Abstract
Aims/hypothesis
Diabetes results in the upregulation of the production of several components of the inflammatory response in the retina, including inducible nitric oxide synthase (iNOS). The aim of this study was to investigate the role of iNOS in the pathogenesis of the early stages of diabetic retinopathy using iNOS-deficient mice (iNos −/−).
Materials and methods
iNos −/− mice and wild-type (WT; C57BL/6J) mice were made diabetic with streptozotocin or kept as non-diabetic controls. Mice were killed at different time points after the induction of diabetes for assessment of vascular histopathology, cell loss in the ganglion cell layer (GCL), retinal thickness, and biochemical and physiological abnormalities.
Results
The concentrations of nitric oxide, nitration of proteins, poly(ADP-ribose) (PAR)-modified proteins, endothelial nitric oxide synthase, prostaglandin E2, superoxide and leucostasis were significantly (p < 0.05) increased in retinas of WT mice diabetic for 2 months compared with non-diabetic WT mice. All of these abnormalities except PAR-modified proteins in retinas were inhibited (p < 0.05) in diabetic iNos −/− mice. The number of acellular capillaries and pericyte ghosts was significantly increased in retinas from WT mice diabetic for 9 months compared with non-diabetic WT controls, these increases being significantly inhibited in diabetic iNos −/− mice (p < 0.05 for all). Retinas from WT diabetic mice were significantly thinner than those from their non-diabetic controls, whereas diabetic iNos −/− mice were protected from this abnormality. We found no evidence of cell loss in the GCL of diabetic WT or iNos −/− mice. Deletion of iNos had no beneficial effect on diabetes-induced abnormalities on the electroretinogram.
Conclusions/interpretation
We demonstrate that the inflammatory enzyme iNOS plays an important role in the pathogenesis of vascular lesions characteristic of the early stages of diabetic retinopathy in mice.
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Introduction
Excessive production of nitric oxide is thought to play a role in inflammatory diseases (reviewed in [1]). Nitric oxide is generated from l-arginine by the catalytic reaction of different isoforms of nitric oxide synthase (NOS), including neuronal NOS (nNOS), endothelial NOS (eNOS) and inducible NOS (iNOS). Normal functions of nitric oxide include regulation of vessel tone, but it can also react with superoxide anion to form peroxynitrite, which can damage proteins, lipid and DNA. It is believed that the relatively smaller amount of nitric oxide generated by eNOS and nNOS are involved in physiological functions, whereas the comparatively larger amount of nitric oxide generated by iNOS is involved in inflammatory diseases [1, 2].
Diabetes results in upregulation of a number of components of the inflammatory response in the retina. Upregulation of iNOS level has been found in retinas of experimental diabetic rodents and human patients in most studies [3–6]. The significance of this enzyme in the development of diabetic retinopathy has not yet been defined, but increased production of nitric oxide is at least closely associated with the development of retinopathy. A possible role of iNOS in this is suggested by studies of aminoguanidine. Aminoguanidine is a relatively selective inhibitor of iNOS [7] and has been found to inhibit the diabetes-induced increase in iNOS levels and nitric oxide production in retina [4]. Importantly, aminoguanidine has also been found to inhibit development of the microvascular lesions of diabetic retinopathy in diabetic dogs [8], rats [9, 10] and mice (T. S. Kern, unpublished data). However, results from these aminoguanidine studies did not suffice to prove that iNOS plays a critical role in diabetes-induced retinal pathology, since aminoguanidine has also been shown to inhibit dicarbonyl-mediated cross-linking and protein modification [11] and can even inhibit eNOS level under some circumstances [12]. Thus, to investigate the role of iNOS in the pathogenesis of diabetic retinopathy, we studied diabetic mice that are deficient in iNos.
Materials and methods
Streptozotocin-induced model of diabetes
Breeder pairs of iNos −/− mice along with wild-type mice (WT; C57BL/6J) were purchased from Jackson laboratories (Bar Harbor, ME, USA). Offspring of iNos −/− and WT mice were housed in ventilated microisolator cages. All experiments followed the guidelines set forth by the Association for Research in Vision and Ophthalmology Resolution on Treatment of Animals in Research. Insulin-deficient diabetes was induced in fasted mice by intraperitioneal injections of streptozotocin (55 mg/kg body weight) on 3–5 consecutive days. Insulin was given as needed to maintain body weight and allow a slow increase in body weight while allowing hyperglycaemia, polyuria and hyperphagia (0–0.2 U every 2–3 days). Hyperglycaemia was quantified every 2–3 months by measuring total glycated haemoglobin levels (Variant II total GHb Program; BioRad, Hercules, CA, USA) and by measuring blood glucose concentrations. Diabetic and age-matched non-diabetic controls were killed at 6 and 9 months of diabetes for assessment of vascular histopathology and at 2–4 months of diabetes for assessment of cell loss in the ganglion cell layer (GCL), as well as biochemical and physiological abnormalities.
Measurement of nitric oxide
Nitric oxide was determined in retina by measuring the stable metabolites of nitric oxide (nitrate+nitrite) using a fluorimetric assay kit (Cayman Chemical, Ann Arbor, MI, USA) as reported previously [4, 13, 14].
Estimation of superoxide anion
The assay was performed as previously reported [15]. Briefly, freshly isolated retinas from mice were first equilibrated in Krebs–HEPES buffer in the dark at 37°C in 95% O2/5% CO2 for 30 min. After incubation, 0.5 mmol/l lucigenin was added and luminescence was detected. Generation of luminescence can be inhibited with Tiron, a cell membrane permeable scavenger of superoxide anion, suggesting the reaction provides a reasonable estimate of superoxide production.
Western blot analysis
Rat retinas were isolated and sonicated. Total amount of protein was determined by a protein assay (BioRad). Proteins were separated by SDS-PAGE and antibodies for nitrotyrosine (Upstate Biotechnology, Lake Placid, NY, USA), eNOS (BD Biosciences, San Jose, CA, USA) and poly(ADP-ribose) (PAR) (Axxora LLC, San Diego, CA, USA) were applied. After extensive washing, protein bands detected by the antibody were visualised by enhanced chemiluminescence (Santa Cruz Biotechnology, Santa Cruz, CA, USA). Membrane was then stripped and re-probed with antibody against β-actin (Sigma, St Louis, MO, USA) to confirm equal protein loading. The films were subsequently scanned and band intensity was quantitated using a software package (Quantity One 1-D Analysis; BioRad).
Measurement of prostaglandin E2
Prostaglandin E2 (PGE2) in homogenised samples of retina was measured by ELISA using a commercial kit (Cayman Chemical) as previously reported [13]. All assays were done in duplicate and at two different dilutions of homogenate. The amount of PGE2 in the retina was normalised by the total amount of protein in the corresponding retinal extracts and the PGE2 content of each sample calculated as pg/mg protein.
Quantitative measurement of leucostasis
At 3 months of diabetes, blood was removed from the vasculature of anaesthetised animals (ketamine 100 mg/ml:xylazine 100 mg/ml = 5:1) by complete perfusion with PBS via a heart catheter. Animals were then perfused with fluorescein-coupled concanavalin A lectin (20 μg/ml in PBS; Vector Laboratories, Burlingame, CA, USA) as described previously [16, 17]. Flat-mounted retinas were imaged via fluorescence microscopy and the number of leucocytes adherent to the vascular wall was counted.
Quantification of vascular histopathology
The retinal vasculature was isolated by the trypsin digest method as described by us previously [8, 17]. Briefly, freshly isolated eyes were fixed with buffered formalin (4% [wt/vol.] formaldehyde, 0.075 mol/l sodium phosphate buffer). Retinas were isolated, washed in water overnight and then incubated with 3% Difco crude typsin (BD, Sparks, MD, USA) at 37°C for 1 h. Non-vascular cells were gently brushed away from the vasculature, the isolated vasculature was mounted on glass slides, air-dried and stained with periodic acid–Schiff and haematoxylin (PASH). Acellular capillaries were quantified in six to eight field areas in the mid-retina (×400 magnification) in a masked manner. Acellular capillaries were identified as capillary-sized vessel tubes having no nuclei anywhere along their length and reported per square millimetre of retinal area. Tubes having a diameter <30% of the diameter of adjacent capillaries were identified as strands and not counted as acellular capillaries. Pericyte ghosts were estimated from the prevalence of spaces in the capillary basement membranes from which pericytes had disappeared. At least 1,000 capillary cells in seven field areas in the mid-retina (×400 magnification) were evaluated and the number of pericyte ghosts reported per 1,000 capillary cells.
Cell count and retinal thickness
The enucleated eyes were fixed in buffered formalin, embedded in paraffin and sectioned. To control for artefacts resulting from the sectioning angle, all sections were cut tangentially through pupil and optic nerve, thus ensuring an essentially tangential cut through the centre of the eye. The cross-sections were stained with PASH for retinal morphology examination. The nuclei in the GCL (not including nuclei of blood vessels in that layer) were counted and the thickness of various retinal layers measured in six locations in the retina (three locations on each side of the optic nerve) under ×400 magnification with Image-Pro 4.0 software (Media Cybernetics, Bethesda, MD, USA).
Electroretinogram
Measurements were made as described previously [18] with three to ten animals per group. Mice were adapted to the dark overnight, anaesthetised and placed on a heating pad during the recording session. Pupils were dilated with 1% (wt/vol.) tropicamide, 1% (wt/vol.) cyclopentalate hydrochloride and 2.5% (wt/vol.) phenylephrine hydrochloride. Recordings were made using a stainless steel wire loop that contacted the corneal surface through a thin layer of 1% (wt/vol.) methylcellulose. Needle electrodes placed in the tail and cheek served as ground and reference electrodes, respectively. Responses were amplified (1–1,000 Hz), averaged and stored on an UTAS signal averaging system (LKC Technologies, Gaithersbug, MD, USA). A darkness-adapted intensity–response series was recorded using a series of Ganzfeld flashes with intensities ranging from −4.2 to 0.5 log cd s/m−2. Cone electroretinograms (ERGs) were obtained to stimuli after 7 min light adaptation in which the animals were exposed to a steady rod desensitising background light of 0.8 log cd/m2 presented in the Ganzfeld bowl. Cone responses were elicited to a series of flash intensities (−0.22 to 0.52 log cd s/m−2). For each intensity, the average response to 25 flashes was calculated. The amplitude and latency of the ERG a- and b-wave were measured conventionally. For the a-wave, amplitude was measured from the pre-stimulus baseline to the trough. For the b-wave, amplitude was measured from the negative trough of the a-wave to b-wave peak. Latency or time-to-peak, was measured from stimulus onset to the a-wave trough and b-wave peak. Summed oscillatory potential values were calculated for as reported previously [19].
Statistical analysis
All results are expressed as the mean±SD. ERG results across different light intensities were analysed by repeated measures ANOVA and oscillatory potential was analysed by ANOVA followed by the Fischer post hoc test. Other data were analysed by the nonparametric Kruskal–Wallis test followed by the Mann–Whitney U test. Differences were considered statistically significant when the p values were less than 0.05.
Results
Total GHb and blood glucose values in diabetic iNos −/− mice were not significantly different from those in diabetic WT mice and were significantly higher than corresponding values in non-diabetic mice (Table 1). Body weights of both groups of diabetic mice remained significantly lower than those of non-diabetic mice. All mice lacking iNos appeared healthy.
Previous work has demonstrated that diabetes can induce excessive nitric oxide production in retinas of diabetic rats and mice [3, 4, 20]. To investigate whether iNOS contributed to this nitric oxide production, we measured nitric oxide production (indicated by total of nitrite and nitrate, the stable metabolites of nitric oxide) in retinas of WT and iNos −/− mice that had diabetes for 3 months, as well as in retinas of their age-matched non-diabetic controls. As shown in Fig. 1a, diabetes in WT mice caused a modest (1.3-fold), but significant elevation of nitric oxide in retinas (p < 0.05 compared with non-diabetic WT controls); however, no such elevation was seen in the retinas of diabetic iNos −/− mice (p < 0.05 compared with diabetic WT) (Fig. 1a). Consistent with this observation, nitration of retinal proteins was increased in WT diabetic mice compared with non-diabetic WT mice (especially in proteins with molecular weights between 70 and 75 kDa, and about 25 kDa), while diabetic iNos −/− mice showed less protein nitration than diabetic WT mice (Fig. 1b). Intensity of all bands of nitrated proteins within the molecular weight range is summarised in Fig. 1c.
The eNOS level has also been reported to be elevated in the retinas of diabetic rats. It has been suggested that eNOS might play a role in the development of diabetes-induced leucostasis and/or diabetic retinopathy [21, 22]. In WT mice, diabetes of 2 months duration induced an approximately twofold increase in eNOS production in retinas (p < 0.05) (Fig. 2), whereas eNOS production in iNos −/− mice was not altered by diabetes.
Excessive production of nitric oxide via iNOS has been shown by many investigators to cause DNA breaks and subsequent activation of poly(ADP-ribose) polymerase (PARP) [23], suggesting that iNOS is upstream of PARP in those acute inflammatory models. Inasmuch as we previously have shown that PARP plays a critical role in the degeneration of retinal capillaries in diabetes [17], we sought to determine whether or not iNOS might be the cause of that PARP activation. In WT mice, diabetes caused an increase in the level of PARP activity (estimated from the amount of PAR-modified retinal proteins) (p < 0.05) (Fig. 3), but there was considerable variability among animals. Diabetic mice lacking iNos tended to have less PAR-modified retinal proteins, but the results did not achieve statistical significance.
The number of degenerate acellular capillaries, an important histological marker of early diabetic retinopathy, was significantly increased in retinas from WT mice that had been diabetic for 9 months (but not 6 months; not shown) compared with age-matched control mice (p < 0.01) (Fig. 4a). The diabetes-induced increase in these degenerate retinal capillaries was significantly inhibited in mice lacking iNos (p < 0.01). The number of pericyte ghosts, another histological marker of retinopathy, was also increased significantly in retinal vessels from diabetic WT mice compared with non-diabetic WT mice, an increase significantly inhibited in diabetic iNos −/− mice (p < 0.05 for both) (Fig. 4b). There was no statistically significant difference in the number of acellular capillaries or pericyte ghosts per retina between non-diabetic WT and non-diabetic iNos −/− mice.
Retinas from WT mice that had been diabetic for 3 to 4 months were significantly thinner than those from their non-diabetic controls (Table 2). Diabetes-induced retinal thinning achieved statistical significance in GCL, inner plexiform layer (IPL) and outer plexiform layer (OPL). However, there was no evidence of retinal thinning in diabetic iNos −/− mice. Neither diabetic WT nor iNos −/− mice showed evidence of cell loss in the GCL compared with their non-diabetic controls at this duration of study.
Prior studies of retinal cells exposed to elevated glucose have demonstrated: (1) that nitric oxide (especially that from iNOS) regulates production of PGE2, the inflammatory prostaglandin generated by cyclooxygenases [13]; and (2) that iNOS contributes to superoxide generation in macrophages [24]. Retinas from diabetic WT mice produced significantly more PGE2 (Fig. 5) and superoxide (Fig. 6) than did retinas from non-diabetic WT animals (p < 0.05 for both), while retinas from diabetic iNos −/− mice produced significantly less of both than did those from diabetic WT mice (p < 0.05 for both).
A diabetes-induced increase in leucostasis (leucocytes adhering to the luminal wall of the vasculature) has been postulated to contribute to endothelial cell death or dysfunction in the retina [25]. A significant increase in leucostasis was demonstrated in WT mice that had been diabetic for 3 months compared with their non-diabetic counterparts (p < 0.05) (Fig. 7). Leucostasis in diabetic iNos −/− mice was significantly less pronounced than that in diabetic WT mice (p < 0.05), demonstrating that iNOS contributes to the observed increase in retinal leucostasis in diabetes.
Diabetes-induced loss of retinal function was studied by ERG in WT and iNos −/− mice that had been diabetic for 6 months. Compared with WT non-diabetic mice, the amplitudes of a-waves (dark-adapted) and b-waves of ERG (dark- and light-adapted) were reduced in diabetic WT mice (p < 0.001 for all). Wave latencies were not significantly altered by diabetes in the WT animals. Dark-adapted a-wave amplitude in both non-diabetic and diabetic iNos −/− mice was significantly less pronounced than in the respective WT controls (p < 0.05; data not shown). The iNos −/− diabetic mice differed from the non-diabetic iNos −/− controls only with respect to dark-adapted b-wave amplitude (p < 0.01) (Fig. 8), where the iNos −/− diabetic mice had a lower amplitude than the WT non-diabetic and iNos −/− non-diabetic mice. Taken together, the data suggested that iNos deficiency did not prevent a diabetes-induced loss of dark-adapted amplitudes. Oscillatory potential was significantly different between: (1) WT diabetic and non-diabetic mice with respect to dark-adapted amplitude (587.5 ± 195.8 vs 847.7 ± 182.8 μV) and light-adapted latency (208.1 ± 26.0 vs 170.2 ± 28.5 ms); and (2) iNos −/− diabetic and non-diabetic mice with respect to dark-adapted amplitude (337.7 ± 57.1 vs 751.1 ± 309.7 μV) and light-adapted amplitude (195.5 ± 23.9 vs 166.1 ± 32.2 μV) (p < 0.05 for all). No significant differences were observed between WT diabetic and iNos −/− diabetic mice.
Discussion
The present studies use iNos −/− mice to demonstrate that iNOS plays an important role in the pathogenesis of the vascular lesions of diabetic retinopathy. We found that mice lacking iNos were protected from the diabetes-induced production of nitric oxide, nitration of retinal proteins and, importantly, from the diabetes-induced degeneration of retinal capillaries. Previous research has demonstrated that inhibition of iNOS or iNos deficiency also inhibits development of early functional alterations in retinal oxygenation in diabetes [26, 27].
Retinal thinning has been found in the inner retina of diabetic rats and human patients [28]. In the present diabetic WT mice, we observed that thinning was due to thinning of the IPL and OPL. Since these plexiform layers represent interconnections between neurons, diabetes-induced reductions in synaptic connections [29] probably contribute to this thinning. Mice lacking iNos in our study did not show the diabetes-induced thinning of the retina, suggesting that the retinal thinning observed in our diabetic WT mice was due in part to iNOS or nitric oxide-mediated shrinkage or retraction of cell processes. Diabetes-induced retinal thinning has also been attributed, at least in part, to loss of retinal ganglion cells [28, 30–32]. However, our studies showed retinal thinning to occur although there was an apparent absence of cell loss in the GCL. The apparent lack of cell loss from the GCL of diabetic WT (C57BL/6J) mice is consistent with prior studies by us and others [33, 34], but is in contrast to another report using the same strain of mouse, where a 20% to 25% loss of cells in the GCL was observed after only 14 weeks of diabetes [35]. A 23% loss of cell bodies in the GCL from another mouse strain (Ins2Akita mice) has been detected at 22 weeks of diabetes [36].
Diabetes-induced alterations in retinal thickness and structure might be expected to result in altered retinal function. Diabetes resulted in reduction of the ERG amplitudes of a- and b-waves in WT mice, but the absence of iNOS did not prevent diabetes-induced retinal dysfunction. Apparently, this retinal dysfunction in diabetic mice is not caused by iNOS-mediated generation of nitric oxide.
Production of large quantities of nitric oxide can inhibit key enzymes in the mitochondrial electron transport chain and citric acid cycle by nitrosylation of reactive groups essential for enzyme catalytic function [37–39]. In addition, nitric oxide directly contributes to tissue damage by combining with superoxide to form peroxynitrite, a highly reactive species that produces lipid peroxidation, mitochondrial and DNA damage, and enzyme and protein inactivation. Levels of nitrotyrosine are a marker of peroxynitrite generation and reaction. iNOS is known to contribute to superoxide production [24], while deficiency of iNos results in less generation of superoxide anion by retina, both in diabetes (Fig. 6) and in experimental galactosaemia (another model of diabetic-like retinopathy) [40]. Besides its role in peroxynitrite formation, superoxide also has other independent effects, including oxidation of retinal proteins, potentially altering activity or turnover of the proteins and contributing to cell death [41, 42]. In the present study, we found that the formation of nitric oxide, nitrotyrosine and superoxide was reduced in diabetic mice lacking iNos, thus probably contributing to the observed resistance of retinal capillaries from these animals to the process of degeneration in diabetes.
Nitric oxide can also contribute indirectly to cell damage. The increased production of nitric oxide induced by elevated glucose in retinal Müller cells and endothelial cells increased production of prostaglandins (via cyclooxygenase-2) and cell death [13]. Inhibition of NOS in retinal cells incubated in concentrations of glucose similar to those in diabetes prevented PGE2 production and cell death, suggesting that nitric oxide regulates cyclooxygenase activity and production of cytotoxic prostaglandins in retinal cells [13]. Findings in the present in vivo study, where retinas from diabetic iNos −/− mice generated less PGE2 than did retinas from diabetic WT mice, are consistent with this interpretation.
Whether or not iNOS is present in vascular cells of the retina in diabetes is controversial. In some studies, iNOS has been detected in retinal capillary endothelial cells in hyperglycaemia [6, 40], whereas others have not detected it [4, 5, 43]. iNOS-mediated degeneration of retinal capillaries in diabetes is probably not initiated in capillary pericytes, since high glucose has been reported to decrease iNOS expression in retinal pericytes [44]. It remains possible that the iNOS-mediated degeneration of retinal capillary cells in diabetes might be secondary to nitric oxide-mediated damage in nearby nonvascular cell types.
In diabetic rats, we found that a specific inhibitor of PARP inhibited the diabetes-induced upregulation of iNOS production in retinas (L. Zheng, T. S. Kern, unpublished data), suggesting that iNOS upregulation was secondary to PARP activation. In contrast, many investigators studying other disease models have found that iNOS-mediated generation of peroxynitrite causes PARP activation via induction of DNA strand breaks [23]. In retinas of our diabetic mice, PARP activation seemed to be less pronounced in diabetic iNos −/− mice than in diabetic WT mice, but the results did not achieve statistical significance. In the retina in diabetes, iNOS levels apparently are regulated by PARP activation and also influences the activation of PARP.
eNOS and nNOS have also been found elevated in the retinas of diabetic rats. It has also been suggested that eNOS and nNOS levels are associated with leucostasis and/or increased retinal vascular permeability, as well as being involved in the development of diabetic retinopathy [21, 22, 45, 46]. Investigation of the role of eNOS in the development of retinopathy remains difficult because of confounding by other important actions of this isoform, e.g. blood pressure regulation [47]. In this study, diabetes did not increase expression of eNOS in the retina of iNos-deficient animals, suggesting that iNOS somehow regulates eNOS level. It remains possible that the observed benefits of iNOS inhibition for the development of retinopathy might occur in part via normalisation of eNOS.
The present demonstration of a critical role of iNOS in the pathogenesis of diabetic retinopathy provides further support for the postulate that diabetic retinopathy develops via an inflammation-like process. A working hypothesis of how iNOS is involved in the development of diabetic retinopathy is summarised in Fig. 9. Inappropriate regulation of nuclear factor kappa B (NF-κB) DNA binding has been observed in the retina in diabetes [17, 48–50], resulting in increased transcription of NF-κB-regulated gene products, including iNOS [51]. Inhibition of inflammatory pathways via inhibition of PARP [17], NF-κB [51], cyclooxygenase [52], intercellular adhesion molecule-1 [16] and now also of iNOS inhibits the diabetes-induced degeneration of retinal capillaries in experimental diabetic animals. Evidence that iNOS plays a critical role in the early stages of diabetic retinopathy points to another therapeutic target for the potential inhibition of this disease.
Abbreviations
- eNOS:
-
endothelial nitric oxide synthase
- ERG:
-
electroretinogram
- GCL:
-
ganglion cell layer
- iNOS:
-
inducible nitric oxide synthase
- IPL:
-
inner plexiform layer
- NF-κB:
-
nuclear factor kappa B
- NOS:
-
nitric oxide synthase
- nNOS:
-
neuronal nitric oxide synthase
- OPL:
-
outer plexiform layer
- PAR:
-
poly(ADP-ribose)
- PARP:
-
poly(ADP-ribose) polymerase
- PASH:
-
periodic acid–Schiff and haematoxylin
- PGE2 :
-
prostaglandin E2
- WT:
-
wild-type
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Acknowledgements
This work was supported by grants from the Medical Research Service of the Department of Veteran Affairs and National Institutes of Health (R01EY00300) to T. S. Kern, from the Juvenile Diabetes Research Foundation and National Institutes of Health (R01EY013831) to B. A. Berkowitz, and the Diabetes Association of Greater Cleveland (fellowship grant) to L. Zheng. Technical help from R. Roberts is greatly appreciated. Histology service was provided by the Case Western Reserve University Visual Science Research Center Core Facilities (P30EY11373).
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An erratum to this article can be found at http://dx.doi.org/10.1007/s00125-007-0772-3
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Zheng, L., Du, Y., Miller, C. et al. Critical role of inducible nitric oxide synthase in degeneration of retinal capillaries in mice with streptozotocin-induced diabetes. Diabetologia 50, 1987–1996 (2007). https://doi.org/10.1007/s00125-007-0734-9
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DOI: https://doi.org/10.1007/s00125-007-0734-9