Abstract
Recent findings have attested the protective effects of erythropoietin (EPO) in ischemically challenged organs. We therefore aimed at elaborating the underlying mechanism of EPO-mediated protection in musculocutaneous tissue undergoing persistent ischemia after acute injury. Mice were assigned to five experimental groups equipped with a randomly perfused flap fixed in a dorsal skinfold chamber, whereas the sixth group did not undergo flap preparation: EPO, L-Name, EPO and L-Name, EPO and bevacizumab, untreated flap, and nonischemic chamber (control). Intravital fluorescence microscopic analysis of microhemodynamics, apoptotic cell death, macromolecular leakage and angiogenesis was carried out over a 10-day period. Further, immunohistochemical analysis was used to study the protein expression of endothelial nitric oxide synthase (eNOS) and vascular endothelial growth factor (VEGF). Increased expression of eNOS in EPO-administered mice correlated with significant arteriolar dilation and thus increased blood flow resulting in a maintained functional capillary density (FCD) at day 10. In addition, EPO induced a VEGF upregulation, which was associated with newly formed capillaries. In addition, EPO was able to reduce ischemia-induced apoptotic cell death and finally to significantly reduce flap necrosis. In contrast, coadministration of L-Name abolished EPO-mediated tissue protection by abrogating the dilatory effect resulting in reduced FCD and tissue survival, without counteracting angiogenesis and apoptotic cell death, whereas additional administration of bevacizumab did not influence the beneficial effect of EPO on flap survival despite abrogating angiogenesis. Macromolecular leakage was found to be increased in all treatment groups. This study shows that EPO administration prevents musculocutaneous tissue from ischemic necrosis as a consequence of an eNOS-dependent arteriolar hyperperfusion maintaining capillary perfusion, thus representing a promising approach to pharmacologically protect ischemically challenged tissue.
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Main
Erythropoietin (EPO), a 30.4 kDa glycoprotein, is the main regulator of erythropoiesis.1 It participates in the proliferation, differentiation and migration of erythroid progenitor cells.2 Accordingly, anemia3 and decreased tissue oxygen tension4 induce the production of EPO in the adult kidney. Recent findings revealed tissue-protective properties of EPO independent of its hematopoietic properties in a variety of organ systems suffering from ischemia, such as the heart,5 brain,6, 7 liver,8 kidney9 and the striated muscle.10 EPO initiates a multitude of EPO receptor-dependent and -independent cellular pathways, including the induction of anti-apoptotic genes11 and anti-inflammatory molecules,12 the increase of vascular endothelial growth factor (VEGF), as well as the production of vasodilative molecules such as nitric oxide (NO).13 NO is an enzymatic product from L-arginine that mediates numerous biological actions through the activation of cyclic guanosine monophosphate, which inhibits intracellular calcium release and induces smooth muscle relaxation.14
As EPO and its receptor are also present in human skin,15 ischemic wound complications and tissue necrosis might be prevented by administration of EPO. Despite advances in surgical techniques, patients may still suffer from wound breakdown and ischemic necrosis.16, 17 The associated morbidity and mortality represents a considerable health-care issue.18, 19
The aim of this study was to evaluate the NO-dependent effect of systemic EPO administration starting before surgical induction of acute persistent ischemia in musculocutaneous tissue of mice. The role of microcirculatory, angiogenic and cellular mechanisms were analyzed by intravital microcopy and immunhistochemical work-up.
MATERIALS AND METHODS
Animals
The experiments were conducted in accordance with the Swiss legislation on the protection of animals. The experimental protocol was approved by the Animal Ethics Committee of the Canton of Geneva, Switzerland. A total of 78 mice (C57BL/6; 12–24 weeks old; 24–28 g body weight (bw); Zootechnie, Centre Médical Universitaire; Geneva, Switzerland) were used in the study. The animals were housed one per cage at room temperature of 22–24°C and at a relative humidity of 60–65% with a 12-h day–night cycle. The animals had free access to standard pellet chow (Altromin, Lage, Germany) and tap water ad libitum.
Anesthesia
Both surgery and repetitive intravital fluorescence microscopy were performed under anesthesia by intraperitoneal (i.p.) injection of 0.1 ml saline solution per 10 g bw of mixture of 90 mg per kg bw ketamine hydrochloride (Ketavet; Parke Davis, Freiburg, Germany) and 25 mg per kg bw dihydroxylidinothiazine hydrochloride (Rompun; Bayer, Zürich, Switzerland).
Flap Preparation
The dorsal skinfold chamber preparation, which takes ∼25 min, was used as the control group. All other experimental groups were equipped with a skinfold chamber and a critically and randomly perfused musculocutaneous flap consisting of one layer of the skin, subcutis and striated muscle (panniculus carnosus).20 As previously described, the musculocutaneous tissue is subjected to persistent ischemia resulting in ∼50% necrosis if kept untreated.21 The preparation starts after depilation by mobilization of the musculocutaneous tissue (that is, induction of ischemia). The rectangular flap of 15 × 11 mm remains attached to the animal only on its lateral border. Then it is fixed to the backside of the frame of the window chamber and sutured back to its previous position. Thereafter, the counterpart of the frame was mounted and the observation window is sealed with a coverglass, which replaces the previously removed musculocutaneous layer of the opposite layer of the skinfold, a fraction of skin that may be used for subsequent histological examination (time-point day 0). This preparation allows for repetitive microscopy of the same tissues. The animals tolerated the titanium chamber with a total weight of ∼3 g and the preparation well, as indicated by normal feeding and sleeping habits.
Intravital Epifluorescence Microscopy
For in vivo microscopic observation, animals were anesthetized and placed on a custom-made plexiglas frame. For intravascular contrast enhancement of the plasma they received intravenous (i.v.) retrobulbar injection of 0.1 ml 5% fluorescein isothiocyanate (FITC)-labeled dextran (molecular weight 150 000; 50 mg/ml saline; Sigma-Aldrich Chemie, Buchs, Switzerland). Subsequently, the animals were positioned under a Zeiss® Axiotech microscope (Zeiss, Feldbach, Switzerland) equipped with a 100-W mercury lamp and a filter set for ultraviolet (330–390 nm excitation/>430 nm emission wavelength) and blue (450–490 nm, >520 nm) light. Microscopic images were captured by a charge-coupled device video camera (Kappa CF 112, Zeiss) and transferred to a DVD recorder (Panasonic LQ-MD 800; Lucerne, Switzerland). All parameters were analyzed off-line using a computer-assisted image analysis system (Cap-Image; Zeintl Software, Heidelberg, Germany).22 The microscopic procedures for analysis of the microcirculation within the musculocutaneous tissue were performed at constant room temperature of ∼23°C.
Microcirculatory and Cellular Analysis
Every observation started with scanning of the window in × 5 magnification to determine the perfused as well as the non-perfused respectively the necrotic part of the tissue. Planimetrical evaluation was carried out thereafter and the percentage of the total area was calculated. Non-perfused tissue and necrosis are given as percentage of the total flap area.
All microcirculatory parameters were measured in perfused flap tissue. Easily identifiable branching patterns of second- or third-order arterioles accompanying collecting venules and capillary fields were selected. Video printouts of these branching patterns using the × 5 and × 20 magnification were made to relocate the same vessels for repetitive measurements during the 10-day observation period. (i) Arteriolar red blood cell (RBC) velocity (mm/s) was analyzed by a computer-assisted image analysis system using the line shift method, which is on the basis of the measurement of the shift (mm) of an individual intravascular gray-level pattern over time (seconds). (ii) Arteriolar diameter (μm) was measured perpendicularly to the vessel path. (iii) Volumetric blood flow (pl/s) was calculated in arterioles from RBC velocity and vessel cross-sectional area (π × r2) according to the equation of Gross and Aroesty, that is, Q=V × π × r2, assuming a cylindrical vessel shape.23 (iv) Functional capillary density (FCD: given in cm/cm2) was defined as the length of all RBC-perfused capillaries per observation field. For assessment of FCD, the surface of the chamber window was subdivided into three horizontal areas of equal length resulting in a proximal zone directly adjacent to the lateral side where the tissue is attached to the animal, an intercalated central zone, and a distal zone most remote from the vascular inflow. (v) Apoptotic cells (n/mm2) were identified by the characteristic nuclear condensation, fragmentation and margination with the aid of DNA-binding fluorochrome bisbenzimide H33342 (Sigma-Aldrich). Recordings were made with a × 100 objective. (vi) The microcirculatory analysis further included the evaluation of the angiogenic response, which was analyzed by the density of all newly formed blood perfused microvessels (MVD). The vessel density was calculated as the total length of these newly formed vessels divided by the area of observation and is given in cm/cm2. (vii) Macromolecular leakage as a parameter of microvascular permeability was assessed after an i.v. injection of FITC-labeled dextran 150 000, a macromolecular fluorescent dye. Gray levels in the tissue directly adjacent to the capillary vessel wall (E1), as well as in the marginal cell-free plasma of the vessel (E2) were determined densitometrically. Macromolecular extravasation (E) was then calculated as the ratio of E1/E2.24
Immunohistochemical Analysis of eNOS and VEGF
To assess the expression of endothelial nitric oxide synthase (eNOS) and VEGF using light microscopy, biopsies were snap-frozen and embedded in tissue-freezing medium (Jung; Leica Microsystems, Nussloch, Germany) or formalin fixed and embedded in paraffin. eNOS samples were cut in 5-μm sections and fixed in 4°C cold acetone for 5 s and in 4% formalin for 10 min, whereas VEGF sections were stained using indirect immunoperoxidase techniques. eNOS sections were incubated with the polyclonal rabbit anti-mouse eNOS antibody (1:25; BD Biosciences, Heidelberg, Germany). VEGF sections were incubated at 4°C overnight with a mouse monoclonal anti-mouse VEGF antibody (1:25; M7273, DakoCytomation, Hamburg, Germany) as primary antibody. A peroxidase-conjugated goat anti-rabbit IgG antibody was used as secondary antibody (1:200; Dianova, Hamburg, Germany) for both primary antibodies. 3,3′-Diaminobenzidine (DakoCytomation) was used as a chromogen. Sections were counterstained with Mayer's hemalaun. All sections were incubated with 3% H2O2 and 2% goat normal serum. Antigen retrieval was achieved by microwaving (10 min, 700 W) in EDTA buffer, pH 9. The markers eNOS and VEGF were quantitatively assessed by counting the number of visible nuclei per mm2 surface within the subcutaneous tissue.
Test Substance
Epoetin β (recombinant human EPO, NeoRecormon; Roche Pharma, Basel, Switzerland) was admixed to 0.3 ml NaCl 0.9% to achieve a final dose of 500 IU per kg bw. The solution was stored at a maximum temperature of 8°C until usage.
Nω-nitro-L-arginine methyl ester (L-Name: Sigma-Aldrich), the L-arginine analog, which inhibits NOS in a nonspecific manner, was dissolved in sterile saline at room temperature to a final dose of 50 mg per kg bw and administered slowly i.v.
Bevacizumab (Avastin; Roche Pharma), a monoclonal antibody that acts as a VEGF receptor blocker, was dissolved in sterile saline at room temperature to a final dose of 5 mg per kg bw and administered i.p.
Experimental Groups and Protocol
A total of 78 animals were equipped with flaps and dorsal skinfold chambers. In all, 42 mice were assigned to 6 experimental groups of 7 animals each: (1) EPO (500 IU per kg bw, i.p.); (2) EPO and L-Name (500 IU EPO per kg bw, i.p. +50 mg L-Name per kg bw, i.v.); (3) L-Name (50 mg per kg bw, i.v.); (4) EPO and bevacizumab (500 IU EPO per kg bw, i.p. +5 mg bevacizumab per kg bw, i.p.); (5) Flap (untreated flap: 0.3 ml NaCl, i.p.); and (6) control (nonischemic chamber: 0.3 ml NaCl, i.p.). All animals were administered three repetitive doses of the substance 30 min before and 30 min after surgery (that is, induction of ischemia), as well as 24 h after flap elevation. In case of combined application (EPO and L-Name, and EPO and bevacizumab), L-Name and bevacizumab were administered 5 min before EPO at each of the three time points. Intravital fluorescence microscopic analysis of microhemodynamics, apoptotic cell death, macromolecular leakage and angiogenesis was carried out at days 1, 3, 5, 7 and 10 after surgery. All animals were killed at the end of the experiment by administration of 1 ml of the anesthetic agent. Finally, four additional mice each (EPO, EPO and L-Name, and untreated flap) were killed at days 1, 3 and 5 after induction of ischemia to study the protein profiling of eNOS and VEGF in viable tissue using immunohistochemical analysis.
Flap preparation, microscopic examinations, as well as the off-line analysis of the collected data were carried out under blinded conditions.
Statistical Analysis
All values are expressed as mean±s.e.m. For comparison between individual time points, ANOVA for repeated measures was carried out, followed by the appropriate post hoc test (SigmaStat, Jandel, San Rafael, CA, USA), which included measures to correct the α-error according to Bonferroni probabilities. Comparison between the groups included ANOVA and the Student Newman–Keuls post hoc test. Differences were considered significant at P<0.05.
RESULTS
Flap Necrosis
Macroscopic analysis of the chamber morphology at day 10 after surgery showed distinct alterations in the central and distal areas of the flaps (Figures 1a–d). The vital tissue was separated from the distal necrosis by a red fringe indicating vasodilation and microvascular remodeling (Figure 1a). Animals treated with EPO only showed an improved tissue survival (Figure 1b), whereas coadministration of EPO and L-Name did not improve survival (Figure 1c). Of interest, application of L-Name alone was associated with further development of necrosis when compared with controls (Figure 1d).
The initial microcirculatory perfusion failure of 40±4% of the chamber surface at day 1 led to necrosis of 50±2% at day 10 in animals equipped with untreated flaps. Exclusive EPO administration showed already at day 1 a significantly decreased microcirculatory perfusion failure, which was associated with a reduction of the non-perfused tissue area of 13±1% (P<0.05 vs untreated flap) and tissue necrosis of 16±2% at day 10 (P<0.05) (Figure 1e). Microcirculatory dysfunction following coadministration of EPO and L-Name was comparable with that of untreated flaps, whereas application of L-Name alone further deteriorated tissue survival when compared with untreated flaps (P<0.05) (Figure 1e). It is interesting that flaps treated with EPO and bevacizumab did not show any change in tissue necrosis when compared with animals receiving EPO only (Figure 1f). Nonischemic controls, for example, mice undergoing chamber preparation without flap surgery did not develop necrosis (Figure 1f).
Arteriolar Perfusion
Red blood cell velocity slightly increased in all animals during the 10-day observation period (Figure 2a). Administration of EPO, as well as coadministration of EPO and bevacizumab led to an arteriolar dilation (Figures 2b and c), whereas all other groups did not show any change in arteriolar diameter, including nonischemic controls (Figures 2b and c). As a consequence, exclusive EPO administration resulted in a significantly increased arteriolar blood flow already briefly after surgery, which further increased during the observation period when compared with untreated flaps, animals receiving L-Name with or without EPO (Figure 2d) and nonischemic chambers (data not shown).
eNOS Expression
Administration of EPO led to a threefold increase of eNOS expression at day 1 and a twofold increase at days 3 and 5 after surgery (that is, induction of ischemia) (P<0.05) (Figures 3b and d), whereas untreated flaps and mice receiving the combination of EPO and L-Name did not show any increase of protein expression when compared with baseline (day 0) (Figures 3a, c and d). Accordingly, diameter augmentation of arteriovenular bundles was observed in animals receiving EPO only (Figure 3d), whereas both untreated flaps and mice administered with L-Name did not develop any noticeable morphological changes in diameter neither in arterioles nor in venules (Figures 3e and f).
Capillary Perfusion
Functional capillary density within the proximal and central area of the chamber preparation was significantly reduced already at day 1 after surgery in all animals receiving L-Name (L-Name, EPO and L-Name) (P<0.05 vs untreated flaps; Table 1), whereas administration of EPO was associated with a significantly increased number of perfused capillaries. In the distal area, FCD was maintained over the 10-day observation period only in the EPO group, whereas all other groups with flaps revealed complete cessation of FCD from day 3 onwards. It is interesting that FCD within the surviving proximal and central flap area of animals receiving EPO only was comparable with FCD observed in corresponding chamber areas of nonischemic controls (Table 1).
Vascular Remodeling, Angiogenesis and Macromolecular Leakage
Vascular remodeling with dilation and increased tortuosity of the microvessels was observed in all experimental groups undergoing flap preparation (Figures 4a, b, d and e). Administration of EPO induced angiogenesis, which was completely abrogated by additional administration of bevacizumab (Figure 4i). The new functional microvascular networks that usually develop from microvascular buds and sprouts were first visible at day 5 (Figures 4b, c and g). Angiogenesis was observed in all animals receiving EPO, regardless of coadministration of L-Name (Figures 4b and c), but not in untreated flaps or in mice receiving L-Name only (Figure 4a, d, g and i). Significant macromolecular leakage, that is, microvascular permeability of capillaries was observed from day 1 onwards and persisted over the entire 10-day observation period in all experimental groups undergoing treatment, that is, EPO, EPO and L-Name, and L-Name. Microvascular permeability was particularly increased if EPO was administered, whereas untreated flaps showed less microvascular leakage, but considerably more than nonischemic chambers (Figures 5a and b; Table 2).
VEGF Expression
The expression of VEGF was time dependent in both groups (untreated flaps and EPO). Although the baseline expression of VEGF was comparable in untreated flaps and mice administered with EPO only, the increased expression at day 3 after surgery was more pronounced and became significant from day 5 onwards in animals administered with EPO (Figure 4h).
Apoptotic Cell Death
Induction of persistent ischemia after acute injury in untreated flaps and animals receiving L-Name only was associated with a considerable number of apoptotic cell death at days 1, 3 and 5 showing one of the characteristic signs, that is nuclear condensation (Figures 6a, b and e). EPO administration significantly decreased cellular apoptosis to a level that was comparable with the surgery-induced apoptotic cell death observed in nonischemic chambers also, if L-Name was coadministered with EPO (P<0.05 vs untreated flap).
DISCUSSION
This study shows that administration of EPO before and after induction of ischemia in musculocutaneous tissue subjected to persistent ischemia is capable of attenuating ischemia-induced tissue injury by modulating microcirculatory properties. This protective effect seems to be predominantly caused by microvascular dilation mediated by the NO-releasing enzyme eNOS. This guarantees sufficient capillary perfusion of the tissue jeopardized by ischemia and results in a significant reduction of tissue necrosis. VEGF-associated formation of new functional capillaries does not seem to have a role in EPO-mediated tissue protection, whereas prevention of apoptotic cell death might occur for some protection in this model.
Induction of ischemia, that is, surgical preparation, caused a microvascular breakdown that resulted in tissue necrosis of ∼50% at day 10 in untreated animals. Three administrations of recombinant human EPO starting at 30 min before surgery significantly improved tissue survival. This was the consequence of an increased dilation of feeding arterioles mediated by an early upregulation of eNOS, which resulted in sustained capillary perfusion. Coadministration of the unspecific NOS antagonist L-Name completely overruled this dilatory response in arterioles and annihilated EPO-mediated tissue protection. This is in line with a previous study that showed that EPO induced basal vasodilation in rHuEPO hypertensive rats in an eNOS-dependent manner.25 This protective effect was completely abolished after additional administration of L-Name increasing blood pressure and total peripheral resistance. In muscle tissue it was shown that a single dose of 5000 IU EPO per kg bw, notably, a 10 × higher dose than the one used in this study, was able to attenuate ischemia/reperfusion injury by increasing NO bioavailability mediated by upregulation of eNOS.10 Further, this single dose of EPO administered before induction of ischemia has shown to induce eNOS, which was associated with a significantly attenuated ischemia-mediated capillary perfusion failure in musculocutaneous tissue despite an absence of arteriolar dilation. The fact that microscopic observation was limited to 5 h, no conclusion concerning tissue survival could be drawn.25 In addition, EPO was capable of preventing hypertension by inducing a dilatory effect through upregulation of the vascular expression of eNOS in rats.26 In this study, exclusive administration of L-Name actually increased tissue necrosis by about 10% to ∼60%, indicating an abrogation of ischemia-induced NO supply, that is, endogenous protection.
Erythropoietin has an important role in the induction of post-ischemic VEGF-mediated angiogenesis, as seen in the ischemic muscle.27, 28 An improvement of myocardial remodeling and function following EPO treatment after infarction was shown,28 and a crucial role for the vascular EPO receptor system in angiogenesis in response to critical hindlimb ischemia mediated through an upregulation of VEGF/VEGF receptor system was shown.27 Moreover, EPO was able to stimulate normal endothelial progenitor cell-mediated endothelial turnover, but the effect on cardiac microvascularization and function was only seen in the presence of ischemia.29 This is in line with our results that show a formation of new microvessels in critically ischemic tissue in all animals with administered EPO independently from coadministration of L-Name, which suggests an EPO-mediated angiogenic response under hypoxic conditions. Animals that simultaneously received EPO and bevacizumab showed a complete abrogation of the EPO-induced angiogenic response without affecting the EPO-mediated tissue protection. This indicates the following: (1) The formation of new functional capillary networks is VEGF driven, as the VEGF antibody bevacizumab prevents from the angiogenic response. (2) The angiogenic response is not involved in EPO-mediated survival of musculocutaneous tissue, most probably because the development of microvessels occurs from days 5–7 onwards. This is in contrast with Galeano et al30 who demonstrated in a murine model of thermal injury that EPO-mediated angiogenesis resulted in significantly improved wound healing if the drug was administered on a daily base for a time period of 14 days. Interestingly, ischemia alone without the administration of EPO (untreated flaps and L-Name) was not able to induce angiogenesis, which indicates that the new functional microvessels in this model only develop in the presence of EPO.
Macromolecular leakage increased significantly after the administration of EPO, as well as L-Name. This may be the result of an overexpression of VEGF-mediating hyperpermeability of microvessels with regard to ischemia-induced microvascular injury. VEGF has previously been shown to induce vascular hyperpermeability in therapeutic angiogenesis.31 Further, significant macromolecular leakage has also been associated with increased VEGF protein content and mRNA concentration in hypoxic brain tissue.32 In addition, enhanced albumin leakage has been observed in post-capillary venules of the mesentery33 and visceral organs,34 after the administration of L-Name, which indicates that endogenous NO may contribute to microvascular integrity during surgery and ischemia-induced tissue injury.
Several studies have attested EPO anti-apoptotic properties in traumatic, ischemic and toxic injury in a multitude of organs, such as the skeletal muscle,35 liver36 and kidney.11 Our results showed that administration of EPO significantly decreased the number of apoptotic cells when compared with untreated flaps and animals receiving L-Name only. This is in line with a previous study of our group, in which we could show that apoptotic cell death was significantly reduced even if EPO was administered only after flap elevation. Tissue survival, however, was not affected when compared with untreated flaps, suggesting that EPO-mediated reduction of apoptotic cell death was not sufficient to protect ischemically challenged tissue if microvascular perfusion was not maintained, which was the case in animals receiving EPO only after surgery.37 These experiments show that a triplicate coadministration of EPO and L-Name before and after surgery is able to counteract tissue necrosis mediated by L-Name by ∼20%, in spite of comparable microvascular parameters, that is, arteriolar dilation and arteriolar blood flow. This indicates that reduction of apoptotic cell death mediated by EPO may account for some protection that is not dependent on microvascular blood flow. This observation is in line with EPO administration that reduced apoptotic cell death and recovery of the impaired microcirculation following ischemia-reperfusion injury of the intestine,38 liver36 and testes.39 This indicates that a reduced apoptotic cell death contributing to final tissue survival is most probably dependent on ischemia followed by reperfusion.
In conclusion, this study shows that a triplicate administration of 500 IU per kg bw EPO started before surgery, that is, induction of ischemia prevents musculocutaneous tissue from necrosis. This can be attributed to an eNOS-dependent vasodilatory response in the arterioles, which maintains the capillary perfusion of the ischemically jeopardized tissue. The protection provided by EPO is almost completely abrogated with concomitant application of L-Name. However, coadministration of EPO and bevacizumab does not affect tissue survival despite complete inhibition of angiogenesis, which suggests that the EPO-mediated angiogenic response is not effective for tissue survival. EPO-mediated anti-apoptotic properties may contribute to tissue survival as long as EPO is administered before induction of ischemia. Altogether, EPO seems to be an up-and-coming approach to pharmacologically influence ischemically challenged tissue.
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Acknowledgements
The authors thank Janine Becker (Institute for Clinical & Experimental Surgery, University of Saarland, D-66421 Homburg/Saar, Germany) for excellent technical assistance, and Anton Haselbeck (Roche Diagnostics GmbH, Penzberg, Germany) and Pierre-Alain Delley (Roche Pharma Schweiz, Reinach, Switzerland) for the drug supply. This study was financially supported by the Swiss National Science Foundation (SNF-No. 3200BO-108408).
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The authors declare no conflict of interest.
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Rezaeian, F., Wettstein, R., Egger, JF. et al. Erythropoietin-induced upregulation of endothelial nitric oxide synthase but not vascular endothelial growth factor prevents musculocutaneous tissue from ischemic damage. Lab Invest 90, 40–51 (2010). https://doi.org/10.1038/labinvest.2009.117
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DOI: https://doi.org/10.1038/labinvest.2009.117
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