Delayed Wound Healing in Keratin 6a Knockout Mice

doi:10.1128/MCB.20.14.5248-5255.2000

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Molecular and Cellular Biology, July 2000, p. 5248-5255, Vol. 20, No. 14
0270-7306/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Delayed Wound Healing in Keratin 6a Knockout Mice

Sonja M. Wojcik,¹ Donnie S. Bundman,¹ and Dennis R. Roop¹^,²^,^*

Department of Molecular and Cellular Biology¹ and Department of Dermatology,² Baylor College of Medicine, Houston, Texas 77030

Received 7 February 2000/Returned for modification 6 April 2000/Accepted 13 April 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Keratin 6 (K6) expression in the epidermis has two components: constitutive expression in the innermost layer of the outerroot sheath (ORS) of hair follicles and inducible expression inthe interfollicular epidermis in response to stressful stimulisuch as wounding. Mice express two K6 isoforms, MK6a and MK6b.To gain insight into the functional significance of these isoforms,we generated MK6a-deficient mice through mouse embryonic stemcell technology. Upon wounding, MK6a was induced in the outerORS and the interfollicular epidermis including the basal celllayer of MK6a^+/+ mice, whereas MK6b induction in MK6a^/ mice was restricted to the suprabasal layers of the epidermis.After superficial wounding of the epidermis by tape stripping,MK6a^/ mice showed a delay in reepithelialization from the hair follicle.However, the healing of full-thickness skin wounds was not impairedin MK6a^/ animals. Migration and proliferation of MK6a^/ keratinocytes were not impaired in vitro. Furthermore, the migratingand the proliferating keratinocytes of full-thickness wounds inMK6a^/ animals expressed neither MK6a nor MK6b. These data indicatethat MK6a does not play a major role in keratinocyte proliferationor migration but point to a role in the activation of follicularkeratinocytes after wounding. This study represents the firstreport of a keratin null mutation that results in a wound healingdefect.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The ability of the epidermis to perform its function as a protective barrier is dependent to a significant degree on the presenceand integrity of its keratin network. Keratin proteins form theintermediate filament cytoskeleton of epithelial cells (1,12, 41). Keratins are subdivided into the slightly smalleracidic type I keratins and the larger more basic type II keratins(26). Type I and type II keratins are expressed in pairs, formingobligate heterodimers, which make up the basic building blockfrom which the keratin filaments assemble (11, 40). Keratinocytesexpress different keratin pairs according to their state of differentiation.Cells in the basal compartment, which contains cells with proliferativecapacity such as stem cells and transit-amplifying cells, expresskeratin 5 (K5) and K14. Postmitotic spinous keratinocytes arecharacterized by the expression of K1 and K10. A strict balanceof proliferation, differentiation, and desquamation is normallymaintained in the epidermis, but in case of an injury keratinocyteshave the plasticity to exit this differentiation pathway and respondwith migration and enhanced proliferation, forming a new epitheliumto cover the wound. Under these circumstances a new set of keratins,K6, K16, and K17, is induced (30). A remarkable feature of K6is that there have been descriptions of multiple functional K6genes in several mammals; humans may have seven active K6 genes(43, 46), bovines may have up to three (5, 27), and micehave at least two (38, 44). In contrast to this, the assumedtype I partners of K6, K16 and K17, appear to have only one functionalgene and several pseudogenes (39, 45). While K6, K16, andK17 share the characteristic inducible expression in responseto perturbations of epidermal homeostasis, their constitutiveexpression patterns are not identical. In hirsute skin, K6 andK16 are expressed constitutively in the innermost layer of theouter root sheaths (ORS) of hair follicles (38, 44, 46).This single-cell layer, also known as the companion cell layer,consists of highly differentiated flattened cells, which lie directlyadjacent to Henle's layer of the inner root sheath (14, 15,29). K17, on the other hand, is expressed early during embryonicdevelopment prior to formation of the hair follicle placodes inthe single-layer ectoderm and is later present in the entire ORSof mature hair follicles as well as in sweat and sebaceous glands(24, 31). In addition to this, some body sites devoid of hairexpress K6 and K16 and K17 to various degrees, such as palms,soles, and the nail bed, as do several mucous epithelia such asthe oral cavity, esophagus, trachea, and the vaginal, and analepithelia (26). Both murine K6 isoforms, MK6a and MK6b (designatedMK6 $alpha$ and MK6 $beta$ , respectively, by Takahashi and colleagues (44)),are expressed in the footpad and oral epithelia, and both areinduced after wounding or treatment with phorbol esters (38,44). However, inducible expression of MK6b in the epidermishas been reported to be more suprabasal than that of MK6a, andMK6a but not MK6b has been shown to be expressed in the companioncell layer of the hair follicle (38, 44).

The integral role that keratin filaments play in the maintenance of the structural integrity of the epidermis has now beenwell established, with a large number of reports which documentkeratin mutations, including mutations affecting K6, K16, andK17, as the cause of several inherited genodermatoses (for a recentreview see reference 7). Apart from its role in human disease,K6, because of its unique expression characteristics, is a fascinatingsubject for the experimental study of keratin function. Elucidationof the significance of K6 expression in wound healing or its functionin the epithelia with constitutive expression would not only furtherour understanding of K6 but also potentially provide insight intothe biological necessity of having different sets of keratinsfor different cell types. We have shown that expression of dominant-negativemutants of K6 in the companion cell layer leads to the destructionof these cells (47), and Takahashi and colleagues reported oninducible skin blistering after induction of a dominant-negativeK6 transgene in the epidermis (42). However, the functionalsignificance of a protein is sometimes better evaluated by analyzingthe consequences of its absence. To date, several keratin knockoutmodels have been generated, and the resulting phenotypes mostlyunderscore the role keratins play in providing mechanical supportto epithelial cells. Mice lacking a functional MK10 gene (33)and MK14-deficient mice (21) exhibit epidermal lesions. MK4-deficientmice suffer from fragility in internal epithelia (28), and MK12knockouts display corneal defects (17). Targeting of the embryonickeratins MK8 and MK18 provided results less clear-cut with respectto keratin function. Deletion of MK8 led to midgestational lethality(3) or colorectal hyperplasia (2), depending on the geneticbackground. Targeting of the type I partner of MK8, MK18, resultedin liver pathology apparent only in older mice (22).

We have targeted the MK6a gene, deleting the entire coding region through homologous recombination in embryonic stem (ES)cells. MK6a-deficient mice have no apparent structural defectsin hair follicles, footpads, oral epithelia, or the periderm.They do however exhibit a delay in reepithelialization from thehair follicle after superficial wounding but not in the healingof full-thickness wounds. The lack of MK6a affects both proliferationand migration of the follicular keratinocytes in vivo, but notproliferation or migration of MK6a^/ keratinocytes in vitro. These data indicate that MK6a^/ keratinocytes may not be impaired in proliferation or migrationas such but rather in the activation of one or both. This is thefirst report of a keratin null mutation where the phenotypic consequencesdo not appear related to the structural deterioration or hyperplasticresponse of the affectedcells.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Targeting-vector construction. PCR primers 5'-CTGCTATTGCTGATGCTGAG-3' and 5'-GTCCAACACCTTCACCATTC-3' were used to identify P1 clones from the Genome Systems129/SvJ library that contained both the MK6a and the MK6b genes.The MK6a gene was subcloned and confirmed by restriction mappingand spot sequencing. To generate the 5' arm of the targeting vector,a 5-kb SalI-XbaI fragment directly 5' to the MK6a coding sequencewas ligated to the hprt $Delta$ 3'-neo cassette (35), which containsthe 5' half of a hypoxanthine phosphoribosyltransferase minigeneand a neomycin cassette. For the 3' arm, a 3.2-kb AvaI-BamHI fragmentdirectly downstream of the MK6a stop codon was subcloned to pickup a NotI restriction site. The MK6a targeting vector was constructedby the simultaneous ligation of the following four fragments:a 9.7-kb SalI-NotI fragment containing the previously ligated5-kb 5' arm and the hprt $Delta$ 3'-neo cassette, a 3.2-kb NotI-BamHIfragment that constitutes the 3' arm, a 2.1-kb BamHI-HindIII fragmentcontaining a thymidine kinase cassette (provided by John Lydon,Baylor College of Medicine), and the 3-kb pSK( $-$ ) backbone cutwith HindIII and NotI. The resulting 18-kb targeting vector wastransformed into SureTM cells (Stratagene) and prepared by CsClcentrifugation. Prior to electroporation, the targeting vectorwas linearized with SalI.

Generation of MK6a knockout mice. Mouse ES cells (129/SvEv AB2.2) and the feeder cell line SNL76/7 (25) were kindly provided by Allan Bradley, Baylor Collegeof Medicine. Electroporation, cell culture, drug selection, expansionof clones in 96-well plates, and Southern screening of ES cellDNA were performed according to published protocols (34, 36).DNA for Southern analysis was digested with EcoRV and probed witha 0.9-kb BglII-SalI fragment that lies just outside the 5' armof the targeting vector (see Fig. 1a). The 3' end of the targetedlocus was confirmed by PCR analysis using primers 5'-GGTGGCCTCAGCTCTTCTAC-3',5'-AGATCCACTAGTTCTAGCCTCG-3', and 5'-ACAGGCAGCCTCAGAGACAG-3' (Fig.1a and c). Chimeras were generated by injection of targeted EScells into C57BL/6Nblastocysts.

Animal protocols. Mice were kept under standard housing conditions at the animal facility at Baylor College of Medicine. Wound-healing protocolswere approved by the Center for Comparative Medicine. Mice wereanesthetized using 0.0175 ml of 2.5% Avertin per g of mouse. Forthe duration of each wound-healing experiment acetaminophen (Children'sTylenol) was added to the drinking water at 1 mg/ml and sulfamethoxazole/trimethoprimoral suspension (Apothecon) was added at 1 ml/150 ml. For tape-strippingwounds, mice were shaved and two 1- to 1.5-cm² areas to the left and right of the spine were depilated withNair (Carter-Wallace). The depilated areas were tape strippedeight times with Tesa tape (Bron Tape) and immediately wiped withBetadine solution. Full-thickness wounds were generated in thecenter of the lower back after shaving and wiping with Betadinesolution. A circle 5 mm in diameter was marked on the skin usinga biopsy punch dipped in methylene blue solution and subsequentlyexcised using curved scissors. Wound-healing samples were analyzedhistologically from five +/+ and five $-$ / $-$ animals per time pointfor both tape-stripping and full-thickness wounds. Tape strippingwas considered successful if a crust had formed on top of thedermis without any inflammatory infiltrate within the dermis.Samples that did not have an intact, superficial crust were excludedfrom the analysis. Reepithelialization of tape-stripping woundswas scored visually according to the continuity and thicknessof the epithelium growing under the crust. Full-thickness woundswere assessed according to the lengths of the epithelial tonguesmigrating from both edges of thewound.

BrdU labeling. In vivo bromodeoxyuridine (BrdU) labeling of wounded mice was carried out by intraperitoneal injection of 0.01 ml of a 10-mg/mlsolution of BrdU triphosphate (Sigma) per gram of mouse. Micewere sacrificed 2 h after the BrdU injection. Samples were preparedas described below. For tape-stripping wounds BrdU-positive cellsin the follicles of a series of tissue sections were counted.A minimum of 300 follicles (sections) were counted for each datapoint presented in Table 1, and the standard deviations (SD)werecalculated.

RNase protection analysis. Total RNA was isolated from ear skin with RNAzol B (Tel-Test) 48 h after a single application of 50 µl of 0.1-mg/ml 12-O-tetradecanoyl-phorbol-13-acetate in acetone. The RNA probe forMK6 detects both MK6a and MK6b and has been described previously(38). RNA probes for MK6 and cyclophilin (Ambion) were generatedusing the Riboprobe Gemini II kit (Promega). The RNase protectionassay was performed with the RPA II kit (Ambion), with overnighthybridization at 42°C.

Western blot analysis. Tissue samples were ground in liquid N₂ and then solubilized, electrophoresed, and blotted onto nitrocellulose as previouslydescribed (4). Blots were blocked with 5% nonfat milk-Tris-bufferedsaline and then probed with rabbit anti-K6, sheep anti-K14 (37),and guinea pig anti-K6 (38), followed by alkaline phosphatase-conjugatedanti-rabbit immunoglobulin G (IgG) (Boehringer Mannheim), anti-sheepIgG (Zymed), and anti-guinea pig IgG (Zymed), respectively. Bandswere visualized using nitroblue tetrazolium-BCIP (5-bromo-4-chloro-3-indolylphosphate)solution (Boehringer Mannheim) according to the manufacturer'sinstructions.

Histology. Pieces of tissue were flattened onto filter paper and fixed overnight in Carnoys' solution (ethanol-chloroform-glacial aceticacid; 6:3:1). Samples were then washed in 100% ethanol and processedfor paraffin embedding, and the blocks were sectioned at 5 to6 µm in thickness. Sections were deparaffinized through a gradedseries of xylenes and ethanol and either stained with hematoxylinand eosin or rinsed twice for 10 min in phosphate-buffered saline(PBS) and incubated with the appropriate antibodies. BrdU-labeledsamples were incubated for 12.5 min in 25% HCl following deparaffinizationand one 10-min incubation in PBS and then rinsed three times for10 min in PBS prior to incubation with the antibodies. Samplesfor frozen sections were prepared as previously described (4).

Primary keratinocyte culture. Primary keratinocytes were isolated and cultured as previously described (4). Keratinocytes of 1- to 3-day-old MK6a^/ and MK6a^+/+ littermates were plated at 10⁵ cells per cm² in low-Ca²⁺ medium (50% Eagle minimal essential medium without Ca²⁺ (Gibco BRL) and 50% fibroblast-conditioned medium (10) withfinal concentrations of 0.05 mM Ca²⁺, 8% fetal bovine serum, and 4 ng of epidermal growth factor/ml).

[³H]thymidine incorporation. Keratinocyte cultures were plated in triplicate, refed at 24 h, and allowed to grow in low-Ca²⁺ medium for a total of 46 h. [³H]thymidine was diluted into the medium to a final concentrationof 1 µCi/ml, and the cells were grown in its presence for 2 h.The cultures were then washed three times with PBS and incubatedwith 8% trichloroacetic acid for 5 min, followed by two briefwashes with 8% trichloroacetic acid. The cells were then solubilizedin 1 N NaOH for 30 min, and the solution was neutralized by adding1 N HCl. The samples were counted in a scintillation counter.The cell number 24 h after plating was assessed for each batchof cells in triplicate with a modified crystal violet stainingprocedure (9). The scintillation counts were then adjustedfor the cellnumber.

Double-label immunofluorescence. All sections were blocked with 1% bovine serum albumin in PBS for 30 min. Two-color immunofluorescence was performed by sequentialincubation with primary antibodies and fluorescein isothiocyanate(FITC)- or Texas red (TxRed)-conjugated secondary antibodies.Primary antibodies used were rabbit anti-K6, rabbit anti-K14,guinea pig anti-K14 (37), and rabbit anti-MK16 (32). Furthermore,a guinea pig anti-K6 antibody (38), which in mice is specificfor MK6b, and guinea pig anti-K6 generated to the synthetic peptideCGSKKSYRQ (corresponding to a CG linker peptide and the last sevenamino acids of MK6a) were used. Secondary-antibody conjugatesused were anti-rabbit FITC (Dako) and anti-guinea pig TxRed (Vector).For BrdU-labeled samples the primary keratin antibody was dilutedinto the FITC-conjugated anti-BrdU (Becton Dickinson) followedby a second incubation with anti-guinea pig TxRed(Vector).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Deletion of the entire MK6a coding region from the genome. Initial Southern analysis of two overlapping P1 clones containing the MK6 locus indicated that there might be as many as fiveMK6 genes, the MK6a and MK6b genes and three additional genessimilar to K6 which lie downstream of the MK6b gene (data notshown). We decided to target the MK6a gene, since previous analysisof MK6a and MK6b transgene expression had indicated that MK6awas the most widely expressed isoform (38). The targeting vectorwas designed to replace the entire MK6a coding sequence with aneomycin resistance selection cassette as well the 5' half ofan hprt minigene and a loxP site; the complete cassette is designatedhprt $Delta$ 3'-neo (Fig. 1a). This cassette was used because it wouldallow us to delete the entire MK6 locus with a second targetingevent followed by transfection with a cre recombinase expressionvector, should the MK6 genes downstream of MK6b prove to be active(for a more detailed explanation of this targeting strategy seereference 35). The MK6a replacement vector was introduced into129/SvEv AB2.2 ES cells. Successful gene targeting was confirmedby Southern blotting, using a 5' external probe (Fig. 1b) as wellas an internal probe to the neomycin cassette (data not shown).Germ line transmission was obtained from chimeras of two independentclones, and one clone was selected for subsequent analyses. Matingsof MK6a^+/ animals produced all genotypes, +/ $-$ , +/+, and $-$ / $-$ , at the expectedMendelian ratio. Offspring from heterozygous crosses were screenedusing a set of three primers to the 3' end of the targeted locus(Fig. 1a and c). MK6a-deficient mice were indistinguishable fromtheir wild-type and heterozygous littermates at birth and grewhair synchronously with their littermates. Subsequent hair cyclesalso showed no abnormalities in onset or duration. Older MK6a^/ mice (1.5 years) showed no abnormal deterioration of coat, mucousepithelia, or footpad compared to wild-type animals of the sameage and genetic background. The absence of the MK6a transcriptin MK6a^/ mice was confirmed by RNase protection analysis (Fig. 1d). Westernblot analysis of whole-skin samples taken on postnatal day 16,when the hair follicles were in anagen, showed that MK6a was absentin MK6a^/ samples (Fig. 1e, left). The MK6 antibody used for the left panelwas raised to the C terminus of MK6a and did not recognize MK6bafter denaturation but did detect MK6b on unfixed frozen sectionsof MK6a^/ samples. Use of another K6 antibody, which in mice reacts onlywith MK6b (anti-MK6b) (38) (Fig. 1e, middle) revealed that MK6bwas expressed at considerably lower levels than MK6a in both theMK6a^+/+ and MK6a^/ mice. MK6b was also expressed at significantly lower levels thanMK6a in the periderm and telogen hair follicles (data not shown).There were no differences in the protein levels of MK6b betweenMK6a^+/+ and MK6a^/ mice in any of the samples tested.

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FIG. 1. Targeting of MK6a. (a) A replacement vector containing the hprt $Delta$ 3'-neo cassette was used to delete the MK6a coding region through homologous recombination. RV, EcoRV restriction sites, digestion of which generates a 9-kb fragment for the wild-type locus and a 7-kb fragment for the targeted allele; short bar, position of the 5' external probe; triangles, positions of the PCR primers used in the 3' screen. (b) Genomic Southern blot showing the wild-type 9-kb and the targeted 7-kb fragments detected with the 5' external probe. (c) Genomic PCR of the 3' end of the targeted locus showing a 359-bp product for the MK6a^+/+ genotype, a 265-bp product for MK6a^/, and both fragments for MK6a^+/. (d) RNase protection assay showing absence of the MK6a transcript in MK6a^/ animals. The RNA was isolated from the 12-O-tetradecanoyl-phorbol-13-acetate-treated ears of littermates. The probe was designed to protect 268 bases in MK6b and 382 bases in MK6a. Note that two bands are generated for the MK6a transcript, most likely due to a polymorphism present in the C57BL/6N strain, resulting in partial degradation of the 382-bp fragment. The probe spans exons three to six, and a single MK6a band was observed in BALB/c mice, the strain from which the cDNA was isolated. A cyclophilin probe was used as a loading control. (e) Western blot analysis of whole skin during anagen showing that MK6a is absent in MK6a^/ mice (left). Note that MK6b is present at lower levels than MK6a and is not upregulated in MK6a^/ mice (middle). MK14 was used as a loading control (right). Note that the doublet bands for MK6a and MK14 most likely are due to differential phosphorylation. Lane M, 84- and 51-kDa size marker bands; arrow, position of the 62.5-kDa band.

MK6a and MK6b are expressed in the companion cell layer and the periderm. To confirm that MK6b expression detected in whole skin by Western blot analysis was due to expression in the companion celllayer, we performed immunofluorescence analysis utilizing theanti-MK6b antibody. MK6b was expressed in the companion cell layerof telogen hair follicles of both MK6a^/ (Fig. 2a) and MK6a^+/+ (Fig. 2a, inset) animals, as well as in the companion cell layersof anagen hair follicles of both genotypes (Fig. 2b). The sameMK6b-specific antibody used on embryonic-day-16.5 skin showedthat MK6b was also expressed in the periderms of both MK6a^+/+ (Fig. 2c) and MK6a^/ (Fig. 2d) mice. The constitutive expression pattern observedfor MK6b in the hair follicle and periderm is identical to theexpression pattern of MK6a in these compartments (38).

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FIG. 2. Immunofluorescence analysis showing MK6a and MK6b expression patterns. (a through d) MK14 staining in green (FITC) and the overlapping MK6b staining in yellow (TxRed). (a) MK6b (yellow) is present in the companion cell layer (arrow) of telogen hair follicles in MK6a^/ animals and MK6a^+/+ animals (inset). (b) MK6b (yellow) expression in the companion cell layer (arrow) of anagen hair follicles in MK6a^/ and MK6a^+/+ mice (inset). Note that the outer ORS is only one cell layer thick in this section and only positive for MK14 (green); the outer ORS and the MK6b-positive companion cell layer are most readily distinguished in the lower part of the section (arrow). (c and d) MK6b is expressed in the periderm (yellow) of embryonic day 16.5 skin of MK6a^+/+ and MK6a^/ animals. Note that the periderm is a single-cell layer covering the developing epidermis, which is highlighted by the MK14 antibody in green. (e and f) Samples taken from the edge of 34-h-old tape-stripping wounds. MK14 staining (TxRed) highlights the epidermis and the ORS of the hair follicles. (e) MK6 induction (yellow) in MK6a^+/+ animals is apparent in the entire epidermis and the ORS of the hair follicle. (f) MK6b in MK6a^/ animals is induced in the suprabasal layers of the epidermis but not in the basal layer of the epidermis or the ORS (arrows). Note that MK6b staining is not seen in the companion cell layer of the follicle because the antibody used here for comparison with the MK6a^+/+ sample does not recognize MK6b in the companion cells of fixed tissue but recognizes it on unfixed frozen sections (not shown). (g) MK6a is expressed throughout the dorsal tongue epithelium in MK6a^+/+ animals (TxRed). The antibody recognizes both MK6a and MK6b. The overlapping yellow staining shows the suprabasal expression of MK16 in the papillae. Note that in the basal layers (arrow) MK6a (red) is expressed but not MK16. (h) MK6b (yellow) is restricted to the uppermost cells of the papillae in MK6a^/ animals. The MK16 staining (green) in the MK6a^/ tongue epithelium is identical to the MK16 staining seen in the MK6a^+/+ sample. (i) MK6b (yellow) is expressed suprabasally in the hard palate (counterstained with MK14; TxRed) in MK6a^/ mice. (j) Suprabasal MK6b expression in MK6a^/ footpad, which was counterstained with MK14 (TxRed). Note that MK6 expression in the footpad is patchy. (a, b, e, and f) Carnoys fixed samples; (c, d, and g to j) unfixed frozen sections. Scale bars, 50 µm.

MK6a but not MK6b is inducible in the basal compartment of the epidermis and the outer ORS of the hair follicles. Our previous analysis of expression of MK6b constructs in transgenic animals (38), as well as in situ hybridization reportedby Takahashi and colleagues (44), had already indicated thatMK6b induction in the epidermis is suprabasal. Immunofluorescenceanalysis of inducible MK6 expression at the edge of a wound inMK6a^+/+ animals showed MK6 induction throughout the entire epidermisand ORS (Fig. 2e). In contrast to this, in MK6a^/ mice no inducible MK6 expression in either the basal layer ofthe epidermis or the outer layers of the ORS of the hair follicleswas observed (Fig. 2f). This confirmed unequivocally that in micethe MK6a isoform alone is responsible for inducible MK6 expressionin the basal layer of the epidermis as well as the outer ORS,while MK6b can only be induced in the suprabasal layers of theepidermis. Constitutive expression of MK6b in tongues (Fig. 2h),palates (Fig. 2i), and footpads (Fig. 2j) of MK6a^/ mice was also suprabasal, whereas wild-type mice showed MK6 expressionin all layers of these epithelia (data for MK6a^+/+ palates and footpads are not shown). Interestingly, the expressionof MK6a in wild-type mice was observed throughout the entire dorsalepithelium of the tongue, whereas MK16 expression was more suprabasaland restricted to the papillae (Fig. 2g). MK6b expression in thetongues of MK6a^/ mice was also restricted to the papillae, but, unlike MK16, MK6bwas only present in the cells at the very upper edge of thesestructures (Fig. 2h).

MK6a^/ mice show a delay in reepithelialization from the hair follicle. If the epidermis of adult mice is destroyed by abrasion, reepithelialization occurs from the hair follicle epithelium. BecauseMK6a^/ mice lack inducible MK6 expression in the outer ORS, we analyzedthe kinetics of reepithelialization in MK6a^+/+ and MK6a^/ mice in an abrasion wound model. The epidermis was destroyedby tape stripping (eight times with Tesa tape) of shaved, depilatedback skin. This procedure removes the suprabasal cell layers andleaves behind but kills the basal layer. A crust then forms underthe dead basal layer, and reepithelialization occurs from thehair follicles, with the new epidermis forming under the crust.Tape stripping during telogen, when the hair follicles are notdeeply anchored in the dermis, proved to be problematic. Althoughsome samples showed less reepithelialization in MK6a^/ than in MK6a^+/+ mice, the majority of samples in these experiments had to bediscarded because tape stripping during telogen often damagedthe underlying connective tissue so severely that reepithelializationoccurred from the edge of the wound rather that from the hairfollicles (data not shown). During anagen, the active growth phase,the hair follicles reach down deep into the hypodermis, stabilizingthe skin during tape stripping. In anagen, keratinocytes in theORS are actively dividing. Tape stripping during anagen revealedno obvious differences between MK6a^+/+ and MK6a^/ mice at 23 h after wounding (data notshown).

To avoid the skin fragility problems of telogen and the activated ORS keratinocytes of anagen hair follicles, mice were tapestripped in late catagen, when the hair follicles have almostcompletely regressed but are still deep enough to stabilize thedermis. C57BL/6N (F4) mice were tape stripped during their secondcatagen, at the age of 39 to 45 days. Since the second hair cycleis not as perfectly synchronized as the first one is, each mousewas checked for the progression of the second anagen over theback, as judged by the disappearance of pigmentation from theback skin. Tape stripping of the epidermis at this stage was successful,and MK6a^/ mice showed a clear delay in reepithelialization from the hairfollicles compared to MK6a^+/+ mice (Fig. 3 and 4). In MK6a^+/+ mice, at 30 h after tape stripping a single layer of new epitheliumcould be observed in some areas under the crust (Fig. 3a and 4a).By 34 h, the cell layer became continuous and one to three cellsthick (not shown), and by 42 h the new epithelium had thickenedto two to four cell layers (Fig. 3c and 4c). In MK6a^/ mice no reepithelialization was observed at 30 h (Fig. 3b and4b), but by 34 h the first follicular keratinocytes had reachedthe dermal surface (not shown). By 42 h MK6a^/ mice showed a discontinuous new epithelium one or two cell layersthick (Fig. 3d and 4d), which was easily distinguishable fromthe thicker epithelium present at this time point in wild-typemice (Fig. 3c and 4c). Two days after wounding, MK6a^/ mice had also formed a continuous multilayered epithelium andthe MK6a^/ samples became harder to distinguish from the MK6a^+/+ samples (data not shown).

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FIG. 3. Immunofluorescence analysis of reepithelialization after tape stripping. All samples were stained with antibodies to MK14 (red) and MK6 (yellow). The dead old basal layer is still present on top of the crust (thick arrows) and is positive for MK14 but negative for MK6. (a) MK6a^+/+ animals show some areas of reepithelialization 30 h after tape stripping. A single-cell layer, positive for MK6, is apparent under the crust (thin arrows). Note the induction of MK6a in the ORS of the hair follicles. (b) MK6a^/ mice show no reepithelialization from the hair follicles 30 h after tape stripping. Arrowheads, boundary of crust and dermis; thick arrows, old basal layer on top of the crust. (c) MK6a^+/+ samples taken 42 h after tape stripping show a continuous epithelium of two to four cell layers under the crust (thin arrows). (d) MK6a^/ samples taken 42 h after tape stripping show a discontinuous mostly single-cell layer epithelium under the crust (thin arrows). Note that the follicular cells that reach the dermal surface do not induce MK6b until a suprabasal layer is present. Scale bar, 100 µm.

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FIG. 4. Histological analysis of reepithelialization after tape stripping. Star, crust covering the denuded dermis; arrows, new epithelium regrowing from the hair follicles. (a) MK6a^+/+ follicle 30 h after tape stripping with a single-cell layer of new epithelium (arrows) beginning to grow out from the follicle. (b) MK6a^/ follicle 30 h after tape stripping without any sign of reepithelialization. (c) MK6a^+/+ follicle 42 h after wounding with a newly formed epithelium (arrows), which is two to four cell layers thick. Note that the thickest part of the epithelium can be found above the follicle. (d) MK6a^/ follicle 42 h after tape stripping with a single-cell layer of new epithelium (arrow) on one side of the follicle. Scale bar, 50 µm.

Both migration and proliferation of MK6a^/ follicular keratinocytes are delayed in vivo. In an attempt to define whether the delay in reepithelialization from the hair follicle in MK6a^/ mice was due to a defect in migration or proliferation of MK6a-deficientfollicular keratinocytes, mice were injected intraperitoneallywith BrdU triphosphate 2 h prior to being sacrificed. If the delaywere solely due to an impairment of migration, one might havepredicted a buildup of labeled follicular keratinocytes in MK6a^/ mice. In both MK6a^+/+ and MK6a^/ mice proliferation of follicular keratinocytes and their migrationout of the follicle appeared to be closely linked. At the 34-htime point, when MK6a^+/+ mice showed a continuous one- to three-cell layer epitheliumand reepithelialization was just beginning in MK6a^/ animals, we counted fewer BrdU-labeled cells per follicle inMK6a^/ mice than in MK6a^+/+ mice (Table 1). At 42 h, when the MK6a^+/+ mice had formed a continuous two- to four-cell layer epitheliumand MK6a^/ animals had formed a discontinuous single-layer epithelium, thenumber of labeled follicular keratinocytes had increased for bothgenotypes but the labeling index for MK6a^/ follicles was still lower (Table 1).

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TABLE 1. Numbers of BrdU-positive cells in follicle sections^a

Full-thickness wounds in MK6a^/ mice heal without delay. Since the lack of MK6a in the follicular keratinocytes in MK6a^/ mice seemingly caused a delay in the migration of those cellsout of the follicle, we next tried to determine whether the absenceof MK6a in basal epidermal keratinocytes would impair the migrationof the epithelial tongue into a full-thickness wound bed. Full-thicknesswounds were created on the lower backs of C57BL/6N (F4) mice duringtelogen. Mice were sacrificed, and the wounds were excised ondays 1 to 3, 5, and 7 after wounding. Histological analysis revealedno differences in the progress of the epithelial tongue from theedge of the wound between MK6a^+/+ and MK6a^/ animals (data not shown). Immunofluorescence analysis of day5 wounds showed MK6 staining throughout the newly forming epitheliumin wild-type mice (Fig. 5a), whereas MK6b was not present in thebasal three or four layers in MK6a^/ animals (Fig. 5b). MK16 was expressed suprabasally in the migratingtongue and double staining for MK16 and MK6 in MK6a^/ animals revealed that MK16 induction occurs in cells below thoseexpressing MK6b (Fig. 5c). The absence of MK6 in the bottom layersand the very tip of the epithelial tongue does not appear to impairthe ability of the keratinocytes to migrate out into the woundbed. In vivo BrdU labeling of day-5 full-thickness wounds showedproliferating cells in the three or four basal cell layers (Fig.5a and b). In MK6a^/ mice the BrdU-positive layers of the epithelial tongue did notexpress MK6b. The fact that BrdU staining and suprabasal MK6bstaining in the MK6a^/ sample do not overlap (Fig. 5b) indicates that in vivo MK6b,unlike MK6a (Fig. 5a), is not expressed in the keratinocytes thatproliferate after wounding.

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FIG. 5. Immunofluorescence analysis of full-thickness wounds. Arrow, direction of migration of the epithelial tongue; star, crust covering the wound; line, boundary of the migrating epithelial tongue and the granulation tissue. (a) MK6a^+/+ 5-day-old full-thickness wound. All layers of the migrating epithelial tongue are MK6 positive (red). Note that in order to show a well-preserved wound, fixed tissue, on which this MK6 antibody results in weaker staining of the basal layers, is shown; however, this is not the case on unfixed frozen sections (not shown). Proliferating keratinocytes in the bottom layers of the epithelial tongue are BrdU (FITC) and MK6a (TxRed) positive and therefore appear to have yellow nuclei. The proliferating cells in the granulation tissue are only BrdU positive, and the nuclei appear green. (b) MK6a^/ 5-day-old full-thickness wound. Note that the BrdU-positive, proliferating keratinocytes are negative for MK6b. (c) Double staining for MK16 (FITC) and MK6 (TxRed) in MK6a^/ animals reveals that MK16 is induced in cells below those expressing MK6b. Scale bar, 50 µm.

Proliferation and migration of MK6a^/ keratinocytes are not affected in vitro. Since MK6a^/ follicles showed lower labeling indices, we compared the abilities of MK6a^+/+ and MK6a^/ keratinocytes to proliferate in vitro. Incorporation of [³H]thymidine resulted in values of 2,661 cpm (standard deviation[SD], 163) for MK6a^+/+ cultures and 2,527 cpm (SD, 76) for MK6a^/ cultures, indicating that there was no significant differencein the proliferation rates in vitro. Migration of MK6a^+/+ and MK6a^/ keratinocytes in vitro was tested on collagen type I, collagentype IV, fibronectin, and laminin substrates by assessing gapclosure rates of scrape wounds (data not shown). No differencesin the migration rates of MK6a^+/+ and MK6a^/ keratinocytes were apparent in vitro. MK6b expression under cellculture conditions was negligible, with less than 0.5% of MK6a^/ keratinocytes expressing MK6b in low-Ca²⁺ media, whereas MK6a was expressed in every cell of MK6a^+/+ cultures (notshown).

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

MK6a is necessary for fast reepithelialization from the hair follicle after wounding. To analyze a wound-healing process where the presence of the suprabasal MK6b isoform would not obscure a possible defect,we chose to look at reepithelialization from the hair follicle.The MK6a^/ mice indeed showed a clear delay in the kinetics of this processcompared to wild-type mice. With the degree of reepithelializationas a gauge, 42-h-old tape-stripping wounds on MK6a^/ mice appear similar to 30-h-old wounds on MK6a^+/+ mice. MK6a^/ follicle reepithelialization could therefore be considered tolag behind MK6a^+/+ follicle reepithelialization a maximum of 12 h. While a delayof half a day or less may appear subtle, outside of the laboratory,especially with the potential for developing an infection, sucha delay may translate into a difference in likelihood ofsurvival.

Implications for the role of MK6 in keratinocyte proliferation. Having established that lack of MK6a impairs follicular reepithelialization, we wanted to assess whether this might be dueto a defect in the proliferation rate or migration speed of thefollicular keratinocytes. While K6, K16, and K17 are frequentlydescribed as hyperproliferation-associated keratins (16, 19),the MK6a-deficient mice make obvious the fact that this associationdoes not mean that MK6 induction is necessary for proliferationof keratinocytes after wounding. In vivo BrdU labeling showedthat the basal keratinocytes of the migrating epithelial tonguein full-thickness wounds proliferate in the absence of MK6 andso do the follicular keratinocytes of MK6a^/ mice, albeit with a delay in the onset of proliferation. Althoughthe MK6a^/ follicles clearly had lower BrdU labeling indices than MK6a^+/+ follicles, this may indicate that migration and proliferationof follicular keratinocytes are closely linked, rather than indicatinga primary proliferation defect. This interpretation is supportedby the observation that, for both genotypes, the follicles thatshowed the most significant amount of reepithelialization tendedto contain the highest number of BrdU-positive cells (not shown).In an organotypic wound-healing model, it has been demonstratedthat the proliferative burst occurs after the onset of migrationfrom the edge of a wound (8). It therefore appears possiblethat the delay in proliferation and migration of the follicularkeratinocytes could be due to a primary defect in either the speedor onset of migration. If the ORS keratinocytes of the MK6a^/ mice were slower to migrate out of the follicle, this might causea delay in proliferation if migration is necessary to stimulateproliferation.

Implications for keratinocyte migration in wound healing. While the delay in follicular reepithelialization could be explained by a migration defect, the absence of a migration defectin vitro and in the reepithelialization of full-thickness woundsargues against a prominent role of MK6a and also of MK6b in keratinocytemigration. The cultured keratinocytes were primarily derived fromthe epidermis, and migration out of the hair follicle cannot beaccurately reproduced in vitro; however the MK6a^/ keratinocytes in full-thickness wounds were migrating in theirnative context of a three-dimensional wound bed. The in vivo stainingpattern of the MK6a^/ epithelial tongue, with MK6b present only in suprabasal, BrdU-negativecells, is compatible with a model where the MK6b-positive cellswere generated through displacement and differentiation from thepool of dividing cells below (23). We think it unlikely thatthe contribution of the MK6b-positive suprabasal cells to theprogression of the epithelial tongue is an actual migration process.Once a keratin is expressed and assembled into the network, itis generally thought to be retained in the filament network evenafter expression ceases; for instance, the MK14 protein, whichis expressed only in basal cells, is detected throughout the entireepidermis. Since the very tip and the bottom layers of the epithelialtongue were MK6b negative, migration of MK6b-positive cells wouldrequire that these cells migrate to the front and bottom of thetongue and then turn off MK6b expression and degrade the protein.A scenario where impairment of follicular reepithelializationis due to slower migration of MK6a^/ follicular keratinocytes therefore implies that migration ofthe cells out of the follicle has different requirements thanmigration in a full-thickness wound bed. Follicular and full-thicknessreepithelialization might, for instance, differ in their requirementsfor MK16. Human K16 has been suggested to play a role in the onsetof reepithelialization of full-thickness wounds through a rearrangementof the preexisting keratin network (30). Although this hypothesiswas partly based on the in vitro properties of HK16 (30), whichMK16 does not appear to share (32), both may still have similarin vivo roles. In the epithelial tongues of full-thickness woundsMK16 was induced in all suprabasal layers but only in isolatedcells of the basal layer. As a consequence of this, two or threecell layers in the MK6a^/ epithelial tongue contain MK16 but not MK6. If K6 and K16 inductionwere critical for the migration of keratinocytes and if the networkproperties were indeed due to K16 alone (30), MK16, upon integrationinto the MK5/MK14 network, could impart its properties onto thekeratin network even in the absence of MK6a. Since follicularreepithelialization was impaired in spite of the fact that MK16was induced in part of the ORS (not shown), follicular and full-thicknessreepithelialization may differ in their needs for not only MK6abut alsoMK16.

Implications for a potential role of MK6a in keratinocyte activation after wounding. Since migration and proliferation of MK6a^/ keratinocytes are not affected in vitro or in full-thickness wound healing, a possibleexplanation for the delay in follicular reepithelialization wouldbe that the MK6a^/ follicular keratinocytes may be slower to be activated than wild-typecells but, once activated, migrate and divide at the same ratesas wild-type cells. A primary effect of the MK6a protein on thestructure and properties of the preexisting keratin network wouldqualify as a role for MK6a in keratinocyte activation. This scenariowould, however, not explain why reepithelialization during anagen,when the ORS keratinocytes are already actively dividing and invadingthe connective tissue, was not delayed in the MK6a^/ mice. Although MK6a is not induced in the outer ORS during anagen,the follicular cells may already be in a state of activation similarto the one achieved after wounding, and all that is required isthe redirection of migration towards the dermal surface. It thereforeappears possible that there is some intersection between the presenceof the MK6a protein in the ORS keratinocytes and the regulationof the migratory phenotype or potentially the cell cycle. We haveno direct evidence for such a scenario, since it would requireproof of a direct interaction between MK6a and a protein involvedin signaling necessary for migration or cell cycle control, ofwhich there are no reports for K6 or K16 and K17. However, anotherkeratin, K18, has been shown to bind 14-3-3 proteins (18, 20),a protein family which has been shown to be involved in cell cyclecontrol (6, 13). Furthermore, the colorectal hyperplasiaobserved in the K8 knockout mice in the FVB/N background pointsto a role for K8 in the proliferation or turnover rate of colonepithelial cells (2). It may therefore be of considerable interestto investigate whether K6, K16, and K17 can be shown to interactwith proteins involved in cell cycle control ormigration.

The delay in reepithelialization from the follicle in MK6a^/ mice is the first report of a keratin knockout mouse in which thephenotype is not related to degenerative changes or the hyperplasticresponse of the affected tissue. While we cannot entirely excludethe possibility that the absence of MK6a has a primary effecton the migration speed of the follicular keratinocytes, our datapoint to a role for MK6a induction in the activation of thesecells afterwounding.

	ACKNOWLEDGMENTS

This work was supported by NIH grantHD25479.

We thank R. Porter and E. Lane for providing the MK16 antibody, A. Bradley for supplying the ES and SNL76/7 cells as wellas the hprt $Delta$ 3'-neo vector, and P. Koch and J. Rothnagel for criticalreading of themanuscript.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Molecular and Cellular Biology, Baylor College of Medicine, One BaylorPlaza, Houston, TX 77030. Phone: (713) 798-4966. Fax: (713) 798-3800.E-mail: roopd{at}bcm.tmc.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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1.	Albers, K., and E. Fuchs. 1992. The molecular biology of intermediate filament proteins. Int. Rev. Cytol. 134:243-279[Medline].
2.	Baribault, H., J. Penner, R. V. Iozzo, and M. Wilson-Heiner. 1994. Colorectal hyperplasia and inflammation in keratin 8-deficient FVB/N mice. Genes Dev. 8:2964-2973[Abstract/Free Full Text].
3.	Baribault, H., J. Price, K. Miyai, and R. G. Oshima. 1993. Mid-gestational lethality in mice lacking keratin 8. Genes Dev. 7:1191-1202[Abstract/Free Full Text].
4.	Bickenbach, J. R., M. A. Longley, D. S. Bundman, A. M. Dominey, P. E. Bowden, J. A. Rothnagel, and D. R. Roop. 1996. A transgenic mouse model that recapitulates the clinical features of both neonatal and adult forms of the skin disease epidermolytic hyperkeratosis. Differentiation 61:129-139[CrossRef][Medline].
5.	Blessing, M., H. Zentgraf, and J. L. Jorcano. 1987. Differentially expressed bovine cytokeratin genes. Analysis of gene linkage and evolutionary conservation of 5'-upstream sequences. EMBO J. 6:567-575[Medline].
6.	Chan, T. A., H. Hermeking, C. Lengauer, K. W. Kinzler, and B. Vogelstein. 1999. 14-3-3 sigma is required to prevent mitotic catastrophe after DNA damage. Nature 401:616-620[CrossRef][Medline].
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