Procurement of Human Skin

Young and aged volunteers were grouped according to age: 21 to 30 years for the young group and 80+ years for the aged group. Full-thickness human skin biopsies were obtained from sun-protected buttock skin of each subject by punch biopsy, as previously described.44,45 All procedures involving human patients were conducted in accordance with the regulations set forth by the University of Michigan Institutional Review Board, and all patients provided written informed consent.

Human Skin Organ Culture

Organ culture of human skin has been previously described.46,47,48 Briefly, replicate 2-mm punch biopsies were obtained from hip skin of volunteers 21 to 30 years of age. Skin samples were incubated in wells of a 24-well dish (one tissue piece per 500 μl of culture medium). Culture medium consisted of keratinocyte basal medium (Lonza, Walkersville, MD), supplemented with CaCl₂ to a final concentration of 1.4 mmol/L. Skin samples were either treated with vehicle or purified, activated human MMP-1 (150 ng/ml), for 24 hours. At the end of the incubation period, organ culture-conditioned medium was collected and analyzed for the presence of collagen fragments by sodium dodecyl sulfate-polyacrylamide gel electrophoresis. Intact collagen and collagen that had been exposed to MMP-1 in vitro served as controls. At the end of the incubation period, tissue was fixed in 10% buffered formalin and processed for light microscopy. Additional tissue pieces were fixed in 2% glutaraldehyde and processed for scanning electron microscopy.

Three-Dimensional Collagen Lattice Fibroblast Cell Culture

Adult human dermal fibroblasts were isolated from 4-mm full-thickness punch biopsies of healthy patients, as previously described.49 Collagen lattices were prepared in a sterile tube, by mixing appropriate volume of rat tail type I collagen (BD Biosciences) to yield a final concentration of 1 mg/ml with medium cocktail [DMEM, NaHCO₃ (44 mmol/L), l-glutamine (4 mmol/L), folic acid (9 mmol/L), and neutralized with 1 N NaOH to pH 7.2]. Collagen solution (0.5 ml per well of a 24-well plate) was placed in an incubator at 37°C for 30 minutes to allow polymerization of the collagen. Partially degraded collagen lattices were prepared by treatment with purified human MMP-1 (50 ng per well, Calbiochem) for 16 hours at 37°C. Before use full length MMP-1 was activated by trypsin treatment (1.25 ng per 100 ng MMP-1) for 1 hour at 37°C. Cleavage by trypsin converted full-length 52-kDa MMP-1 to a catalytically active 42-kDa form (see Supplemental Figure 1A at http://ajp.amjpathol.org). Trypsin activity was inhibited by addition of trypsin inhibitor (12.5 ng). Active MMP-1 released characteristic ¾ and ¼ length collagen fragments from the collagen lattices (see Supplemental Figure 1B at http://ajp.amjpathol.org). MMP-1 was inactivated by adding ethylenediaminetetraacetic acid (10 mmol/L) followed by addition of CaCl₂ (15 mmol/L), and gels were washed three times with fresh DMEM. Control lattices were prepared as above, without addition of MMP-1. Early passage (fewer than nine passages) primary adult human dermal fibroblasts (5 × 10⁴/well) were placed on top of each collagen lattice, and allowed to attach. After attachment, collagen lattices were covered with 1 ml of media (DMEM, 10% fetal bovine serum) and incubated 72 hours at 37°C, 5% CO₂. For analyses, collagen lattices were either embedded in OCT and frozen for cryostat sectioning, or fibroblasts were harvested by digesting collagen with 1 mg/ml of bacterial collagenase (Sigma Chemical Co.) for 1 hour at 37°C. Fibroblasts were collected by centrifugation. Recovery of viable fibroblasts averaged greater than 90%.

Laser Capture Microdissection (LCM) Coupled with Real-Time Reverse Transcriptase-Polymerase Chain Reaction (RT-PCR)

LCM were performed as previously described.45,49,50 Briefly, human skin punch biopsies were embedded in OCT, sectioned (10 μm), and stained with the HistoGene LCM slide preparation kit (Arcturus, Mountain View, CA). Approximately 200 dermal fibroblasts were captured using LCM (Leica ASLMD system; Leica Microsystems, Wetzlar, Germany). Total RNA was extracted from LCM-captured dermal fibroblasts using a commercial kit (RNeasy micro kit; Qiagen, Chatsworth, CA), and was used for amplification of mRNA using the RiboAmp HS RNA amplification kit (Acturus). The quality and quantity of amplified mRNA were determined with the Agilent 2100 bioanalyzer (Agilent Technologies, Santa Clara, CA). Typically, we were able to obtain 50 to 100 ng of amplified mRNA from LCM-captured 200 dermal fibroblasts (1 to 2 ng of total RNA). Only 5 ng of amplified mRNA is required for quantitative analysis of transcript levels by real-time RT-PCR. Therefore, we are able to quantify transcript levels of 10 to 20 different genes in one sample. We find that quantitation of transcript levels of several different genes in samples of total RNA and amplified mRNA yield essentially identical results. Quantitation of transcript levels were performed by real-time RT-PCR, as described previously.45,49,50 MMP-1, integrin α1, integrin α2, and integrin β1, PCR primers and probes were purchased from Applied Biosystems (Foster City, CA). Other PCR primers and probes including 36B4, an internal control, have been described previously.51

Immunofluorescence Staining

Immunohistology was performed as described previously.45,52 Briefly, OCT-embedded frozen tissue or three-dimensional collagen gels were sectioned, and the slides were fixed in 2% paraformaldehyde and permeabilized with for 0.5% Triton X-100 in phosphate-buffered saline (PBS) for 10 minutes at room temperature. The slides were blocked with appropriate serum (5% in PBS) for 1 hour at room temperature. Subsequently, the slides were incubated for 1 hour at room temperature with primary antibodies followed by incubation of appropriate secondary antibody for 1 hour at room temperature. After staining the slides were mounted with mounting media (Vector Laboratories, Burlingame, CA), and examined using a fluorescence microscope.

In Situ Zymography

In situ zymography was performed as previously described.29,53 Briefly, FITC-labeled calf skin type I collagen (50 μl, Elastin Products Co.) was coated onto glass slides. Cryostat skin sections (5 μm) were placed on top of the collagen coating, and incubated for 24 hours in a sealed, humidified chamber at 37°C. Sections were visualized by fluorescence microscopy. MMP-1-catalyzed degradation of FITC-collagen causes loss of fluorescence, which was visualized by fluorescent microscopy.

Western Analysis

Western blot was performed as previously described.45,51 Briefly, whole cell proteins were resolved on 10% sodium dodecyl sulfate-polyacrylamide gel electrophoresis, transferred to polyvinylidene difluoride membrane, and blocked with PBST (0.1% Tween 20 in PBS) containing 5% nonfat milk. Primary antibodies were incubated with polyvinylidene difluoride membrane for 1 hour at room temperature, and membranes were washed three times with PBST solution and incubated with appropriate secondary antibody for 1 hour at room temperature. After washing three times with PBST, the blots were developed with ECF (Vistra ECF Western blotting system, GE Health Care) following the manufacturer’s protocol. The Western bands were scanned with the STORM PhosphorImager (Molecular Dynamics, Sunnyvale, CA), and the intensities of each band were quantified by ImageQuant (GE Health Care), and normalized using β-actin as a marker for equal protein loading.

Measurement of ROS

Three-dimensional collagen lattice were cultured in DMEM containing 2,3,4,5,6-pentafluorodihydrotetramethylrosamine (1 mmol/L RedoxSensor Red CC-1, Molecular Probes), for 1 hour at 37°C, 5% CO₂. After incubation, samples were embedded in OCT and frozen. Oxidation of RedoxSensor Red CC-1, an indicator of levels of ROS,54 were visualized in cryostat sections (10 μm) by confocal fluorescence microscopy using an Olympus (Tokyo, Japan) FluoView 500 laser-scanning confocal microscope, housed in the Morphology and Image Analysis Core, University of Michigan Diabetes Research and Training Center. Image analysis was performed using ImageJ software (National Institutes of Health, Bethesda, MD).

Activator Protein (AP-1) Activity Assay

AP-1 transcription activity was determined using TransAM AP-1 transcription factor assay kit (Active Motif) according to the manufacturer’s protocols. Briefly, the cells were harvested by digesting collagen gel with bacterial collagenase (Sigma), as described above. The nuclear extract was prepared using nuclear and cytoplasmic extraction reagents (NE-PER; Pierce, Rockford, IL), and c-Jun-dependent AP-1 transcriptional activation was determined by phospho-c-Jun antibody (New England Biolabs, Beverly, MA).

Collagen-Degrading MMP-1 Is Elevated in the Dermis of Aged Human Skin in Vivo

In human skin, degradation of mature collagen fibrils can be initiated by interstitial collagenase (MMP-1). Oxidative stress, shown above to be increased in aged dermis, has been shown to increase MMP-1 expression in cultured cell models. Therefore, we dissected dermis from whole skin and measured MMP-1 mRNA levels. As shown in Figure 2A, MMP-1 mRNA was increased eightfold in aged, compared with young dermis. Consistent with these data, MMP-1 protein levels, detected by immunofluorescence, were significantly elevated in aged, compared with young human dermis (Figure 2B). Increased MMP-1 expression in aged human skin was predominantly localized to fibroblasts in the upper dermis, where fibroblasts display increased levels of oxidants. Quantitation of immunostaining indicated twofold increase in MMP-1 protein in aged, compared with young dermis (Figure 2B). In addition, aged skin exhibited higher levels of collagenase activity as revealed by in situ zymography. This elevated activity, revealed as darkened areas resulting from hydrolysis of FITC-labeled collagen, was localized to the upper dermis, consistent with localization of MMP-1 protein (Figure 2C).

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Figure 2

MMP-1 mRNA, protein, and activity are increased in the dermis of aged human skin in vivo. A: MMP-1 mRNA levels in dermal fibroblasts in young (21 to 30 years old) and aged (>80 years old) human skin. Fibroblasts (150 cells) were obtained by LCM, total RNA was isolated, mRNA was amplified, and MMP-1 mRNA was quantified in 5 ng of amplified mRNA by real-time RT-PCR. Results are means ± SEM of MMP-1 mRNA normalized to 36B4 (housekeeping gene internal control) mRNA. n = 6, *P < 0.01. B: Quantitation of MMP-1 protein immunostaining in young and aged human skin. Figures show representative immunostaining. White line indicates dermal-epidermal boundary. n = 4, *P < 0.02. C: MMP-1 activity in young and aged human skin in vivo. MMP-1 activity was detected by in situ zymography, using FITC-labeled type I collagen as substrate (green fluorescence). MMP-1-catalyzed collagen cleavage causes loss of green fluorescence, resulting in darkened areas, which are most noticeable in the upper dermis of aged skin. Images are representative of three experiments.

Tissue Inhibitors of Matrix Metalloproteinases (TIMPs) Are Not Elevated in Aged Human Skin in Vivo

TIMPs are a family of proteins that bind directly to MMPs and inhibit their catalytic activity. MMPs and TIMPs are often coordinately regulated as a means to control excess MMP activity.55 We used LCM to obtain epidermis and dermis from skin of aged and young individuals. The upper half of the dermis, corresponding to the region where increased MMP-1 expression was observed (Figure 2), was captured for analyses. TIMP-1, -2, -3, and -4 mRNA levels in epidermis or dermis were not significantly different between young and aged skin (see supplemental Figure 2A at http://ajp.amjpathol.org). In both young and aged skin, transcripts for all four TIMPs were lower in epidermis than in dermis. TIMP-1, -2, -3, and -4 protein levels in whole dermis did not differ between young and aged skin (see supplemental Figure 2B at http://ajp.amjpathol.org).

c-Jun, a Major Regulator of MMP-1 Expression, Is Elevated in the Dermis of Aged Human Skin in Vivo

MMP-1 expression is primarily mediated by transcriptional regulation. Transcription factor AP-1, typically composed of c-Jun and c-Fos, is a major transcriptional regulator of MMP-1 expression. We have previously reported that in human skin in vivo, AP-1 activity is limited by the level of c-Jun, which can be induced, whereas c-Fos is constitutively expressed.56 c-Jun mRNA was increased 2.4-fold in aged (>80 years old) dermis, compared with young (21 to 30 years old) (Figure 3A). c-Fos mRNA expression was similar in the aged and young dermis (data not shown). In addition, c-Jun protein was elevated fivefold in the of aged (>80 years old) dermis, compared with young (21 to 30 years old) (Figure 3B). These data suggest that increased expression of c-Jun may contribute to increased levels of MMP-1 observed in aged human dermis in vivo.

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Figure 3

c-Jun mRNA and protein are elevated in aged human dermis in vivo. A: c-Jun mRNA levels in young (21 to 30 years old) and aged (>80 years old) human dermis were analyzed by real-time RT-PCR. Results are means ± SEM of c-Jun mRNA normalized to 36B4 (internal control) mRNA. n = 6, *P < 0.0001. B: c-Jun protein levels in young and aged human dermis was quantified by Western analysis. Inset shows representative immunoblot. Results are means ± SEM. n = 6, *P < 0.05.

α2β1 Integrin Is Elevated in the Dermis of Aged Human Skin in Vivo

Integrins are the major cell surface receptors for extracellular matrix. Activation of α2β1 integrin activates a signal transduction cascade that results in increased expression of c-Jun and MMP-1. This MMP-1 induction via α2β1 integrin is thought to play an essential role in connective tissue remodeling and wound healing. Therefore, we examined α2 and β1 integrin expression in young and aged human dermis. α2 and β1 integrin mRNA levels were increased 2.9-fold and 9.8-fold, respectively, in aged (>80 years old) dermis, compared with young (21 to 30 years old) (Figure 4).

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Figure 4

α2 and β1 integrins are elevated in aged human dermis in vivo. α2 integrin (A) and β1 integrin (B) mRNA levels were determined in young (21 to 30 years old) and aged (>80 years old) human dermis by real-time RT-PCR. Results are means ± SEM of integrin α2 and β1 mRNA normalized to 36B4 mRNA (internal control). n = 3 to 6, *P < 0.05.

Exposure of Normal Human Skin to MMP-1 ex Vivo Generates Collagen Fragmentation that Resembles Aged Human Skin

To directly investigate the ability of MMP-1 to degrade human skin collagen, sun-protected skin, from young individuals was exposed to purified human MMP-1 in organ culture. This treatment resulted in collagen fragmentation, as demonstrated by the release of characteristic three-quarter/one-quarter proteolytic fragments into the media (see supplemental Figure 3 at http://ajp.amjpathol.org). MMP-1 treatment caused alterations in the structure and organization of collagen fibrils, and fibroblast shape that were qualitatively similar to those observed in aged skin (Figure 5).6 These alterations included thinning and reduced density of collagen fibrils, and rounding of fibroblasts in areas of decreased collagen density, in comparison with the stretched morphology of fibroblasts in nontreated young skin. Scanning electron microscopy revealed fragmentation of collagen fibrils in MMP-1-treated young skin similar to that seen in aged human skin (Figure 5).

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Figure 5

MMP-1 treatment of young human skin in organ culture causes collagen fragmentation similar to that observed in aged human skin in vivo. Samples of young skin were treated with vehicle (left, top and bottom) or MMP-1 (middle, top and bottom). Top panels display paraffin-embedded sections stained with H&E. MMP-1 treatment causes fibroblasts (circled in white) to appear less stretched and more rounded. Bottom panels display scanning electron micrographs of dermal collagen, showing fragmentation of collagen fibrils in MMP-1-treated versus vehicle-treated young skin. Alterations of fibroblast morphology and collagen fragmentation observed in young skin after MMP-1 treatment resemble those observed in aged human skin (right, top and bottom).

Three-Dimensional Cell Culture Model to Study Regulation of MMP-1

Data presented above provide a foundation for investigating molecular mechanisms that lead to MMP-1-mediated collagen fragmentation in aged human dermis in vivo. Although observations of human skin in vivo are invaluable for understanding the biology of aging, in vivo observations alone generally do not reveal cause and effect mechanistic relationships. The reason for this limitation is the obvious restrictions on the type of experimental manipulations that are possible in humans in vivo.

Therefore, we sought to establish a fibroblast culture model that exhibited similar phenotypic and molecular alterations observed in aged human skin in vivo. We found that fibroblasts cultured from young and aged individuals were primarily indistinguishable (see supplemental Figures 4 to 7 at http://ajp.amjpathol.org). Additionally, we have been unable to observe increased expression of senescence markers in human dermal fibroblasts in vivo. Therefore, we have used dermal fibroblasts cultured in intact or partially MMP-1-degraded three-dimensional collagen lattices to model young and aged, respectively, human dermis. This model has been shown to mimic the fragmented collagen matrix that is observed in aged human skin.6,33 For these studies, we used fibroblasts cultured from the skin of younger individuals. We found that the age of the donor from which fibroblasts were obtained did not significantly influence their behavior in either monolayer or three-dimensional intact collagen gel culture (see supplemental Figures 8 at http://ajp.amjpathol.org). In other words, changes in fibroblast morphology and function, described below, result from culture in partially fragmented collagen lattice, rather than fibroblast donor age.

Dermal Fibroblasts Cultured in Fragmented Collagen Lattices Are Smaller, Generate Increased Levels of Oxidants, and Have Increased Levels of Oxidized Proteins

A red fluorescent dye (Cell Tracker), which is taken up into the cell cytoplasm, was used to assess the morphology of fibroblasts in three-dimensional collagen lattices. Dermal fibroblasts cultured in intact collagen lattices displayed spread flattened appearance (Figure 6A, left). In contrast, fibroblasts in MMP-1-treated collagen gels, had reduced cytoplasmic area, and a contracted appearance (Figure 6A, right), similar to fibroblasts in aged human skin in vivo.6 These data are consistent with reduced mechanical tension in fibroblasts in a three-dimensional lattice that contains fragmented collagen.

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Figure 6

Dermal fibroblasts cultured in MMP-1-fragmented three-dimensional collagen lattices have reduced spreading and increased levels of oxidants. Human skin dermal fibroblasts were cultured in intact or MMP-1-fragmented collagen lattices. A: Fibroblast morphology was assessed by incubation of cultures with CellTracker fluorescent dye for 1 hour. Fibroblasts were imaged by confocal microscopy. Reddish fluorescence delineates cell cytoplasm; blue fluorescence delineates nuclei. Results are means ± SEM. n = 5, *P < 0.05. Images are representative of three experiments. B: Oxidant levels were assessed by incubation of cultures with RedoxSensor Red CC-1 for 1 hour. Cells were imaged by confocal microscopy. Reddish fluorescence indicates relative oxidant levels; blue fluorescence delineates nuclei. Relative red fluorescence levels were quantified by ImageJ (NIH). Results are means ± SEM. n = 3, *P < 0.05. Top panels show representative images. C: Cellular lysates were analyzed for protein oxidation (carbonyls) by Western blot. Immunoreactive oxidized proteins were visualized by chemifluorescence, and quantified by ImageQuant software. Results are means + SEM of signal intensity in the entire lane. n = 3, *P < 0.05.

As discussed above, cellular damage from ROS likely plays a key role in the aging process. We therefore examined the relative oxidant levels in fibroblasts cultured in intact and partially-degraded collagen gels, using the redox-sensitive fluorescent dye RedoxSensor Red CC-1. Fibroblasts in intact collagen lattices displayed a relatively low level of oxidant-generated fluorescence (Figure 6B, left). In contrast, fibroblasts in MMP-1-treated, partially degraded collagen lattices displayed intense oxidant-generated fluorescence (Figure 6B, right). The level of oxidant-generated fluorescence was threefold greater in fibroblasts cultured in partially degraded collagen lattices, than in intact collagen lattices (Figure 6B). Increased oxidative stress in fibroblasts cultured in partially degraded collagen was associated with significantly more oxidation of intracellular proteins, as measured by Western analyses of protein carbonyls (Figure 6C). Taken together, these data indicate that reduced mechanical tension, brought about by culture in partially degraded collagen, induces oxidative stress and causes increased protein oxidation in human dermal fibroblasts.

MMP-1 Is Elevated in Fibroblasts Cultured in Fragmented Collagen Lattices

As described above, the collagenous extracellular matrix in aged dermis is partially fragmented, and fibroblasts residing in this fragmented extracellular matrix have increased levels of endogenous oxidants and express higher levels of MMP-1. MMP-1 mRNA and protein were also significantly increased in fibroblasts cultured in partially degraded collagen lattices, compared with fibroblasts cultured in intact collagen lattices. MMP-1 mRNA was elevated eightfold (Figure 7A), and immunostaining revealed twofold increased intracellular MMP-1 protein (Figure 7B). Secreted MMP-1 protein, quantified by enzyme-linked immunosorbent assay, was elevated threefold (Figure 7C). Western analysis revealed that expression of both full-length pro-MMP-1 and cleaved active MMP-1 were increased in partially degraded collagen lattice cultures (Figure 7C).

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Figure 7

MMP-1 is elevated in dermal fibroblasts cultured in MMP-1-fragmented three-dimensional collagen lattices. Human dermal fibroblasts were cultured in intact or MMP-1-fragmented, collagen lattices. A: Total RNA was extracted and MMP-1 mRNA levels were determined by real-time RT-PCR. Results are means ± SEM of MMP-1 mRNA normalized to 36B4 (internal control) mRNA. n = 4, *P < 0.05. B: MMP-1 protein expression in fibroblasts was determined by laser confocal immunofluorescence microscopy, and quantified by image analysis. Top panels show representative images. Cell nuclei are stained blue, and MMP-1 protein is stained red. Results are means ± SEM. n = 3, *P < 0.05. C: Secreted MMP-1 protein was quantified by enzyme-linked immunosorbent assay. Inset shows representative Western blot demonstrating increased levels of both full-length MMP-1 and cleaved activated MMP-1 secreted by fibroblasts in fragmented collagen lattices. n = 4, *P < 0.05.

Key Regulators of MMP-1 Expression c-Jun/AP-1 and α2β1 Integrin Are Elevated in Fibroblasts Cultured in Fragmented Collagen Lattices

Transcription factors AP-1 and α2β1 integrin are major regulators of MMP-1 gene expression in human fibroblasts. As shown in Figure 8A, culture of fibroblasts in MMP-1-treated, partially degraded collagen-induced c-Jun protein expression twofold, compared with fibroblasts cultured in intact collagen lattices. Increased c-Jun was localized in the nucleus, and DNA binding of the phosphorylated, active form of c-Jun was increased 3.5-fold (Figure 8B). α2β1 integrin is the major cell surface extracellular matrix receptor that positively regulates expression of MMP-1. As shown in Figure 8C, α2 and β1 integrins mRNA were increased 2.8-fold and 1.7-fold, respectively, in dermal fibroblasts cultured in fragmented collagen lattices, compared with fibroblasts cultured in intact collagen lattices.

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Figure 8

c-Jun protein and DNA-binding are elevated in dermal fibroblasts cultured in MMP-1-fragmented three-dimensional collagen lattices. Human dermal fibroblasts were cultured in intact or MMP-1-fragmented lattices. A: c-Jun protein levels were determined by laser confocal immunofluorescence microscopy and quantified by image analysis. Top Panels show representative images. Cell nuclei are stained blue, and c-Jun protein is stained red. Results are means ± SEM. n = 3, *P < 0.05. B: Nuclear extracts were prepared and c-Jun DNA binding was determined using the TransAM AP-1 kit (Active Motif). Results are means ± SEM. n = 3, *P < 0.05. C: α2 and β1 integrins are elevated in dermal fibroblasts cultured in MMP-1-fragmented three-dimensional collagen lattices. Human dermal fibroblasts were cultured in intact and MMP-1-fragmented three-dimensional collagen lattices. Total RNA was extracted. α2 and β1 integrin mRNA levels were analyzed by real-time RT-PCR (10 ng total RNA). Results are mean ± SEM of α2 or β1 integrin mRNA normalized to 36B4 (internal control) mRNA. n = 3, *P < 0.03.

We thank Rui Wang for the technical contribution and Diane Fiolek and Laura Van Goor for graphic support.