Figures
Abstract
Molecular mechanisms leading to pressure ulcer development are scarce in spite of high mortality of patients. Development of pressure ulcers that is initially observed as deep tissue injury is multifactorial. We postulate that biomechanical forces and inflammasome activation, together with ischemia and aging, may play a role in pressure ulcer development. To test this we used a newly-developed bio-mechanical model in which ischemic young and aged human skin was subjected to a constant physiological compressive stress (load) of 300 kPa (determined by pressure plate analyses of a person in a reclining position) for 0.5–4 hours. Collagen orientation was assessed using polarized light, whereas inflammasome proteins were quantified by immunoblotting. Loaded skin showed marked changes in morphology and NLRP3 inflammasome protein expression. Sub-epidermal separations and altered orientation of collagen fibers were observed in aged skin at earlier time points. Aged skin showed significant decreases in the levels of NLRP3 inflammasome proteins. Loading did not alter NLRP3 inflammasome proteins expression in aged skin, whereas it significantly increased their levels in young skin. We conclude that aging contributes to rapid morphological changes and decrease in inflammasome proteins in response to tissue damage, suggesting that a decline in the innate inflammatory response in elderly skin could contribute to pressure ulcer pathogenesis. Observed morphological changes suggest that tissue damage upon loading may not be entirely preventable. Furthermore, newly developed model described here may be very useful in understanding the mechanisms of deep tissue injury that may lead towards development of pressure ulcers.
Citation: Stojadinovic O, Minkiewicz J, Sawaya A, Bourne JW, Torzilli P, de Rivero Vaccari JP, et al. (2013) Deep Tissue Injury in Development of Pressure Ulcers: A Decrease of Inflammasome Activation and Changes in Human Skin Morphology in Response to Aging and Mechanical Load. PLoS ONE 8(8): e69223. https://doi.org/10.1371/journal.pone.0069223
Editor: Christophe Egles, Université de Technologie de Compiègne, France
Received: March 19, 2013; Accepted: June 5, 2013; Published: August 14, 2013
Copyright: © 2013 Stojadinovic et al. This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
Funding: This work was supported by funds from National Institutes of Health AG030673, DK086364, AR060562(MT-C), NS059836 (RWK),TL1RR024998 (JWB) from the Weill-Cornell Clinical and Translational Science Center. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.
Competing interests: The authors have declared that no competing interests exist.
Introduction
Pressure ulcers (PU), defined as breaks in the integument caused by continuous pressure of the body weight to skin have been implicated as one of the most frequent causes of death in elderly, wheelchair and bed–bound individuals. As many chronic wound types, PU is multifactorial disease. Multiple physical factors lead to the development of PU including: static pressure or stress, shearing forces, friction, and moisture, but these alone are insufficient to produce tissue damage resulting in a PU. However, if these factors are combined with host-specific factors such as immobility, aging, neurologic disease, incontinence and malnutrition, a PU may form.
Prolonged load/pressure in conjunction with tissue ischemia is believed to play a major role in PU development. A PU can develop in as little as 2 hours of immobility [1], [2]. Initial changes, observed as deep tissue injury (DTI), can develop in patients even during prolonged surgeries [1], [3]. The National Pressure Ulcer Advisory Panel reports wide ranges of prevalence among patients in the United States estimated to be 1.3 to 3 million [4]. Approximately 2.5 million PU require treatment annually, representing the second most frequent cause for hospital readmissions [5], with estimated costs of hospital-acquired PU at $2.2 – $3.6 billion [6]. Federal Government issued guidelines for hospitals and care-takers for risk assessment, documentation and prevention because PUs are the source of numerous complications and often result in multiple hospitalizations [7]. Due to limited knowledge regarding the molecular pathogenesis of these ulcers there is no treatment currently approved by FDA as efficacious.
The challenge in studying the development of PU results from lack of adequate experimental models that accurately resemble human disease. Current knowledge originates mostly from analyses of human tissue, wound fluid and a few animal models. Reports from studies showed elevated levels of IL1, TNF, MMP's and defensins in PU [8]–[15]. Animal studies suggest synergistic effects of age and ischemia as contributing factors [16]. Study conducted to assess the effect of prolong mechanical load using bioengineered skin showed involvement of pro-inflammatory mediators [17], [18].
Keratinocytes participate in innate immune signaling and are the first responders to the danger signals by secreting pro-inflammatory cytokines, namely interleukin-1β (IL1-β) [19], [20]. The inflammasome, a cytosolic, multiprotein platform that activates pro-inflammatory caspases and IL-1β is expressed in human keratinocytes both in vitro [21] and in vivo [22], [23]. It is activated by diverse molecular patterns released from stressed and damaged cells [24]–[26].
Here, we report development of a novel experimental pressure model utilizing a Mechanical Explant Test System (METS) [27], [28] to assess the effect of load and ischemia on human skin explants of different age. To the best of our knowledge, this report is the first experimental approach aiming to determine specific changes that occur in human skin due to static pressure in conjunction with ischemia. We found that the morphology of skin differed among young and aged individuals in response to load. We observed subepidermal separation and a change in collagen alignment in aged skin in response to load. We also report that young skin has significantly higher levels of inflammasome proteins than aged skin. Loading young skin resulted in a rapid increase in inflammasome proteins levels that was maintained for 4 hours. In contrast, no significant alteration in inflammasome protein expression was found in loaded aged skin. Taken together, our findings support the idea that the effects of aging and load synergize to contribute to morphological changes that lead to development of DTI and further to PU. Not only morphological changes occurred more rapidly in aged skin but no change in inflammasome protein expression was found in aged skin, underscoring the role of aging as an important factor that influences the innate inflammatory response and may contribute to the pathogenesis of PU.
Materials and Methods
Pressure Plate Measurements
In vivo skin contact stress measurements were made on a male subject weighing 183 pounds/83 mg (813.4 Newtons). This portion of the study was found to be exempt under 45 CFR46.101.2 by the IRB at the Hospital for Special Surgery. The written consent was obtained during original data collection during a routine educational demonstration and data in our present study did not contain any of the 18 identifiers noted in the privacy rule and as such no further consent was needed. The subject was seated on a flat surface and positioned on the approximate center of an EMED-X pressure sensor array platform (Novel, Munich, Germany). The sensor array was embedded flush with the surrounding surface and consisted of 6,080 force transducers at a resolution of four sensors per cm2, a total sensor area of 1,520 cm2 and measuring 47.5 cm by 32.0 cm [29]. Pressure measurements were recorded for 30 second intervals and the recorded pressure measurements were analyzed using standard EMED software (model EMED X/R®, version 13.3.50, Novel, Munich, Germany and St. Paul, MN) [29].
Specimen Loading and Tissue Processing
After IRB approval, skin specimens were obtained from 6 Caucasian female patients undergoing abdominoplasty within 15 minutes post-surgery were grouped based on age into: young (29–35 years old) and aged (54–60 years old) groups. The skin was cleaned of blood and fat and ten full thicknesses, 7 mm biopsies were obtained per skin specimen.
We have used previously described Mechanical Explant Test System (METS) [27] to apply load to 7 mm full thickness skin specimens. A flat porous platen was used to equally distribute the load over the entire specimen, producing a uniaxial static compressive stress (hydrostatic pressure) throughout the specimen. The METS applied a static stress of 300 kPa for 0.5, 1, 2 and 4 hrs. Unloaded skin maintained at the air-liquid interface served as control for each corresponding time point. Samples were either snap frozen or 10% formalin fixed, processed and paraffin embedded. 8 µm sections were subjected to hematoxylin and eosin staining (H&E) and picrosirius red staining using previously described protocol [20], [30], [31].
TUNEL and Collagen Alignment Assays
De-paraffinisation and rehydration were carried out as previously described [32]. TUNEL assay was performed using kit (GenScript USA Inc), following commercial protocol. The slides were mounted using Fluorescein-FragEL™ Mounting Media. Digitally captured picrosirius red stained images of sections were analyzed with ImageJ (version 1.47; http://rsbweb.nih.gov/ij/) using a protocol adapted from Noorlander et al. [33]. Briefly, images were processed using a binary filter, resulting fiber outlines were then fitted with ellipses, then mean length of the major axis was then determined as a measurement for orientation of the bundles of aligned collagen fibers in the plane of the section [33].The mean value of this length parameter was based on three images per section, with a total of 15 specimens per age group, in three serial sections of a specimen was used as a collagen alignment index; the collagen alignment indices of control and loaded skin were compared and differences were analyzed.
Immunobloting
Proteins were extracted using Tissue-PE LB Kit (Geno technology, inc., MO) with addition of Protease (Sigma-Aldrich, MO) and Phosphatase inhibitor Cocktail Set III (Calbiochem, Ca) according to the manufacturer protocols. Protein lysates were mixed with 5× SDS Laemmli Sample Buffer (Sigma Aldrich, St. Louis, MO) and then resolved in 10–20% Tris-HCl Criterion precasted Gels (Bio-Rad, Hercules, CA), transferred to polyvinylidene difluoride membranes (Applied Biosystems, Foster City, CA) and placed in blocking buffer for 1 hour (Applied Biosystems) Membranes were incubated with the primary antibodies (1∶500) against NLRP3 (Enzo Life Sciences, Farmingdale, NY), ASC (kindly provided by Dr. Robert Keane), caspase-1 (Imgenex, San Diego, CA) and IL-1β (Cell Signaling, Danvers, MA), washed in blocking buffer and incubated with either rat or mouse secondary horseradish peroxidase (HRP)-linked antibodies (Cell Signaling, Danvers, MA). Proteins were visualized by chemiluminescence with a phototope-HRP detection kit (Cell Signaling Danvers, MA). Immunoblots were stripped with Restore, Western Blot Stripping Buffer (Pierce, Rockford, IL), and blotted using mouse monoclonal anti-β-actin antibody (1∶5000; Sigma, St. Louis, MO) to test protein loading. The band densities were quantified with UN-SCAN-IT software, and all data were normalized to β-actin.
Results
Development of ex vivo human model to study deep tissue injury in response to static pressure
We used a pressure sensor array to directly measure skin contact pressure. By taking direct measurements on a subject placed in a reclined position we determined in vivo physiological contact surface area and, applied force, and these were used to calculate the contact stress/pressure at sub-cm2 spatial resolution. This allowed us to quantify and visualize the peak pressure and pressure variations across the subject's contact with the flat plate using the EMED-X pressure sensor system (Figure 1). The maximum peak pressure measured was 280 kPa as illustrated by the contact pressure heat maps (Figure 1A, B, C). The point of maximum pressure occurred below the sacrum with additional regions of elevated pressure below the ischial tuberosities. Based on in vivo animal data [11], [34] and our own measurements with the pressure sensor arrays, we decided to apply a static 300 kPa stress for the purpose of the present study.
An EMED-X sensor array was used to measure contact pressure with sub-cm2 resolution on a seated individual. A maximum pressure map is shown in the horizontal view (A) and rotated to illustrate the spatial pressure distribution in 3-D (B). The graph shows the pressure in N/cm2 (1 N/cm2 = 10 kPa) as a function of time for the region of peak pressure(C). METS system used for skin loading (D).
To assess changes in tissue morphology in response to load we utilized previously developed METS system [27], [28] to load a skin in confined, uniaxial static compression of 300 kPa. Skin derived from young and aged individuals was loaded for 0.5, 1, 2 and 4 hrs (Figure 1D). We chose these particular time points due to evidence indicating that the frequency and intervals between turning a patient may be more critical than pressure magnitude in the development of PU. In fact, it has been suggested to turn patients every 2 hrs, and this practice remains the basis of prevention strategies since 1959 [35], [36]. Therefore we aimed to study changes in shorter time-span (0.5 and 1 hr), suggested time (2 hrs) and prolonged load (4 hrs). Furthermore, skin explants utilized in this model do not have a vascular supply, and thus mimicked ischemic conditions.
Tissue morphology reveals differences between young and aged skin 2 and 4 hours after exposure to uniaxial static compressive stress (load/pressure)
To characterize skin changes we employed routine H&E staining and analyzed skin of young (avg.32.5 y.o) and aged (avg. 57.5 y.o) individuals in response to load. Loaded samples were compared to unloaded, control skin kept under the same conditions for an equal duration. Thus, each sample pair, loaded and unloaded, originated from the same individual. In addition, to minimize diversity we analyzed only Caucasian female patients and specific skin location. We did not observe morphological differences in the epidermis of both age groups in response to load. Keratinocytes in control and loaded skin did not show necrotic keratinocyte cell death preceding or following skin loading at any time point.
To determine if loading induced apoptosis in epidermal keratinocytes we utilized TUNEL assay. We did not observe double-stranded DNA fragmentation, TUNEL positive cells, in any tested specimens or time points (data not shown). However, we observed subepidermal separation in both young and aged skin but at the different time points (Figure 2 A, B). These subepidermal separations were seen consistently in skin from all tree donors. The extent of sub-epidermal separation showed variability among loaded biopsies. Morphological changes were found in dermis of young skin upon 4 hrs of loading (Figure 2A). Interestingly, similar changes occurred in aged skin at earlier time point, 2 hrs, and were maintained at 4 hrs (Figure 2B), suggesting that aged skin is more susceptible to morphological changes due to applied load and present ischemia than the skin derived from young individuals.
H&E staining of unloaded and loaded young (A) and aged (B) skin for 0.5, 1, 2 and 4 hrs (n = 15 specimens per n = 3 experimental replicates). Breaks in a near proximity to basement membrane, as indicated by black arrows, are observed 4 hrs after loading in young and 2 and 4 hrs after loading in aged skin. Inserts represent enlarged images of the areas indicated by black arrows. Magnification 20×. Scale bar 100 µm. Orientation of collagen fibers in a dermis of unloaded and loaded young (C) and aged (D) skin. Quantification of collagen orientation in a plane of section indicates significantly higher mean value in loaded aged skin after 2 and 4 hours of loading. Values are expressed as mean ± SD (n = 15 specimens per n = 3 experimental replicates). * Indicates p<0.05 by paired Student t-test.
Two hours of load alters orientation of collagen fibers in dermis of aged skin
Collagen fiber orientation was evaluated using picosirius red staining viewed with polarized light microscopy. To further analyze changes occurring in dermis of young and aged individuals in response to loading we utilized a quantitative microscopic method to assess changes in the orientation of collagen fibers using a protocol adapted from Noorlander et al. [33]. To quantitatively determine the orientation of collagen fibers in the dermis we converted digital images of sections into binary images and analyzed them on the basis of the measured length of the collagen fibers in the plane of the section as a measure for the fibers orientation [33]. The orientation of collagen fibers in sections of aged skin loaded for 2 and 4 hrs differed significantly when their length was measured compared to control, unloaded, aged skin (Figure 2, C, D). The earliest detectable changes observed in aged skin were found at 2 hrs of loading (Figure 2D). In contrast, no significant changes were found in young skin (Figure 2C). These results indicate that aged skin might be more susceptible to changes in collagen alignment in response to prolonged load and ischemia.
Aged skin shows no detectable levels of active IL-1β, which is not regulated by load
IL-1β is present and released from epidermal keratinocytes upon UV-radiation, sterile skin trauma and injury [20], [37], [38]. Therefore, we performed western blot analysis to determine IL-1β protein levels. As shown in Figure 3 (A–B), young human skin ex vivo expressed the active form of IL-1β, whereas aged skin samples showed barely detectable levels. In response to load, IL-1β decreased only in young whereas it remained low in aged skin, suggesting a decreased inflammatory response to loading and ischemia.
IL-1β levels in loaded and unloaded young and aged skin was determined by Western blots (A). Quantification of these immunoblots by densitometry using β-actin as a control (n = 3) (B) shows that loading decreased IL-1β expression in young skin. Levels of IL-1β in aged skin are negligible as compared to young skin regardless of load. Levels of NLRP3 inflammasome proteins quantified by Western blot are significantly lower in aged skin as compared to young skin. Caspase-1(C), ASC (D) and NLRP3(E) protein levels, quantified by densitometry using β-actin as a control (n = 3), show that loading induced a significant increase in NLRP3 and caspase-1 expression in young skin 0.5 and 4 hrs upon loading, but not in aged skin. Values are expressed as mean ± SEM. * Indicates p<0.05 by Student t-test.
NLRP3 inflammasome proteins levels are decreased in aged skin
To determine inflammasome protein expression levels in human skin of the two age groups we quantified components of NLRP3 inflammasome complex by immunoblotting. As shown in Figure 3 (C–E), NLRP3 inflammasome components were differentially expressed in young and aged skin. Specifically, caspase-1(Figure 3C), ASC (Figure 3D) and NLRP3 (Figure 3E) were significantly lower in aged skin when compared to young skin. The higher levels of NLRP3 inflammasome proteins in young skin may indicate that aging alters the innate immune inflammatory response.
Load does not alter NLRP3 inflammasome proteins levels in aged skin
To test whether load alters levels of NLRP3 inflammasome proteins, we quantified NLRP3, ASC and caspase-1 in specimens of both age groups by immunoblotting. As shown in Figure 3 (C–E), load did not alter NLRP3 inflammasome proteins in aged skin. In contrast, in young skin, loading significantly increased levels of NLRP3 inflammasome proteins in a time-dependent manner. After exposure to 0.5 hr of load, caspase-1 and NLRP3 levels significantly increased. These protein increases were maintained for up to 4 hrs of load. No changes in the levels of ASC were observed. However, 4 hr continuous load induced levels of caspase -1 and NLRP3 in young skin.
Discussion
In this report, we describe a novel mechanism by which biomechanical load (compressive confined pressure) leads to changes in skin morphology and inflammasome activation as early changes that lead to development of DTI, and possibly PUs. Furthermore, we also describe a novel experimental approach of DTI in human ischemic skin and skin response to confined compressive load/pressure (Figure 4). Exposure of human skin to confined compressive load results in significant morphological changes, including subepidermal separation, and altered orientation of collagen fibers. These changes are affected by age and length of exposure. Aged skin showed changes as early as 2 hrs of loading, and changes in collagen alignment were only observed in aged skin. We found that aged skin expressed NLRP3 inflammasome proteins at very low levels and that loading did not alter their expression. Interestingly, we found that loading induced significant alterations in NLRP3 inflammasome protein levels in young skin in a time-dependent manner. Interestingly, extended continuous load induced NLRP3 inflammasome proteins, suggesting that prolonged load may lead to excessive inflammatory response in ischemic young skin. Taken together, these data demonstrate that load/pressure triggers specific tissue response in skin, morphological changes and rapid inflammatory response that may not be entirely preventable. Furthermore, we provide evidence that aging markedly influences response to load, underscoring its role in development of PUs among elderly.
Keratinocytes play a major role in the inflammatory response, a well-tuned tissue response that initiates wound healing process in skin and other tissues [20], [39]–[41]. Inflammasome proteins are synthesized by keratinocytes [37], [42], activated in psoriasis model [23] and IL-1β is released from cells in response to the injury and metabolic stress [43], [44]. NLRP3 induces activation of caspase-1 via interactions with the adaptor protein ASC. Based on our present findings showing presence of NLRP3, ASC and caspase-1 in control young skin, we conclude that human skin ex vivo constitutively expresses NLRP3 inflammasome proteins. Similarly, human melanoma cells and central nervous system cells show constitutive levels of inflammasome proteins [45]–[48]. The levels of NLRP3 inflammasome proteins decrease with age, offering possible explanation for decreased immune response in elderly [49]–[51] further supporting the notion that NLRP3 is engaged in the inflammasome signaling in skin. Our studies provide novel findings on how aging and pressure/load regulate inflammasome in skin.
We show that loading of young skin leads to increased levels of NLRP3 and active form of inflammatory caspase-1 (12 kDa), whereas levels of ASC do not change. It appears that initial increase resolves quickly whereas prolonged load (4 hrs) leads to its extended increase. This correlates with morphological changes observed in young ischemic skin at 4 hrs, perhaps suggesting that prolonged load extends inflammasome activation leading to tissue damage. ASC did not show significant change, which is not surprising since it serves as the adaptor protein that brings the NLRP3 and caspase-1 together, which in turn, results in inflammasome activation.
Surprisingly, much lower levels of inflammasome constituents tested were found in aged skin. Loading of aged skin did not cause additional changes in NLRP3 inflammasome proteins. This age-mediated decrease in levels and failure to activate the NLRP3 inflammasome may represent important insights to the skin's innate inflammatory response to load. The mechanism by which the inflammasome regulates wound healing and how aging affects it are under current investigations. Based on our initial observations presented here, coupled with common knowledge that PUs are mostly developed in aged, immobilized individuals [52], [53], [54], we conclude that the inflammasome complex may contribute to pathogenesis of PU.
Inflammatory cytokine IL-1β undergoes maturation and release after cleavage by active caspase-1 [55]. Using METS system we showed that both aging and loading decrease IL-1β levels at every time points studied, suggesting involvement of active IL-1β in pathogenesis of DTI. Decreased levels of IL-1β in aged skin may be due to an altered inflammatory response and dysfunctional inflammasome activation. These findings are consistent with our data showing that the NLRP3 inflammasome protein levels are low in aged skin, regardless if the skin was loaded or not. One can argue that aging may lead to defective IL-1β processing, whereas loading may lead to abolition or delayed IL-1β activation. In young loaded skin the inflammasome protein levels were high but IL-1β levels were low after load, which may suggest that load disrupts the interactions between the inflammasome proteins and inhibits processing of IL-1β even if inflammasome proteins are present. It has been shown, in other systems for instance, that IL-1β can undergo caspase-1 independent activation [56]–[58] and that caspase-1 inhibitors are not able to interfere with the whole spectrum of IL-1 β production [59]. This could explain why the levels of inflammasome proteins remained high in young loaded skin but levels of mature IL-1β (17 kDa) was low. On the other hand, one should keep in mind that reports from studies showed elevated levels of IL1, TNF, MMP's and defensins in human PU [8]–[15], which appears to be in contrast to the findings described here of decreased IL-1 β production in aged skin after loading. The ability to quickly respond to external injury, such as load, should not be interpreted as inability to mount an inflammatory response. In addition, this discrepancy can originate from difference in bacterial presence, which will be included in our future experiments, since presence of infection is one of the frequent problems in PU [60].
In addition to providing new evidence of inflammasome role in development of DTI and underscoring the role of aging in this process, we also describe a model to study initial tissue response to load, early changes that may lead to DTI and further to PU skin response to load. There are number of experimental models that study how mechanical forces affect wound healing [61], though their primary focus was to examine how various devices, such as vacuum-assisted closure or shock-waves, may accelerate wound healing [62], [63], [64], [65]. However, models that utilize application of compressive load to skin to study development of DTI are very scarce. Current animal models include use of magnetic devices [15], [66] or spinal cord injury models [67]. Although important knowledge was gained from these studies, the correlation to human condition is limited, mostly because of anatomical difference between rodents and humans and limitations in precise control of the applied load/pressure. Conversely, early tissue changes leading to the development of PU cannot be captured directly from patients because by the time of specimen collection the PU has already advanced. Here we describe a novel experimental model that utilizes METS to apply confined compressive load to human ischemic skin ex vivo and describe age-specific response to it. This model does not include vascular supply that represents both limitation and advantage. Although it cannot measure cellular infiltrate and its role in repair, the advantage is that it resembles profound ischemic conditions. Therefore, the development of the model that utilizes human skin, applies confined compressive load that reflects actual pressure on skin in sacral area of a patient in reclining position and controls the loading time represents very useful and relevant new experimental approach to study mechanisms of DTI/PU development and complements both animal models and patients' biopsies approaches.
It has been shown in vitro that small loads cause structural changes to the dermis [68], [69]. Histological changes observed in patients suffering from different stages of PUs [68], [69] showed that the earliest signs of damage appear in the upper dermis. Subepidermal separation and subepidermal bullae occurring without epidermal damage were also found [68], which is strikingly similar to the morphological changes we detected, supporting the value of the model. We report that a continuous load of 300 kPa leads to subepidermal separation in ex vivo human skin upon loading for 4 hrs in both, aged and young ischemic skin, suggesting that tissue damage may not be entirely preventable. Changes occur more rapidly in aged skin and alterations in collagen fibers orientation are feature of aged skin. Thinning of dermis, reduced collagen production, increased MMP-1 and slow proliferation of fibroblast in aged skin [70]–[74] are contributing factors. Our findings suggest that compressive load further affects tissue collagen fiber orientation. This added damage to the matrix may contribute to additional decrease in stiffness of dermis, making skin more susceptible to PU development with age, supporting clinical observations of high incidence of PU in elderly [52], [53].
Taken together, although external load/pressure is viewed as one of the key factors in the development of DTI/PU, observed decrease in NLRP3 inflammasome proteins in aged skin may indicate diminished innate immune response in skin due to aging, providing an explanation why PU develop more frequently in elderly. These findings coupled with the changes in skin morphology, collagen orientation and molecular composition of skin underscore the role of aging and compressive load in the pathogenesis of DTI. Our findings may provide important new insights for development of treatment strategies for patients with DTI that may be helpful for future preventions of PU formation among individuals at risk.
Acknowledgments
We would like to acknowledge Dr. Hillstrom and the Leon Root Motion Analysis Laboratory (Hospital for Special Surgery, New York, NY) for assistance with pressure measurements, Dr R.B. Jetter and Dr A. Labruna for providing skin specimens from reduction surgeries and all the members of Tomic-Canic laboratory for technical assistance and overall support.
Author Contributions
Conceived and designed the experiments: OS PAT RWK MT-C. Performed the experiments: OS JM AS JWB PAT MT-C. Analyzed the data: OS JM AS JWB JPdRV RWK MT-C. Contributed reagents/materials/analysis tools: PAT RWK WDD MT-C. Wrote the paper: OS JM JWB WDD RWK MT-C. Wrote IRB protocol and obtained approval: OS MT-C.
References
- 1. Bansal C, Scott R, Stewart D, Cockerell CJ (2005) Decubitus ulcers: a review of the literature. Int J Dermatol 44: 805–810.
- 2. Baumgarten M, Margolis DJ, Localio AR, Kagan SH, Lowe RA, et al. (2006) Pressure ulcers among elderly patients early in the hospital stay. J Gerontol A Biol Sci Med Sci 61: 749–754.
- 3. Ankrom MA, Bennett RG, Sprigle S, Langemo D, Black JM, et al. (2005) Pressure-related deep tissue injury under intact skin and the current pressure ulcer staging systems. Adv Skin Wound Care 18: 35–42.
- 4. Lyder CH (2003) Pressure ulcer prevention and management. JAMA 289: 223–226.
- 5. Ducker A (2002) Pressure ulcers: assessment, prevention, and compliance. Case Manager 13: 61–64 quiz 65.
- 6. Beckrich K, Aronovitch SA (1999) Hospital-acquired pressure ulcers: a comparison of costs in medical vs. surgical patients. Nurs Econ 17: 263–271.
- 7.
Services UDoHaH (2004) Guidance to Surveyors for Long Term Care Facilities.
- 8. Barone EJ, Yager DR, Pozez AL, Olutoye OO, Crossland MC, et al. (1998) Interleukin-1alpha and collagenase activity are elevated in chronic wounds. Plast Reconstr Surg 102: 1023–1027 discussion 1028–1029.
- 9. Taverna D, Nanney LB, Pollins AC, Sindona G, Caprioli R (2011) Multiplexed molecular descriptors of pressure ulcers defined by imaging mass spectrometry. Wound Repair Regen 19: 734–744.
- 10. Ladwig GP, Robson MC, Liu R, Kuhn MA, Muir DF, et al. (2002) Ratios of activated matrix metalloproteinase-9 to tissue inhibitor of matrix metalloproteinase-1 in wound fluids are inversely correlated with healing of pressure ulcers. Wound Repair Regen 10: 26–37.
- 11. Bosboom EM, Bouten CV, Oomens CW, van Straaten HW, Baaijens FP, et al. (2001) Quantification and localisation of damage in rat muscles after controlled loading; a new approach to study the aetiology of pressure sores. Med Eng Phys 23: 195–200.
- 12. Sisco M, Liu WR, Kryger ZB, Mustoe TA (2007) Reduced up-regulation of cytoprotective genes in rat cutaneous tissue during the second cycle of ischemia-reperfusion. Wound Repair Regen 15: 203–212.
- 13. Salcido R, Popescu A, Ahn C (2007) Animal models in pressure ulcer research. J Spinal Cord Med 30: 107–116.
- 14. Goldstein B, Sanders J (1998) Skin response to repetitive mechanical stress: a new experimental model in pig. Arch Phys Med Rehabil 79: 265–272.
- 15. de la Garza-Rodea AS, Knaan-Shanzer S, van Bekkum DW (2011) Pressure ulcers: description of a new model and use of mesenchymal stem cells for repair. Dermatology 223: 266–284.
- 16. Bonomo SR, Davidson JD, Tyrone JW, Lin X, Mustoe TA (2000) Enhancement of wound healing by hyperbaric oxygen and transforming growth factor beta3 in a new chronic wound model in aged rabbits. Arch Surg 135: 1148–1153.
- 17. Bronneberg D, Spiekstra SW, Cornelissen LH, Oomens CW, Gibbs S, et al. (2007) Cytokine and chemokine release upon prolonged mechanical loading of the epidermis. Exp Dermatol 16: 567–573.
- 18. Cornelissen LH, Bronneberg D, Bader DL, Baaijens FP, Oomens CW (2009) The transport profile of cytokines in epidermal equivalents subjected to mechanical loading. Ann Biomed Eng 37: 1007–1018.
- 19. Freedberg IM, Tomic-Canic M, Komine M, Blumenberg M (2001) Keratins and the Keratinocyte Activation Cycle. J Invest Dermatol 116: 633–640.
- 20. Vukelic S, Stojadinovic O, Pastar I, Rabach M, Krzyzanowska A, et al. (2011) Cortisol synthesis in epidermis is induced by IL-1 and tissue injury. J Biol Chem 286: 10265–10275.
- 21. Contassot E, Beer H, French L (2012) Interleukin-1, inflammasomes, autoinflammation and the skin. Swiss Med Wkly 142: 0.
- 22. Feldmeyer L, Werner S, French LE, Beer HD (2010) Interleukin-1, inflammasomes and the skin. Eur J Cell Biol 89: 638–644.
- 23. Dombrowski Y, Peric M, Koglin S, Kammerbauer C, Goss C, et al. (2011) Cytosolic DNA triggers inflammasome activation in keratinocytes in psoriatic lesions. Sci Transl Med 3: 82ra38.
- 24. Martinon F, Tschopp J (2007) Inflammatory caspases and inflammasomes: master switches of inflammation. Cell Death Differ 14: 10–22.
- 25. Rajamaki K, Lappalainen J, Oorni K, Valimaki E, Matikainen S, et al. (2010) Cholesterol crystals activate the NLRP3 inflammasome in human macrophages: a novel link between cholesterol metabolism and inflammation. PLoS One 5: e11765.
- 26. Salskov-Iversen ML, Johansen C, Kragballe K, Iversen L (2011) Caspase-5 expression is upregulated in lesional psoriatic skin. J Invest Dermatol 131: 670–676.
- 27. Torzilli PA, Bhargava M, Chen CT (2011) Mechanical Loading of Articular Cartilage Reduces IL-1-Induced Enzyme Expression. Cartilage 2: 364–373.
- 28. Torzilli PA, Grigiene R, Huang C, Friedman SM, Doty SB, et al. (1997) Characterization of cartilage metabolic response to static and dynamic stress using a mechanical explant test system. J Biomech 30: 1–9.
- 29. Brophy RH, Gamradt SC, Ellis SJ, Barnes RP, Rodeo SA, et al. (2009) Effect of turf toe on foot contact pressures in professional American football players. Foot Ankle Int 30: 405–409.
- 30. Vukelic S, Stojadinovic O, Pastar I, Vouthounis C, Krzyzanowska A, et al. (2010) Farnesyl pyrophosphate inhibits epithelialization and wound healing through the glucocorticoid receptor. J Biol Chem 285: 1980–1988.
- 31. Tomic-Canic M, Mamber SW, Stojadinovic O, Lee B, Radoja N, et al. (2007) Streptolysin O enhances keratinocyte migration and proliferation and promotes skin organ culture wound healing in vitro. Wound Repair Regen 15: 71–79.
- 32. Pastar I, Stojadinovic O, Krzyzanowska A, Barrientos S, Stuelten C, et al. (2010) Attenuation of TGFbeta Signaling Pathway in Chronic Venous Ulcers. Mol Med 16: 92–101.
- 33. Noorlander ML, Melis P, Jonker A, Van Noorden CJ (2002) A quantitative method to determine the orientation of collagen fibers in the dermis. J Histochem Cytochem 50: 1469–1474.
- 34. Nola GT, Vistnes LM (1980) Differential response of skin and muscle in the experimental production of pressure sores. Plast Reconstr Surg 66: 728–733.
- 35. Kosiak M (1959) Etiology and pathology of ischemic ulcers. Arch Phys Med Rehabil 40: 62–69.
- 36. Smith AM, Malone JA (1990) Preventing pressure ulcers in institutionalized elders: assessing the effects of small, unscheduled shifts in body position. Decubitus 3: 20–24.
- 37. Feldmeyer L, Keller M, Niklaus G, Hohl D, Werner S, et al. (2007) The inflammasome mediates UVB-induced activation and secretion of interleukin-1beta by keratinocytes. Curr Biol 17: 1140–1145.
- 38. Sjogren F, Anderson C (2009) Sterile trauma to normal human dermis invariably induces IL1beta, IL6 and IL8 in an innate response to “danger”. Acta Derm Venereol 89: 459–465.
- 39. Tomic-Canic M, Komine M, Freedberg IM, Blumenberg M (1998) Epidermal signal transduction and transcription factor activation in activated keratinocytes. J Dermatol Sci 17: 167–181.
- 40.
Tomic-Canic M, Magnus SA, Oscar MA (2004) Epidermal repair and the chronic wound. In: David T Rovee, Maibach HI, editors. The epidermis in wound healing. Boca Raton: CRC Press LLC. pp. 25–57.
- 41. Suter MM, Schulze K, Bergman W, Welle M, Roosje P, et al. (2009) The keratinocyte in epidermal renewal and defence. Vet Dermatol 20: 515–532.
- 42. Sollberger G, Strittmatter GE, Kistowska M, French LE, Beer HD (2012) Caspase-4 is required for activation of inflammasomes. J Immunol 188: 1992–2000.
- 43. Dinarello CA (2006) Interleukin 1 and interleukin 18 as mediators of inflammation and the aging process. Am J Clin Nutr 83: 447S–455S.
- 44. Nakamura Y, Franchi L, Kambe N, Meng G, Strober W, et al. (2012) Critical role for mast cells in interleukin-1beta-driven skin inflammation associated with an activating mutation in the nlrp3 protein. Immunity 37: 85–95.
- 45. Kopfnagel V, Wittmann M, Werfel T (2011) Human keratinocytes express AIM2 and respond to dsDNA with IL-1beta secretion. Exp Dermatol 20: 1027–1029.
- 46. de Rivero Vaccari JP, Lotocki G, Marcillo AE, Dietrich WD, Keane RW (2008) A molecular platform in neurons regulates inflammation after spinal cord injury. J Neurosci 28: 3404–3414.
- 47. de Rivero Vaccari JP, Lotocki G, Alonso OF, Bramlett HM, Dietrich WD, et al. (2009) Therapeutic neutralization of the NLRP1 inflammasome reduces the innate immune response and improves histopathology after traumatic brain injury. J Cereb Blood Flow Metab 29: 1251–1261.
- 48. Abulafia DP, de Rivero Vaccari JP, Lozano JD, Lotocki G, Keane RW, et al. (2009) Inhibition of the inflammasome complex reduces the inflammatory response after thromboembolic stroke in mice. J Cereb Blood Flow Metab 29: 534–544.
- 49. Youm YH, Kanneganti TD, Vandanmagsar B, Zhu X, Ravussin A, et al. (2012) The NLRP3 Inflammasome Promotes Age-Related Thymic Demise and Immunosenescence. Cell Rep 1: 56–68.
- 50. Kauppinen A, Niskanen H, Suuronen T, Kinnunen K, Salminen A, et al. (2012) Oxidative stress activates NLRP3 inflammasomes in ARPE-19 cells-Implications for age-related macular degeneration (AMD). Immunol Lett 147: 29–33.
- 51. Salminen A, Ojala J, Kaarniranta K, Kauppinen A (2012) Mitochondrial dysfunction and oxidative stress activate inflammasomes: impact on the aging process and age-related diseases. Cell Mol Life Sci 69: 2999–3013.
- 52. Brem H, Tomic - Canic M, Taranovskaya A, Ehlich HP, Baskin-Bay E, et al. (2003) Healing of Elderly Patients with Diabetic Foot Ulcers, Venous Stasis Ulcers, and Pressure Ulcers. Surgical Technology International 161–167.
- 53. Foglia E, Restelli U, Napoletano AM, Coclite D, Porazzi E, et al. (2012) Pressure ulcers management: an economic evaluation. J Prev Med Hyg 53: 30–36.
- 54. Linder-Ganz E, Scheinowitz M, Yizhar Z, Margulies SS, Gefen A (2007) How do normals move during prolonged wheelchair-sitting? Technol Health Care 15: 195–202.
- 55. Dinarello CA (1997) Interleukin-1. Cytokine Growth Factor Rev 8: 253–265.
- 56. Guma M, Ronacher L, Liu-Bryan R, Takai S, Karin M, et al. (2009) Caspase 1-independent activation of interleukin-1beta in neutrophil-predominant inflammation. Arthritis Rheum 60: 3642–3650.
- 57. Nagarajan UM, Sikes JD, Yeruva L, Prantner D (2012) Significant role of IL-1 signaling, but limited role of inflammasome activation, in oviduct pathology during Chlamydia muridarum genital infection. J Immunol 188: 2866–2875.
- 58. Pelegrin P, Barroso-Gutierrez C, Surprenant A (2008) P2X7 receptor differentially couples to distinct release pathways for IL-1beta in mouse macrophage. J Immunol 180: 7147–7157.
- 59. Joosten LA, Netea MG, Fantuzzi G, Koenders MI, Helsen MM, et al. (2009) Inflammatory arthritis in caspase 1 gene-deficient mice: contribution of proteinase 3 to caspase 1-independent production of bioactive interleukin-1beta. Arthritis Rheum 60: 3651–3662.
- 60. Braga IA, Pirett CC, Ribas RM, Filho PP, Filho AD (2013) Bacterial colonization of pressure ulcers: assessment of risk for bloodstream infection and impact on patient outcomes. J Hosp Infect 83: 314–320.
- 61. Agha R, Ogawa R, Pietramaggiori G, Orgill DP (2011) A review of the role of mechanical forces in cutaneous wound healing. J Surg Res 171: 700–708.
- 62. Qureshi AA, Ross KM, Ogawa R, Orgill DP (2011) Shock wave therapy in wound healing. Plast Reconstr Surg 128: 721e–727e.
- 63. Ichioka S, Watanabe H, Sekiya N, Shibata M, Nakatsuka T (2008) A technique to visualize wound bed microcirculation and the acute effect of negative pressure. Wound Repair Regen 16: 460–465.
- 64. Derrick KL, Norbury K, Kieswetter K, Skaf J, McNulty AK (2008) Comparative analysis of global gene expression profiles between diabetic rat wounds treated with vacuum-assisted closure therapy, moist wound healing or gauze under suction. Int Wound J 5: 615–624.
- 65. Orgill DP, Bayer LR (2011) Update on negative-pressure wound therapy. Plast Reconstr Surg 127 Suppl 1: 105S–115S.
- 66. Demiot C, Sarrazy V, Javellaud J, Gourloi L, Botelle L, et al. (2011) Erythropoietin restores C-fiber function and prevents pressure ulcer formation in diabetic mice. J Invest Dermatol 131: 2316–2322.
- 67. Lin F, Pandya A, Cichowski A, Modi M, Reprogle B, et al. (2010) Deep tissue injury rat model for pressure ulcer research on spinal cord injury. J Tissue Viability 19: 67–76.
- 68. Witkowski JA, Parish LC (1982) Histopathology of the decubitus ulcer. J Am Acad Dermatol 6: 1014–1021.
- 69. Edsberg LE (2007) Pressure ulcer tissue histology: an appraisal of current knowledge. Ostomy Wound Manage 53: 40–49.
- 70. Oikarinen A (1994) Aging of the skin connective tissue: how to measure the biochemical and mechanical properties of aging dermis. Photodermatol Photoimmunol Photomed 10: 47–52.
- 71. Waller JM, Maibach HI (2006) Age and skin structure and function, a quantitative approach (II): protein, glycosaminoglycan, water, and lipid content and structure. Skin Res Technol 12: 145–154.
- 72. Uitto J (1986) Connective tissue biochemistry of the aging dermis. Age-related alterations in collagen and elastin. Dermatol Clin 4: 433–446.
- 73. Khorramizadeh MR, Tredget EE, Telasky C, Shen Q, Ghahary A (1999) Aging differentially modulates the expression of collagen and collagenase in dermal fibroblasts. Mol Cell Biochem 194: 99–108.
- 74. Quan T, He T, Shao Y, Lin L, Kang S, et al. (2006) Elevated cysteine-rich 61 mediates aberrant collagen homeostasis in chronologically aged and photoaged human skin. Am J Pathol 169: 482–490.