Transcriptomic analysis of human skin wound healing and rejuvenation following ablative fractional laser treatment

Ablative fractional laser treatment is considered the gold standard for skin rejuvenation. In order to understand how fractional laser works to rejuvenate skin, we performed microarray profiling on skin biopsies to identify temporal and dose-response changes in gene expression following fractional laser treatment. The backs of 14 women were treated with ablative fractional laser (Fraxel®) and 4 mm punch biopsies were collected from an untreated site and at the treated sites 1, 3, 7, 14, 21 and 28 days after the single treatment. In addition, in order to understand the effect that multiple fractional laser treatments have on skin rejuvenation, several sites were treated sequentially with either 1, 2, 3, or 4 treatments (with 28 days between treatments) followed by the collection of 4 mm punch biopsies. RNA was extracted from the biopsies, analyzed using Affymetrix U219 chips and gene expression was compared between untreated and treated sites. We observed dramatic changes in gene expression as early as 1 day after fractional laser treatment with changes remaining elevated even after 1 month. Analysis of individual genes demonstrated significant and time related changes in inflammatory, epidermal, and dermal genes, with dermal genes linked to extracellular matrix formation changing at later time points following fractional laser treatment. When comparing the age-related changes in skin gene expression to those induced by fractional laser, it was observed that fractional laser treatment reverses many of the changes in the aging gene expression. Finally, multiple fractional laser treatments, which cover different regions of a treatment area, resulted in a sustained or increased dermal remodeling response, with many genes either differentially regulated or continuously upregulated, supporting previous observations that maximal skin rejuvenation requires multiple fractional laser treatments. In conclusion, fractional laser treatment of human skin activates a number of biological processes involved in wound healing and tissue regeneration.

Lasers have been used since the early 1980s to deliver skin rejuvenation benefits [22]. The first clinically used laser treatment was total ablative laser-based rejuvenation [22]. This treatment resulted in significant dermal remodeling and epidermal regeneration that improves both skin texture and tone; however, as a consequence of removal of most of the epidermis and significant amount of dermis, long healing times and significant side effect profiles were observed [23,24]. Nonablative laser rejuvenation procedures were subsequently developed, and while these approaches reduced the damage to the epidermis, they had limited rejuvenation efficacy [22]. Next, fractional ablative laser rejuvenation procedures were developed, using a grid pattern of separate individual micrometer laser shots to ablate only a fraction of the epidermis and dermis, resulting in dermal remodeling and improved texture and tone with much faster healing times and a significantly improved side effect profile [22][23][24][25]. Of these three approaches, ablative laser rejuvenation is considered the best treatment in terms of efficacy for the treatment of photoaging, acne scars and rhytides, although it is associated with serious side effects including long healing times, scarring and delayed onset hypopigmentation [22,25]. In contrast, because the laser does not injure the epidermis and just heats the dermis, non-ablative laser rejuvenation is very safe but not as effective as ablative lasers in skin rejuvenation [24,27]. Finally, fractional ablative laser rejuvenation combines both the safety of nonablative laser rejuvenation with the efficacy of ablative laser rejuvenation and has become the new gold standard for skin rejuvenation with long lasting rejuvenation effects in multiple ethnicities at multiple body sites [22][23][24][25][26][27][28][29][30].
Fractional laser skin rejuvenation works by creating microscopic thermal holes in a grid pattern through the epidermis and deep into the dermis, thus stimulating dermal and epidermal regeneration while leaving most (up to 95%) of the epidermis and dermis intact [31]. This allows the laser-induced damage to be more quickly repaired [25,[32][33][34]. To achieve maximum benefit, an average of at least four sessions are needed because with each treatment only a fraction (20-25%) of the treated area is covered [31]. The depth and width of the thermal damage and laser intensity can be altered to achieve maximal dermal rejuvenation, often with efficacy like ablative laser treatment, without lengthy re-epithelialization (2 days for fractional laser versus 2-3 weeks for ablative laser), fewer infections, fewer acneiform eruptions and greatly reduced erythema [25,31,35,36]. Significant work has been performed to understand how ablative, non-ablative and fractional lasers work to rejuvenate skin. Histopathological studies have demonstrated that fractional laser treatment of skin results in columnar ablative zones surrounded by thermal coagulation zones containing denatured proteins in the epidermis and dermis. Epidermal repair occurs within 1-3 days, the epidermal/dermal junction is repaired by 7 days while dermal repair takes weeks to months [31,32,33,37,38]. Finally, Fraxel laser resurfacing is FDA approved for use on all regions of the body and skin types [31]. Also observed was an increase in epidermal thickness, an increase in dermal collagens and a decrease in dermal elastin (elastosis) [39,40]. These observations have been confirmed using the non-invasive techniques of confocal microscopy and two-photon microscopy [26,41]. Histochemical studies looking at specific proteins demonstrated an increase in collagens (COL-1, COL-3), tropoelastin, vimentin, cytokines (EGF, bFGF, PDGF, VEGF, TGF-β, FGF9), heat shock proteins (HSP70, HSP47, HSP72), apoptosis markers (annexin-VII, Bcl-2, caspase-9), inflammatory cells (CD3+, CD20+, CD68+, CD31+), proteases (MMP1, MMP3, MMP9, neutrophil elastase) and a decrease in p53 [42][43][44][45][46][47][48]. Gene expression studies (typically using qPCR evaluating a limited number of genes) demonstrate an increase in proteases (MMP1, MMP2, MMP3, MMP9, MMP10, MMP11, MMP13), protease inhibitors (TIMP), hyaluronic acid synthesis enzymes (HAS, HYAL), collagens (COL1A1, COL3A1), extracellular matrix components (ELN, EMILIN1), cytokines (IL-1β, IL-8), and defensins (CAMP, HBD2) [23,[49][50][51][52]. Many of the observations of the effects of fractional laser treatment on human skin have been confirmed using animal and human skin organotypic models with the advantage that more detailed time courses and larger, more numerous sampling can be performed [33, [53][54][55][56][57][58][59][60][61][62][63]. These analyses have provided a more complete picture of fractional laser treatment; however, the human and/or in vivo relevance of these findings need to be confirmed by actual human studies. More recently, transcriptomic analyses have been performed using microarrays, gene chips and RNAseq approaches, and have identified several gene expression changes occurring following fractional laser treatment on human skin [54,64,65]. Because of the global nature of these approaches, many gene expression changes have been observed following fractional laser treatment, albeit the generation of a holistic understanding of how this treatment results in skin rejuvenation has been hampered by small and limited sampling. Thus, a study evaluating a larger base size of individuals over longer time periods, with frequent sampling using sensitive transcriptomics, is needed to better understand how fractional laser treatment rejuvenates skin. Here, we present our findings from a detailed time course transcriptomic analysis of in vivo fractional laser treated human skin with the goal of providing a holistic understanding of how fractional laser-induced wounding and healing rejuvenates aged human skin.

Study design
This study was approved by the Schulman Associates Institutional Review Board (IRB# 201203768). All subjects provided written informed consent prior to undergoing any study procedures and were compensated for their participation. Fourteen women in good general health, aged 30-55, with Fitzpatrick skin type I-IV, were enrolled in this study. Fractional laser treatments were performed using a Fraxel1 laser set to 12 mJ and 250 mtz with a 1 cm 2 treatment area, with all treatments and biopsy sampling performed by licensed medical personnel. For this study, the 14 study participants were treated on the back at 9 different equally spaced sites between the neck, upper buttocks and the left/right edges of the back with a minimum distance of 5 cm between each treatment site (plus one untreated site), and all sites received a 1 mm tattoo for site recognition. The treatment sites were also randomized to account for any potential variability between the lateral, superior or inferior portions of the back. The timing of the treatments was designed such that all biopsies were collected by a licensed dermatologist on the last day of the study. Sixty minutes prior to Fraxel1 laser treatment, the treatment site was dosed with a topical anesthetic (BLT Cream: 20% benzocaine, 6% lidocaine, 4% tetracaine) after which the hand-held Fraxel1 laser was moved over the treatment site 8 times. The treatment groups were as follows: (1) single laser treatments at 1, 3, 7, 14, 21 and 28 days before biopsy and (2) multiple laser treatments at 28-day intervals with 1, 2, 3, and 4 treatments. Following the final treatment, a 4 mm full thickness biopsy was collected at each site by a licensed dermatologist (including a non-treated site), the biopsy site was sutured for closure and good healing, and the biopsy sample was placed in a cryotube and flash frozen in liquid nitrogen. A total of 140 biopsy samples were generated for analysis. The study participants returned to the test site 7-10 days following biopsy to have their biopsy sites assessed by a Physician's Assistant and to have sutures removed. Following completion of the healing assessment, the study was considered completed. No subject had issues with healing of their biopsy sites and no study related adverse events were reported. Study design, cohort description, and sample collection for the aged dermis study has been previously described [8].

Microarray profiling
Microarray profiling was performed on 140 untreated or laser-treated samples using the HG-U219 array (Affymetrix) as similarly described for the aged dermis samples [8]. Flash-frozen, bisected 4 mm full-thickness skin punch biopsies were homogenized in TRIzol reagent (ThermoFisher, Waltham, MA) and total RNA was extracted according to the manufacturer's protocol. RNA was further purified using RNEasy spin columns (QIAGEN, Hilden, Germany). Biotinylated cRNA libraries were synthesized from 500 ng of total RNA using the Affymetrix HT 3' IVT Express kit (Affymetrix, Santa Clara, CA) and the Beckman Biomek FXp Laboratory Automation Workstation (Beckman Coulter, Brea, CA). Biotinylated cRNA was subsequently fragmented by limited alkaline hydrolysis and then hybridized overnight to the Affymetrix Human Genome U219-96 GeneTitan array. Plates were scanned using the Affymetrix GeneTitan Instrument utilizing AGCC GeneTitan Instrument Control software version 4.2.0.1566. Image data was summarized using Affymetrix PLIER algorithm with quantile normalization. Microarray data from this study as well as the aged dermis study have been deposited in the Gene Expression Omnibus (GEO) under GSE168760 and GSE139300, respectively.

Statistical analyses
After rigorous quality check using methods and metrics described by Canales, et al [66], a linear mixed ANOVA model was fitted to the microarray data using SAS software PROC GLIM-MIX, version 9.4 of the SAS System for Windows. Gene expression (in log scale) of each single treatment site was compared to that of the baseline (day 0) untreated site, and each of the multiple treatment sites was compared to the single treatment site at day 28. Subject, Affymetrix plate (samples from 14 subjects were processed on two plates with seven subjects per plate) and Site were class variables. Subject (nested within Plate) was the random effect in the model. No multiple comparison adjustment was used due to the exploratory nature of the study.

Bioinformatic analyses
Gene signature analyses were performed using GeneSpring version 14.8 (Agilent Technologies, Santa Clara, CA). In brief, low-expressed probe sets were removed based on establishing a minimum expression threshold (>20th percentile across all samples within any one treatment group) and condensed to a single Entrez gene ID using the arithmetic mean. Log 2 fold changes were calculated for the single treatment sites relative to untreated sites (Day 0) or, for the multiple treatment sites, relative to the single treatment site (Day 28). Hierarchical clustering of the log 2 fold change values using Euclidean distance was performed to create the single treatment and multiple treatment dendrograms. Biological pathway enrichment was performed on the filtered single treatment signatures (p < 0.01, absolute fold change > 1.1) and multiple treatment signatures (p < 0.05) using Ingenuity Pathway Analysis version 01-07 (QIAGEN). Fisher's exact t test was used to assess significantly associated pathways, and zscores were calculated to predict pathway activation states (activated pathways, z-score >0; inhibited pathways z-score <0).

Results
In order to understand how fractional laser treatment works to rejuvenate human skin, an Affymetrix gene chip based transcriptomic analysis was performed on human skin biopsies from fractional laser treated skin at various time points after a single and multiple treatments. The experimental design was two-fold: (1) to understand the biological process that occurs during healing following one fractional laser treatment, 6 different sites on the backs of 14 individuals were treated with a single fractional laser treatment followed by biopsy sampling of those sites at 1, 3, 7, 14, 21 and 28 days after treatment; and (2) to understand if multiple treatments sustain the transcriptional response, 3 different sites on the backs of the same 14 individuals received either 2, 3 or 4 fractional laser treatments at the same site (with the treatments 28 days apart) followed by biopsy sampling. All the single treatments were compared to an untreated biopsy sample, allowing the use of the same individual as their own control (see Materials and Methods for a detailed description). For single treatment sites, the number of differentially expressed probe sets was highest 1 day after treatment and continued to drop throughout the 28-day treatment period (Table 1). Interestingly, multiple treatments of the same site, spaced 28 days apart, showed an increase in differential gene expression when compared to a single treatment after 28 days (Table 1). Investigating the nature of the gene expression changes with time after fractional laser treatment demonstrated both increases and decreases in gene expression with a gradual normalization over time ( Fig 1A). Clustering analysis showed several interesting patterns including a sharp increase in gene expression at 1 day post treatment followed by a sharp decline between 3-7 days post treatment-this cluster contains a number of keratin genes, S100 family alarmin genes and metalloproteinase genesindicative of early epidermal and dermal wound healing responses. Also observed was a sharp decrease in gene expression at 1 day post treatment followed by an increase in expression 3 days post treatment and normalization to background levels by 7 days post treatment of a wide variety of genes. Finally, a sharp decrease in gene expression at 1 day post treatment was observed followed by a gradual increase in expression over the 28 day treatment period-this cluster contains a number of dermal extracellular matrix genes (Fig 1B-1D).

Skin wound healing involves inflammatory, epidermal and dermal processes
A bioinformatic analysis of the top differentially regulated genes demonstrated a collection of activated inflammation related pathways was differentially regulated as early as 1 day after fractional laser treatment with most inflammatory processes normalized by 14 days post treatment ( Table 2). Epidermal related biological pathways involving proliferation and migration were similarly activated 1 day after treatment with many of the processes normalized by 7 days post treatment (Table 3). Interestingly, in addition to proliferation and movement of epidermal cells, an epidermal-mesenchymal transition pathway was activated 3 to 7 days post treatment (Table 3), which returned to baseline levels by day 14. This suggests the epidermis as a potential source for the mesenchymal cells participating in tissue repair at this early stage. Evaluation of dermal related biological pathways were complex with some processes initiating 1 day after fractional laser treatment such as proliferation and differentiation of connective tissue cells while other processes beginning much later such as the formation and maturation of collagen fibrils (Table 4). An analysis of the top 20 molecular functions 28 days post treatment supports the observations that cell death and removal, cell proliferation/movement and extracellular matrix maturation are the key processes during the wound healing process (Table 5). A more granular display of the top 20 molecular functions over time and with multiple treatments is shown in S1-S9 Tables. An evaluation of the canonical signaling pathways associated with fractional laser treatment demonstrated that apoptosis/proliferation, stress/inflammation and cell adhesion were the key pathway groupings activated (Table 6). In these 3 key pathway groupings, individual pathways demonstrated unique kinetics with peak activation of some pathways such as remodeling of epithelial adherens junctions, ephrin receptor signaling, cell cycle control, and inflammation (IL-6 and IL-8 signaling) occurring at early time points (days 1-7). Other pathways including activated interferon signaling and negative inhibition of MMP signaling remained elevated throughout the time points. Finally, the HOTAIR regulatory pathway remained active the entire 28 days of observation (Table 6 and Fig 2).
Fractional laser treatment is very effective in reversing skin aging changes. Thus, the transcriptional changes induced by fractional laser resurfacing were compared with the gene expression changes that occur during facial epidermis and dermis aging. The overlap of genes in common between the fractional laser treatment differentially expressed genes at 28 days post treatment and the differentially regulated genes in 50 versus 20-year-old epidermis (Fig Table 2. Stress and immune response biological pathways associated with laser resurfacing kinetics.

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Transcriptomic analysis of human skin wound healing and rejuvenation following fractional laser treatment 3A and 3B) and the 50 versus 20-year-old dermis were compared (Fig 3C and 3D). A large number of genes in common was observed with several genes being expressed in opposite directions in the fractional laser samples compared to the 50 versus 20-year-old epidermis and dermis samples (Fig 2B and 2D). A closer analysis revealed several extracellular matrix-related genes; in particular, collagen genes were the most highly upregulated with fractional laser treatment at day 28 yet showed the greatest decrease in expression in aged versus young skin (Figs 3B, 3D, 4A and 4B). Notably, many of the genes shared across multiple pathways displayed an increasing expression pattern over time following fractional laser treatment while their expression was decreased in 50-year-old individuals (Fig 4C). This indicates one of the major effects of fractional laser treatment is the reversal of the loss of extracellular matrix with skin aging. Finally, based on the clinical observation that multiple fractional laser treatments result in the best skin rejuvenation outcome, the gene expression changes that occur following 2, 3 or 4 sequential fractional laser treatments were examined (Fig 5). When compared to a single fractional laser treatment, increased numbers of differential gene expression changes were observed following 2 treatments (Fig 5A), many of which were maintained following 3 and 4 treatments and some which were only observed following 3 treatments (Fig 5B and 5C). An evaluation of two specific genes illustrated that multiple treatments are required for maximal effect for COL1A1 expression (Fig 5D) and NR4A1 (Fig 5E), albeit with different trajectories.

Discussion
In this report, temporal transcriptomic analysis has been utilized to better understand how fractional laser treatment functions to rejuvenate aged skin. This temporal analysis was conducted on back skin because it allowed for the extensive investigative transcriptional analysis

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Transcriptomic analysis of human skin wound healing and rejuvenation following fractional laser treatment into the mechanism of Fraxel-induced skin rejuvenation. Because Fraxel laser resurfacing has been successfully performed on multiple skin sites, such as face, lips, neck, and hands [22,25,28], it is believed that the treatment of back skin is still relevant for yielding meaningful mechanistic insights. In addition, no long-term clinical measures of skin rejuvenation were measured in this study, given the large amount of published evidence (22-30) that supports the diverse skin benefits obtained from Fraxel laser resurfacing. Thus, this study focused on the transcriptional response of the skin to Fraxel treatment and demonstrated that fractional laser treatment induces many biological processes related to wound healing and tissue regeneration, in a highly orchestrated manner, resulting in rejuvenation of long-lived skin macromolecules like components of the extracellular matrix. These data greatly expand the previously published temporal analysis of the effects of laser treatment on skin by providing a much more detailed analysis of the changes in gene expression that occur (whole genome) compared to the approximately 20 genes previously analyzed [23,[49][50][51][52]. In addition, this study greatly extends previous transcriptomic analyses by including more sampling times, larger number of study participants and increased number of laser treatments [54,64,65].
As part of the wound healing process following fractional laser-induced treatment, immediate gene expression changes were observed indicative of epidermal and dermal repair mediated by keratinocytes, fibroblasts and immune cells which were followed by longer term repair of the dermis mediated by fibroblasts and immune cells. Activation of keratinocytes as early as 1 day post fractional laser treatment is exemplified by the large changes in keratin gene expression and the activation of epithelial cell pathways (necrosis of epithelial tissues, proliferation and cell movement of epithelial cells) and is consistent with current knowledge concerning the speed of epidermal repair following fractional laser treatment [32,33,37,38]. Two pathways important in the re-epithelization of a wound (ephrin receptor signaling pathway and HOTAIR regulatory pathway) were analyzed in more detail. The ephrin receptor signaling pathway, which is important in wound closure and healing [67], is strongly activated as early as 1 day post treatment followed by a gradual decrease over the 28-day treatment period. The long non-coding RNA HOTAIR regulatory pathway was also activated following fractional laser treatment as would be required for proper wound healing [68]. Additionally, the large changes in S100 gene expression at 1 day post fractional laser treatment, along with the rapid induction of gene expression of several inflammatory pathways, confirms a quick immune response to the damage and greatly expands previous histochemical study findings [42][43][44][45][46][47][48]. Interestingly, other immune-related pathways showed prolonged (e.g., antimicrobial response) or even bi-phasic (e.g., activation of leukocytes) waves of activation over the course of 28 days post-laser resurfacing treatment. These observations are consistent with the published reports demonstrating unique roles of both innate and adaptive immune cells during distinct phases of the wound healing response in skin. For instance, in mouse models of acute wound healing, macrophages have been shown to have critical roles in the early and midphase inflammation and tissue repair responses, respectively, but are dispensable for tissue maturation in the late phase [69]. Conversely, γδ T cells within the epidermis display pleiotropic functions and maintain close, continuous interaction with keratinocytes to provide an immediate response to cellular damage as well as on-going surveillance for damage [70].

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Additional studies are needed to tease apart the precise components of the immune system that are involved in the resolution and repair of epidermal and dermal wound healing following laser resurfacing treatment.
In the dermis, fibroblast mediated gene expression changes occurred immediately after treatment and continued throughout the four-month observation period. An interesting observation was the early (1 day after treatment) coordinated decrease in gene expression of fibroblast cell death and fibrogenesis pathways with an increase in gene expression of connective tissue growth, proliferation of connective tissue and cell movement of connective tissue pathways. These results indicate a complex fibroblast response to damage which appears to be focused on increasing fibroblast numbers and movement to damaged dermal areas. In contrast, later in the dermal wound healing process we observed an increase in the formation of collagen fibrils, tensile strength of skin, and attachment of cells pathways, all of which indicate a maturation of the wound healing response by synthesis and maturation of the extracellular matrix. Interestingly, negative inhibition of MMP signaling and MMP expression levels also remained elevated throughout the time points The observation that MMPs are induced with fractional laser treatment is consistent with previous studies demonstrating MMP expression upon injury in a variety of cell types, including mesenchymal, epithelial and immune cells [71]. It is furthermore well established that MMPs are necessary for normal regulation and remodeling of the ECM, and that MMP activity is tightly regulated at multiple levels, beyond regulation of transcription [71]. The observation that the later dermal gene expression changes following fractional laser treatment are associated with activated tensile strength of skin, in particular, supports a direct relationship between the molecular changes induced by fractional laser treatment and the biomechanical properties of the skin. Activation of this pathway 28 days after treatment is consistent with the delayed onset of the skin appearance benefits following fractional laser treatment, and further supports that the late-stage dermal remodeling processes are crucial to the ultimate cosmetic benefits delivered by this gold standard anti-aging procedure. Together, the temporal analysis of gene expression changes following fractional laser wounding demonstrate a complex, yet orderly, repair process and provides significant insight into which biological processes are required for skin repair and rejuvenation.
Given that each treatment covers only a fraction (20-25%) of the treatment area [31], the effects of multiple fractional laser treatments on the transcriptional response in the epidermis and dermis were evaluated. The results showed that an overall strong wound healing response is maintained or increased after multiple laser treatments, which is best exemplified by the increase in COL1A1 and other extracellular matrix genes, with at least 2-3 treatments needed for maximal increase in gene expression and this drives remodeling of the extracellular matrix. An evaluation of NR4A1, a nuclear receptor that functions as a transcriptional repressor of TGF-β targeted genes whose expression is decreased during wound healing [72], demonstrated at least 3 fractional laser treatments were required before NR4A1 levels increased to pretreatment levels. These observations fit well with the clinical experience in which maximal skin rejuvenation is observed following multiple fractional laser treatments [73].
Multiple cosmetic procedures work to rejuvenate skin by activating the wound repair process (e.g., Fraxel1 Thermage1, Ultherapy1); however, fractional laser is considered the gold standard treatment for aging related skin rejuvenation. The analysis of the gene expression changes observed following fractional laser treatment identified many biological and molecular pathways that are activated following treatment. These pathways were compared to the biological pathways that are modulated during skin aging using our previously described aging transcriptomics dataset [8], in order to better understand how this treatment works for skin rejuvenation. A large number of genes in common between fractional laser treatment and aging of both the epidermis and dermis of human skin were observed, with treatment leading to reversal of many aging associated gene expression changes. These findings are notable given the differences in body site sampled (back vs. face), tissue matrices (full-thickness biopsies vs. separated tissue) and individual variability, suggesting that fractional laser treatment acts holistically across both epidermal and in dermal compartments to restore a more youthful skin structure. Many of the key biological processes affected by fractional laser treatment that are instrumental in skin rejuvenation are the processes involved in the regeneration of the dermal extracellular matrix. Reversal of the age associated loss of extracellular matrix gene expression (most notably collagen genes) was observed along with changes in gene expression indicative of significant remodeling of the extracellular matrix. These observations demonstrate that approaches to rejuvenate aged skin should ideally provide these two functions. Interestingly, several material-based approaches that achieve similar increases in extracellular matrix production to rejuvenate skin include peptides (such as matrikines) and combinations of peptides [74][75][76] and retinoids [77,78]. Together these observations provide evidence that maximal skin rejuvenation requires a multi-faceted approach addressing both epidermal and dermal aging, with a key driver being the modulation of the long-lived dermal extracellular matrix. The transcriptome-wide effects of fractional laser induced skin repair and rejuvenation, analyzed in the present study with both a high degree of temporal precision and across multiple treatments, provides many new potential intervention targets to improve the structure, function and appearance of aging skin.