Abstract
Background: Burn wound progression refers to the phenomenon of continued tissue loss following abatement of an initial thermal insult, which makes the treatment more difficult, prolongs hospital stay, increases medical costs, and raises the likelihood of scar formation. Autophagy is a highly conserved pathway that delivers intracellular macromolecule waste to lysosomes, where they are degraded into biologically active monomers, such as amino acids, that are subsequently reused to maintain cellular metabolic turnover and homeostasis. We aimed to observe the expression of autophagy in burn wounds in a deep second‐degree rodent burn model and further investigate the role of autophagy on burn wound progression and wound healing.
Keywords
- Autophagy
- Burn
- injury progression
- wound healing
- rapamycin
1. Introduction
After the initial thermal insult, tissue necrosis is continued in burn wound, which is referred to as the phenomenon of “burn wound progression” [1]. The progression of burn wound is an important problem in clinic, largely determining the morbidity and mortality of burn patients. Generally, the burn wound can be divided into three concentric zones [2]: the zone of coagulation, the zone of stasis, and the zone of hyperemia. While the central zone of coagulation is distinguished by irreversible tissue necrosis and the outer zone of hyperemia can always naturally recover, the intermediate zone of stasis may either progress into necrosis or can be salvaged if optimal treatments be available [3].
It has been demonstrated that burn wound progression is attributed to many mechanisms, including tissue hypoperfusion, prolonged inflammation, edema, hypercoagulability, and free radical damage [4]. Many studies have aimed to ameliorate burn wound progression by intervening these above mechanisms, and certain advance has already been achieved. However, further studies are still needed to help us better understand this complicated process.
Autophagy is a lysosomal‐dependent degradation pathway, which is indispensable for survival, development, differentiation, and cellular homeostasis [5]. Autophagy has been reported to protect against ischemic injuries, inflammatory diseases, and other disease models [6]. To understand the role of autophagy in burn wound progression, firstly, we designed an animal study to examine the expressing pattern of autophagy in burn wounds. We found that autophagy level in the zone of stasis was increased when comparing to the normal unburned tissue. We speculated that the increase of autophagy level in the zone of stasis was a survival mechanism against tissue ischemia, excessive inflammatory response, and oxidative stress in burn wounds [7].
Rapamycin is a macrolide antibiotic agent, which was initially used as an antifungal drug, and
3. Results
3.1. Expression rule of autophagy proteins in burn wounds
Levels of LC3 and Beclin‐1 protein were maintained at a certain degree in normal skin tissue. After burn was inflicted, levels of these proteins declined continuously in wound tissue until 24 h after the burn. Levels then increased slightly, but remained far lower than in normal skin samples. Quantitative analysis show that autophagy level decreased about fourfold over 24 h, and then began to increase but still could not reach their normal level (Figure 1).
3.2. Change of apoptosis level in burn wounds
To investigate the apoptosis level of burn wounds, we conducted TUNEL staining to see how the apoptosis level in burn wounds would change after burn was inflicted. We found more cells undergoing apoptosis in burn wounds than control. The apoptotic rates in burn wounds at 6, 24, 48, and 72 h are 4.56 ± 0.27, 11.76 ± 0.7, 13.16 ± 0.65, and 8.14 ± 0.62%, respectively, versus 2.23 ± 0.23% of controls (mean ± SD,
3.3. Change of Laser Doppler Flowmetry (LDF) value and Myeloperoxidase (MPO) activity in burn wounds
LDF value in burn wounds is an indicator of burn wound blood flow, while MPO activity reflects the inflammatory response in the burn wound. We found that the LDF values decreased fourfold over 12 h after burn and then began to increase but still far lower normal level. The MPO activity increased about 5.3‐fold over 48 h after burn and then decreased slightly, yet still significantly higher than control (Figure 3).
3.4. LC3 staining in the zone of stasis
We found that LC3‐positive cells in the deep dermis adjacent to the subcutaneous tissue, which in this deep second‐degree burn model, may represent the zone of stasis, which were much more than that of control. We conducted a quantitative analysis and found that the increase of LC3‐positive cells in the deep dermis was significant at 6, 24, and 48 h post burn (Figure 4).
3.5. Rapamycin enhanced the autophagic level in burn wounds
Western bolt analysis showed that the protein levels of two autophagy markers, LC3 and Beclin‐1, were significantly augmented in the thermal burn wounds of the rapamycin‐treated group as compared with the levels seen in the control group (Figure 5). The expression of both proteins in burn wounds were at their lowest 24 h post‐thermal burn injury and then gradually increased with time. The patterns of LC3‐II/LC3‐I and Beclin‐1 expression were almost identical (Figure 5). Moreover, the increases in expression of these proteins were statistically significant at 6 h (
3.6. Rapamycin treatment inhibited apoptosis in burn wounds
To further investigate if the enhanced autophagy had any effects on apoptosis of burn wounds, we conducted TUNEL staining to see if the apoptosis level in burn wounds of treated rats were different from controls. Cells with shrunken brown stained nuclei were considered positive. We found fewer cells undergoing apoptosis in rats treated with rapamycin. The apoptotic rates in burn wounds of treated rats at 6, 24, 48, and 72 h are 2.99 ± 0.33, 8.85 ± 0.6, 12.48 ± 0.67, and 6.7 ± 0.31%, respectively, versus 4.56 ± 0.27, 11.76 ± 0.7, 13.16 ± 0.65, and 8.14 ± 0.62% of controls (mean ± SD,
3.7. Rapamycin treatment reduced inflammatory infiltration and restored blood perfusion in burn wounds
The LDF values and Na/K‐ATPase activities in burn wounds of the treatment group were significantly increased when compared to those of the control group (Figure 7A, B). Furthermore, both LDF values and Na/K‐ATPase activities in burn wounds were lower than those of normal unburned skin. The IL‐8 level, MPO activity, and MDA content in burn wounds of the treatment group were significantly decreased when compared to those of the control group. In addition, these measurements were almost all higher than those of normal unburned skin (Figure 7C–E). Changes in the activities of Na/K‐ATPase and MPO between the treatment and control groups were significantly different at the time points of 1 day and 2 days post‐thermal burn injury. The changes in LDF, MDA, and IL‐8 content between the treatment and control groups were also significant at the time points of 1, 2, and 3 days post‐thermal burn injury.
3.8. Rapamycin treatment reduced burn wound progression
Histopathological examination demonstrated that the burn wound progression was reduced in the treatment group when compared to the controls (Figure 8). Fewer residual hair follicles, deeper tissue necrosis, more severe collagen denaturation, and more inflammatory infiltrations in burn wounds of the control group were seen when compared to those of the treatment group. Masson staining showed that less intense staining with Masson red were seen in the treated rats when compared to control, which may indicate less tissue necrosis in the treated rats (Figure 8A–F).
3.9. Rapamycin treatment promoted burn wound healing
Finally, the time to wound re‐epithelialization was shorter in treated rats as compared with controls (22.5 ± 1.4 vs. 24.8 ± 1.3 days, respectively). (mean ± SD,
4. Discussion
The phenomenon of burn wound progression has long been considered a complex and challenging clinical and theoretical challenge. For over half a century, investigators in the field have been attempting to study the mechanisms of burn wound penetration of the epidermal and dermal layers of the skin with the objective of gaining greater insights into the pathology. Several studies [10] have demonstrated that a number of factors contribute to the invasive deepening of thermal burn wounds including a deficiency in local burn wound perfusion, edema, thrombosis, free radical damage, accumulation of factors that contribute to cell‐mediated toxicity and inflammatory cell infiltration.
The first part of our study showed that after the occurrence of burn injury, laser Doppler flow values and Na/K‐ATPase enzyme activities, which collectively represent the burn wound blood circulation and index of energy metabolism, decreased significantly. Moreover, both MPO and MDA activities, which respectively represent wound inflammation and free radical generation, increased significantly. Moreover, the autophagy level was at first reduced and then increased, yet remained far below those in normal skin. We speculate that at the early stage when the tissue necrosis due to thermal injury was inevitable, autophagy may not be a principal cellular activity as necrosis did in burn wounds and which is why autophagy level decreased at first. At the latter stage, when the inevitable tissue necrosis ceased, the remain viable tissue adjacent to coagulation was subject to ischemic and inflammatory damage among others, and then autophagy may protect against these stress stimuli as a survival mechanism which account for the latter rise of autophagy level. The prosurvival role of autophagy is supported by our another finding in IHC staining, which demonstrated significantly activated autophagy in the deep dermis which in this burn model, and represents the zone of stasis (or ischemia). In addition, at the latter stage (48–72 h) after burn, tissue perfusion as determined by LDF was restored and inflammatory infiltration in burn wounds as shown by MPO activity was reduced, in coincidence with the increase of autophagy level at the same time, which may add to evidence for the pro‐survival roles of autophagy in this burn model.
To further dissect the role of autophagy in burn wound progression, we used rapamycin as treatment intervention in the second part of the study. The results demonstrated that the autophagic levels in burn wounds were enhanced following treatment with rapamycin. Furthermore, both LDF values and Na/K‐ATPase activities (indicators of blood perfusion and energy metabolism) in the wounds of treatment group were significantly increased as compared to those of the control group. However, the IL‐8 level, MPO activities, and MDA content (representative of inflammatory reaction and free radial damage) in the wounds of rapamycin‐treated group were significantly decreased as compared to those of the control group [11]. Therefore, these results suggested that enhanced autophagy restored blood perfusion and energy metabolism, and inhibited inflammatory reaction and oxidative damage in burn wounds. Thus, it can be inferred that autophagy maintained cellular metabolic turnover and homeostasis in this experimental burn model [12].
Histopathological results showed that the burn wound depth of the rapamycin‐treated group was less remarkable and “more superficial” than that seen in the control group, particularly at 2 and 3 days following thermal tissue injury. Additionally, as compared with the burn wounds of the treatment group, there were fewer residual hair follicles, more severe denatured collagen events recorded, evidence of deeper tissue necrosis, and more obvious inflammatory infiltrates in the burn wounds of the control group. These results suggested that burn wound progression in the treated rats was ameliorated. At last, burn wounds in treatment group re‐epithelialized faster than those of control group, further indicating that prevention of burn wound progression were beneficial to burn wound healing.
5. Conclusion
Autophagy protects from burn wound progression and promotes burn wound healing through protecting the zone of stasis from further necrosis, which is probably mediated by phagocytizing damaged organelles to sustain homeostatic response and remodeling in the injured tissue.
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