinocyte attachment and spreading and mediated induction of
collagenase-1 expression (Table I) in a dose-dependent
manner (Fig. 2A). The number
of cells attached was equivalent at all concentrations of type I
collagen (data not shown), indicating that this dose response was not
an artifact of cell adhesion. The apparent inhibitory effect with high
coating concentrations of collagen (500 and 1000 µg/ml) may be due to
sequestering of some enzyme in the matrix or to negative cooperativity.
This decrease in collagenase-1 was not a consequence of the collagen
contributing to the quantification of total cell protein used to
normalize the ELISA data. Stimulation of collagenase-1 expression in
keratinocytes on native type I collagen was specific relative to total
protein synthesis, which did not differ among cells plated on collagen, gelatin, or Matrigel (data not shown).
Purified type IV collagen and vitronectin also induced collagenase-1 production (Table I) equal to that induced by native type I collagen. As we discussed, we propose that the effect with type IV collagen represents an in vitro artifact. In contrast, vitronectin, similar to type I collagen, may provide a wound-specific factor that maintains or stimulates collagenase-1 expression during re-epithelialization (see "Discussion").
We performed various controls to assure that collagen-mediated induction of collagenase-1 expression was due to contact with the matrix protein and not to a contaminating factor. The same induction of collagenase-1 was detected in keratinocytes plated on type I collagen isolated from rat, mouse, and bovine tissue (Table I). Because these proteins were isolated by different methods, collagenase-1 induction was likely mediated by a specific interaction with collagen. In addition, keratinocytes were plated on gelatin generated by heat denaturation of native type I collagen at 45 °C, a temperature which would be permissive to maintaining the activity of a contaminating inductive factor, or at 80 °C, which would likely inactivate most protein factors. Keratinocytes were also grown on type I collagen that had been digested with highly purified bacterial collagenase, which specifically cleaves Gly-X-Y domains and does not degrade noncollagenous proteins. Collagenase-1 production was induced only in cells cultured on intact, native type I collagen, and only background levels were detected in the cultures grown on the denatured or digested collagen substrata (Fig. 2B). These results indicate that contact with native type I collagen, and not a contaminating factor, induces collagenase-1 expression by keratinocytes.
Contact with Type I Collagen Rapidly Initiates Collagenase-1 ExpressionBecause only a defined subpopulation of keratinocytes
expressed collagenase-1 in response to collagen (Fig. 1), we used
RT-PCR to assess the temporal expression of collagenase-1 mRNA upon
contact with native type I collagen. Signal strength for collagenase-1 RT-PCR cDNA product increased exponentially between 19 and 27 cycles using 10 ng of RNA and increased linearly between 1 and 25 ng of
RNA at 25 cycles (data not shown). Only collagenase-1-specific products
were seen by Southern hybridization or by ethidium bromide staining,
and sequencing and restriction enzyme analysis confirmed the identity
of the cDNA product (data not shown). No collagenase-1 mRNA was
detected in keratinocyte RNA isolated from intact skin (Fig.
3, 0 h). In contrast, low
levels of collagenase-1 mRNA were detected 2 h after plating
keratinocytes on native type I collagen at a high density, and
expression increased markedly and progressively over the next 10 h. Collagenase-1 mRNA dropped to low levels between 24 to 48 h
post-plating (Fig. 3) coincident with the keratinocytes reaching
confluency.
Collagen Induces Collagenase-1 Promoter Activity in Transiently Transfected Keratinocytes
To determine if contact with native
type I collagen induces collagenase-1 gene transcription, primary
keratinocytes plated on collagen or gelatin were transiently
transfected with a CAT expression construct containing 2.2 kilobase
pair of the human collagenase-1 promoter. As we demonstrated in other
studies (16), changes in the activity of this promoter construct
parallel changes in endogenous transcriptional activity of the
collagenase-1 gene. In addition, we demonstrated that both downstream
(72 to
66) and upstream (
2010 to
1954) elements are required
for full and appropriately regulated activity of the collagenase-1
promoter (16). Consistent with secreted enzyme and steady-state
mRNA levels, relative CAT activity was about 5-fold greater in
cells plated on native collagen than in keratinocytes on gelatin (Fig. 4). No CAT activity was detected in cells
transfected with a promoterless construct (data not shown), indicating
that the collagen-responsive elements lie within the collagenase-1
promoter. Luciferase activity, which was expressed from a
co-transfected plasmid under control of a thymidine kinase promoter,
did not differ significantly among samples (Fig. 4). Transfection with
a pCMV-
-galactosidase construct revealed that greater than 80% of
the primary keratinocytes were transfected (data not shown). Because
CAT activity conferred from this region of the collagenase-1 promoter
reflects endogenous production, these results indicate that
collagen-stimulated expression of collagenase-1 is controlled at the
level of transcription.
Collagen Does Not Induce Collagenase-1 in Keratinocyte Cell Lines
Six human keratinocyte cell lines derived from squamous cell carcinomas were screened for their ability to express collagenase-1 production in response to native type I collagen. EGF and PMA were used as positive controls because these agents potently stimulate collagenase-1 production in keratinocytes (15). All keratinocyte cell lines had low to undetectable basal levels of collagenase-1 production, and only a subset of lines increased enzyme expression in response to PMA and/or EGF. None of the cell lines tested responded to collagen (Table II). Furthermore, stimulation of collagenase-1 by either PMA or EGF was not modulated by either substrate. These results suggest that transformed keratinocytes respond differently to signals from the extracellular matrix than do primary cells, suggesting that properly regulated wound healing responses may be lost in oncogenically transformed cells.
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In vivo observations by Inoue et al. (6) and our group (3) demonstrate that collagenase-1 expression in wounded skin is down-regulated upon the completion of re-epithelialization. At this stage, cell:cell contacts and keratinocyte interactions with the basement membrane are restored, and we assessed which or if both of these events regulate the turn-off of collagenase-1. As shown by in situ hybridization of cultured cells (Fig. 1), collagenase-1 is expressed only by keratinocytes that are at the edge of monolayer foci or separate from other cells. Keratinocytes with obvious, well formed cell:cell contacts did not express collagenase-1. Thus, because keratinocytes have the capacity to deposit their own basement membrane matrix, either cell:cell interactions or contact with basement membrane proteins may down-regulate collagenase-1 expression in these stationary keratinocytes.
To assess the role of cell:cell contacts, we plated primary
keratinocytes on collagen-coated dishes or glass slides at different densities and assessed collagenase-1 expression by in situ
hybridization at 1 day post-plating and enzyme accumulation in the
medium by ELISA at 72 h post-plating. Cells plated at 3 × 106 cells per dish were nearly confluent when plated,
whereas the other groups were at variable stages of confluency
proportional to their initial plating density. At 24 h
post-plating, subconfluent cultures showed strong mRNA expression,
whereas only occasional cells in confluent cultures had a weak signal
for collagenase-1 mRNA (Fig. 5,
B and C). Similarly, collagenase-1 mRNA, as
detected by RT-PCR, was expressed briefly and transiently in
keratinocytes plated at confluent density (Fig. 4). At 72 h, when
the medium was collected for ELISA of collagenase-1, cells plated at 2 or 3 × 106 cells/dish were confluent; those plated at
1 × 106 or 1.5 × 106 cells/dish
still had areas of unoccupied surface (data not shown). Collagenase-1
levels were inversely proportional to the initial plating density (Fig.
5A). Thus, barring cells from migrating (by plating at a
high density), and possibly the formation of cell:cell contacts, blocks
collagen-mediated induction of collagenase-1.
In wounded or intact skin, keratinocytes on basement membrane do not
express collagenase-1 (17). Similarly, primary keratinocytes on a
complex mix of basement proteins (Matrigel®) do not express this MMP
(Table I). Because collagenase-1 expression is induced by type IV
collagen but not by laminin-1 (Table I), contact with laminin-1 within
the newly formed basement membrane may participate in down-regulating
collagenase-1 production. To assess if laminin-1 inhibits
collagen-mediated stimulation of keratinocytes, we plated cells on
dishes coated with 100 µg/ml type I collagen, the lowest concentration that mediated maximal stimulation of collagenase-1 production (Fig. 2A), mixed with various concentrations of
purified laminin-1. Collagen-mediated induction collagenase-1 was
inhibited about 50% with relatively low concentrations (between 0.01 and 0.1 µg/ml) of laminin-1, and enzyme levels were reduced to near basal amounts with 100 µg/ml laminin-1 (Fig.
6A). Migrating keratinocytes produce and deposit laminin-5 (18), but this component of the epidermal
basement membrane did not inhibit or significantly augment collagen-mediated induction of collagenase-1 (Fig. 6B).
These data support the idea that reformation of the basement membrane and contact with specific components, particularly laminin-1, provides
a signal to repress collagen-mediated collagenase-1 expression. Taken
together, our data suggest that both the restoration of cell:cell
contacts and interactions with the basement membrane contribute to the
regulation of collagenase-1 during wound repair.
In this report, we demonstrate that contact with native type I collagen induces collagenase-1 expression in migrating keratinocytes. These findings suggest that altered cell:matrix interactions regulate the invariable and prominent expression of collagenase-1 by basal keratinocytes seen during active stages of re-epithelialization in all human wounds with a breached basement membrane. In addition, we show that matrix-mediated regulation of collagenase-1 is dependent on the native, triple helical conformation of type I collagen. Although collagen that had been denatured, solubilized, or enzymatically degraded supported cell attachment, these non-triple helical substrates did not induce or stimulate collagenase-1 expression in keratinocytes. In addition, type III collagen, which is structurally similar to type I collagen, did not induce collagenase-1 expression (Table I). Together these findings suggest that cell contact with type I collagen, the most abundant protein in the dermis, comprising greater than 70% of its dry weight (19), provides a critical and specific determinant regulating collagenase-1 production by keratinocytes. Furthermore, our findings suggest that re-establishment of the basement membrane and cell:cell contacts at the completion of wound closure mediates down-regulation of collagenase-1 expression. Thus, contact with specific components of different matrix compartments mediate functionally distinct cellular activities.
Three key in vivo observations support the idea that altered cell:matrix interactions regulate the spatially precise pattern of collagenase-1 production in migrating keratinocytes during wound repair. One, as we (3, 4) and others reported (6), immunostaining for type IV collagen or laminin showed that collagenase-1-positive keratinocytes are not in contact with a basement membrane but rather are moving over the dermal or wound bed matrix. Two, collagenase-1 is not expressed by basal keratinocytes in nonulcerative pyogenic granuloma or in blisters, such as bullous pemphigoid, which separate above basement membrane, but this MMP is expressed by migrating keratinocytes in blisters that form below the basement membrane, such as in recessive dystrophic epidermolysis bullosa (3, 4). Three, in acute wounds (3, 6) and in cultured skin equivalent models (20), collagenase-1 expression ceases once re-epithelialization is completed and a basement membrane has re-formed. Together, these findings support the hypothesis that keratinocytes acquire a collagenolytic phenotype upon contact with the dermal matrix, and the data we provide here indicate that native type I collagen is the inductive molecule in the dermis that controls this response. Furthermore, this induction is specific for collagenase-1. Although keratinocytes also produce 92-kDa gelatinase, stromelysin-1, and stromelysin-2, we have not detected any changes in expression of these MMPs mediated solely by matrix (21).
The type I collagen-binding receptor, 2
1, is constitutively
expressed on keratinocytes (22, 23), and as we reported recently, this
integrin transduces collagen-mediated induction of collagenase-1 (5).
Similarly, collagen stimulates collagenase-1 expression in fibroblasts
via ligand binding to
2
1 (24, 25). Although basal keratinocytes
also express
1
1 and
3
1, keratinocytes preferentially use
2
1 to bind to type I collagen (26). The interaction of
keratinocytes with the dermal matrix, and in particular with type I
collagen, may provide an early and critical signal to initiate the
epithelial response to wounding. Because the epidermis is not normally
in contact with type I collagen, it is tempting to speculate that the
basal production of
2
1 keeps keratinocytes primed and ready to
respond to injury.
Earlier studies by Woodley and associates showed that keratinocytes on nonviable dermis produce collagenolytic enzymes (27) and that contact with type I collagen enhances basal production of this activity (28). Although seemingly similar, there are notable differences between their and our experimental conditions that impact on our respective findings. Whereas we grew keratinocytes in high Ca2+ medium, which promotes differentiation and duplicates the subpopulations of keratinocytes seen in vivo (Fig. 1), Petersen et al. (29) used low Ca2+ medium which maintains the keratinocytes in a basal phenotype (30). Thus, this change in culture conditions may lead to changes in cell behavior and responsiveness. Indeed, Petersen et al. (31) demonstrated that keratinocytes grown in low Ca2+ medium constitutively expressed collagenase-1, whereas, as we show here, collagenase-1 is induced in keratinocytes in high Ca2+ medium only if plated on the appropriate substratum.
In addition to native type I collagen, contact with vitronectin and
type IV collagen also mediated induction of collagenase-1 in
keratinocytes (Table I). The wound bed is rich in vitronectin (32), and
contact with this serum glycoprotein may provide an additional
matrix-derived signal that can regulate keratinocyte behavior during
wound healing. However, the vitronectin receptor, v
5, is not
present in intact skin but is expressed in migrating basal cells in
response to injury (33) but is apparently activated in isolated
keratinocytes (34). Thus, this matrix protein is likely not involved in
rapid induction of collagenase-1 after wounding but may play a role in
maintaining the collagenolytic phenotype of migrating keratinocytes.
The wound environment is also rich in fibrin and fibronectin, but
primary keratinocytes did not attach to these substrates (Table I).
These findings were not surprising. Grinnell and co-workers
demonstrated that keratinocytes freshly isolated from skin do not
adhere to fibronectin (35), and keratinocytes in intact skin do not
express
5
1 or the
v subunit (33, 36), the integrins that bind
fibronectin and fibrin, respectively (34). As for
v
5,
5
1 is
induced in response to wounding and is expressed on the basal surface of the same population of keratinocytes producing collagenase-1 (3).
The lack of
5
1 in intact skin supports the conclusion that
binding to fibronectin does not induce collagenase-1 expression in
keratinocytes. In contrast, fibronectin fragments binding
5
1 stimulate collagenase-1 expression in fibroblasts (37), indicating that
fundamentally distinct mechanisms control MMP expression in different
cell types.
We believe that type IV collagen-mediated induction of collagenase-1 by
keratinocytes, which has also been reported by others (28), is an
in vitro artifact. Because they constitutively express 1
integrins, keratinocytes in intact skin can interact with type IV
collagen in the basement membrane. However, our in vivo
observations (3) and our RT-PCR data (Fig. 4) demonstrate that
keratinocytes in intact skin do not express collagenase-1. In addition,
primary keratinocytes grown on Matrigel®, which contains type IV
collagen, do not make collagenase-1 (Table I), presumably because
laminin-1 overwhelms any potential inductive effect of type IV
collagen. Because type IV collagen in the context of a basement
membrane does not induce collagenase-1 expression in keratinocytes, the relevance of its ability to do so in a pure form is questionable. After
all, other than that in anchoring plaques, keratinocytes in
vivo would likely not interact with "pure" type IV
collagen.
The observation that cultured keratinocytes on basement membrane or cells in intact skin do not express collagenase-1 suggests that a basal lamina protein blocks enzyme production. We show here that laminin-1, but not laminin-5, effectively represses type I collagen-mediated induction of collagenase-1 (Fig. 6). Analogously, laminin-1 and type I collagen mediate opposite effects on breast epithelial cell differentiation (38, 39). During wound healing in vivo, laminin-5 and collagenase-1 are expressed by migrating keratinocytes (18). Zhang and Kramer (40) reported that laminin-5 promotes keratinocyte migration, and we recently reported that keratinocyte migration on a collagen matrix requires the activity of collagenase-1 (5). (Incidentally, laminin-5, as well as laminin-1 and type IV collagen, are not substrates for collagenase-1.) Thus, this basement membrane glycoprotein and this MMP serve distinct yet required functions during re-epithelialization.
Laminin-1 is deposited in the newly formed basement membrane just behind the migrating front of epidermis (33). As re-epithelialization progresses, the mass of laminin-1 deposited under the previously migrating keratinocytes would accumulate, providing a site-specific mechanism to down-regulate collagenase-1 expression. Consistent with this idea, our data (Fig. 6) demonstrate that relatively small concentrations of laminin-1 can block the inductive effect of native type I collagen. The molecular mass of a triple helical type I collagen monomer is about 300 kDa and is about 900 kDa for a fully processed laminin-1 heterotrimer. Thus, assuming one binding event per molecule, one laminin-1 molecule effectively blocked the induction of collagenase-1 mediated by about 3,000 collagen molecules. Because type I collagen is so abundant in the dermis, it is not surprising that the inhibitory effect of laminin-1 is so potent.
In addition to cell:matrix interactions, our data suggest that cell:cell contacts influence the turn-off of collagenase-1 expression at the completion of re-epithelialization. Plating keratinocytes at a confluent density prevented induction of collagenase-1, even though the cells were in contact with type I collagen (Fig. 5). Because collagenase-1 expression was assessed soon after plating, inhibition of enzyme production was not due to accumulation of keratinocyte-derived basement membrane proteins. These data indicate that contact with type I collagen is not sufficient to induce collagenase-1 expression in keratinocytes; the cells must also have the ability to migrate. Conversely, keratinocyte migration in and of itself does not induce collagenase-1 expression. For example, collagenase-1 is not expressed by keratinocytes involved in re-epithelialization of lesions with an intact basement membrane, such as suction blisters or early bullous pemphigoid blisters (3, 4). In addition, collagenase-1 is not expressed by cultured keratinocytes on gelatin, even though these cells can migrate on this substrate (5). Thus, induction of collagenase-1 requires both contact of the keratinocytes with the appropriate matrix stimulus (native collagen) and the ability of the cells to migrate.
In summary, our findings suggest that, as keratinocytes move from the basement membrane onto the dermal matrix, contact with native type I collagen mediates induction of collagenase-1. The invariable expression of collagenase-1 by migrating basal keratinocytes in all forms of wounds indicates that the activity of this MMP serves a critical and required function during re-epithelialization. In contrast, collagenase-1 is not expressed in squamous or basal cell carcinomas (41, 42), and cells derived from squamous cell carcinomas did not express collagenase-1 in response to collagen or other stimuli (Table II). These findings suggest that the proteolytic requirements of normal epithelial repair differ from those needed for invasion of carcinoma cells.
We thank Dr. Alice Pentland and her associates for their assistance in obtaining tissue for keratinocyte cultures, Dr. E. C. Crouch for supplying highly purified bacterial collagenase, Dr. Steven Frisch for the collagenase-1 promoter construct, Dr. Robert E. Burgeson for laminin-5, Dr. Douglas Dean for the luciferase construct, Dr. Norbert Fusenig and Dr. John C. Ansel for keratinocyte cell lines, and Dr. Ulpu Saarialho-Kere, Jill Roby, and Teresa Tolley for assistance with in situ hybridization studies.