Abstract
Unilateral hypoxia–ischemia (HI) was induced in C57/BL6 male mice on postnatal day (P) 5, 9, 21 and 60, corresponding developmentally to premature, term, juvenile and adult human brains, respectively. HI duration was adjusted to obtain a similar extent of brain injury at all ages. Apoptotic mechanisms (nuclear translocation of apoptosis-inducing factor, cytochrome c release and caspase-3 activation) were several-fold more pronounced in immature than in juvenile and adult brains. Necrosis-related calpain activation was similar at all ages. The CA1 subfield shifted from apoptosis-related neuronal death at P5 and P9 to necrosis-related calpain activation at P21 and P60. Oxidative stress (nitrotyrosine formation) was also similar at all ages. Autophagy, as judged by the autophagosome-related marker LC-3 II, was more pronounced in adult brains. To our knowledge, this is the first report demonstrating developmental regulation of AIF-mediated cell death as well as involvement of autophagy in a model of brain injury.
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Introduction
The extent of hypoxic–ischemic (HI) injury depends on the degree of maturation of the brain as well as on the severity and duration of the insult.1, 2, 3, 4, 5, 6, 7 It is generally accepted that neurons in the immature brain tolerate a longer period of oxygen deprivation and/or ischemia than those in the adult brain.1, 3 However, there are conflicting reports, showing that the immature brain is less resistant to HI brain damage than its adult counterpart.4 This is supported by other studies after HI or excitotoxic injury.8, 9 Furthermore, clinical data suggest that outcome and mortality after acute brain injury are age dependent, with more severe injuries in infants than in adults.8, 10
Cell death is usually classified as apoptotic or necrotic based on biochemical and morphological criteria,11, 12 even though recent data suggest that mixed morphological phenotypes are frequently observed after ischemic insults.12, 13, 14 Necrotic cell death is a pathological process resulting from tissue damage and loss of energy. Apoptosis is a genetically controlled cell death that was initially recognized for its role in development. In some brain regions, more than half of the neurons die by apoptosis during brain development.15 Many apoptosis-related factors have been demonstrated to be upregulated in the immature brain, such as caspase-3, Apaf-1, Bcl-2 and Bax.16, 17, 18, 19 Activation of apoptotic mechanisms contributes to the pathogenesis of brain damage in acute neuropathological disorders, such as HI, particularly in the immature brain.1, 14, 16, 20, 21, 22, 23, 24, 25 Autophagy is another type of cell death mechanism with distinct morphological features whereby lysosome-mediated engulfment of injured cells or cellular fragments can occur.26 It seems clear that, depending on the developmental level of the brain at the time of injury, different cell types and regions will be injured, at different rates, and different mechanisms of injury will be activated.1, 3, 22, 27, 28 Understanding the nature of cell death after HI at different developmental stages is essential to be able to choose effective therapeutic targets,29, 30 and since these vary during development, prevention and treatment of brain injury need to be adjusted accordingly. To better understand the mechanisms and developmental variations of HI neuronal cell death, we developed a mouse model where a similar extent of injury could be achieved by adjusting the duration of the hypoxia time, thereby enabling us to study the relative contribution of different mechanisms at different ages. Specifically, we investigated caspase-dependent and caspase-independent apoptotic mechanisms as well as one marker of oxidative stress (NOS-dependent, peroxynitrite-mediated nitrotyrosine formation), necrosis-related activation of calpains and autophagy.
Results
HI brain injury
Similar tissue injury was seen in the cortex, striatum, hippocampus and thalamus in the ipsilateral hemisphere at all ages (Figure 1a). The nucleus habenularis (NH), however displayed a marked developmental change in its susceptibility to HI. The NH is very sensitive to HI in the immature brain,31 but this vulnerability decreased with age and the NH was resistant to HI in P60 mice (Figure 1b).The neuropathological score and tissue loss were virtually identical at P5, P9, P21 and P60 using the different durations of hypoxic exposure indicated in Materials and Methods (Figure 1c).
Apoptosis-inducing factor (AIF) translocation and cytochrome c (Cyt c) release from mitochondria after HI
The levels of AIF protein in mouse brain homogenates were virtually unchanged during normal brain development from P5 to P60 (Figure 2a). In the mitochondrial fraction, there was about 20% less AIF in the ipsilateral hemisphere compared with the contralateral hemisphere in P5 mice 24 h post-HI, indicating that this amount had been released. This AIF release was reduced to about 10% in juvenile and adult brains (Figure 2b). In tissue sections, AIF immunoreactivity was non-nuclear in normal neurons; however, in damaged brain areas, as judged by the loss of MAP-2, AIF was translocated from mitochondria to nuclei very early after HI, producing a distinct nuclear staining (Figure 2c), in agreement with our earlier findings in the neonatal rat brain after HI,32 in the adult mouse brain after focal ischemia33 and in progenitor cells of the developing brain after irradiation.34 The number of AIF-positive nuclei increased significantly at 3 h post-HI and reached a peak at 24 h after the insult in most regions of the immature brain, more pronounced in P5 mice (Figure 3). Significant, but much fewer, AIF-positive nuclei were observed in the mature mouse brain regions (except for the denate gyrus (DG)), especially in P60 mice. In the NH, the number of AIF-positive nuclei decreased dramatically with development reflecting the resistance to HI at P21 and P60 (Figure 3).
Another mitochondrial, proapoptotic protein, Cyt c, displayed an approximately two-fold increase during normal brain development (Figure 4a). It was released from mitochondria in the ipsilateral hemisphere after HI, more pronounced in the immature brain than in the adult brain (Figure 4b). In tissue sections, neuronal Cyt c staining was found to be more intense and distinct in the cytosol of damaged brain areas (Figure 4c), presumably indicating release of Cyt c from mitochondria, as demonstrated earlier.32, 33 Counting of cells with strong cytoplasmic Cyt c staining, revealed a pattern similar to that of AIF-positive nuclei, with higher numbers in the immature brains, but the total number of strongly Cyt c staining cells was smaller than that of AIF-positive nuclei (Figure 5).
Caspase-3 activation after HI
Caspase-3, the most abundant effector caspase in the immature brain, decreased dramatically with brain maturation (Figure 6a), displaying an inverse correlation with Cyt c, as demonstrated earlier in the rat brain.16, 32 The 32 kDa proform was cleaved and produced the calpain-dependent 29 kDa and the caspase-dependent active 17 kDa fragments after HI in the ipsilateral hemisphere in the immature brains. The cleavage products were difficult to detect in the juvenile and adult brains (Figure 6b). Using an antibody against the 17 kDa active form of caspase-3 on tissue sections, conspicuous staining was obtained in numerous neurons in MAP-2-negative areas in the immature brains (Figure 6c), and this staining has earlier been shown to colocalize with other markers of cellular injury.16, 21, 32 DEVDase assays showed that the caspase-3-like activity increased 31-fold in P5 and 25-fold in P9 mice 24 h post-HI, compared with the normal control brains (Figure 6b), consistent with when the peak of caspase-3 activation occurs in the neonatal rat brain after HI.16, 23 Caspase-3 activity increased about 40% in P21 and P60 mice, compared with the normal control brains (Figure 6d). Active caspase-3 staining in tissue sections increased at 3 h and reached a peak at 24 h post-HI in most regions in the immature and juvenile brains (P5, P9 and P21) (Figure 7). In the adult brains (P60), the caspase-3-positive cells appeared gradually and reached a peak at 72 h in all injured areas (Figure 7). The total number of active caspase-3-positive cells was lower in the juvenile and adult brains than in the immature brains, except for the CA3 (P21 and P60) and DG (P21) subfields of the hippocampus (Figure 7).
Calpain activation after HI
Calpain 1 did not change appreciably in the normal brains during development (Figure 8a), but after HI almost half of the calpain 1 was lost in the immature brains (Figure 8b), most likely as a result of activation and subsequent degradation.35 In the juvenile and adult brains, however, the loss was significantly lower, only about 5% in P60 mice (Figure 8b). Calpain 2 was not significantly regulated during development, except for a somewhat higher level in P5 mice (Figure 8c). About 20–30% of the calpain 2 protein was lost after HI, but there was no significant difference between ages (Figure 8d). Activation of calpains results in specific fodrin cleavage products, alpha-fodrin breakdown product (FBDP), of 145 and 150 kDa, relatively resistant to further degradation. FBDPs have been used extensively as markers of calpain activation, including after neonatal HI.16, 31, 35, 36, 37 In this study, FBDPs were prominent after HI at all ages (Figure 8e), unlike the caspase-dependent 120 kDa cleavage product, which was apparent only in P5 and P9 mice (Figure 8e). In tissue sections, an antibody specific for the n-terminal 145 kDa FBDP, produced strong staining in injured neurons early after HI (Figure 8f). FBDP-positive cells accumulated and reached a peak in injured and borderline regions ipsilaterally as early as 3 h post-HI in the cortex, striatum and NH of P5 mice (Figure 9). FBDP-positive cells appeared in a somewhat delayed fashion in P60 mice in those regions (Figure 9). In the hippocampus, especially in the CA1, unlike the cortex, very few FBDP-positive cells could be detected in P5 and P9 animals, but more positive cells were observed in P21 and P60 animals (Figure 9).
Nitrotyrosine formation after HI
Both nNOS and iNOS showed a similar developmental pattern, displaying approximately three-fold higher protein levels at P5 than P60 (Figure 10a and b). In tissue sections, NOS-dependent, peroxynitrite-mediated nitrotyrosine immunoreactivity was mainly located in the nuclei of injured cells (Figure 10c). The number of nitrotyrosine-positive cells increased immediately after HI and reached a peak around 8–24 h in most of the brain regions (Figure 11), as described earlier in the neonatal rat brain.38 The number of nitrotyrosine-positive cells did not vary appreciably between the different ages (Figure 11). The lack of staining in the NH reflected its resistance to HI, as in the case of all the other stainings. The only injured area that displayed a developmental difference was the DG, having fewer positive cells in the juvenile and adult brains (Figure 11).
Autophagy after HI
Immunoblots of homogenates using an antibody against microtubule-associated protein 1 light chain 3 (LC3) showed that LC3-I (16 kDa) was abundant in the brain. LC3-I is cytosolic, whereas LC3-II (14 kDa) is membrane-bound, and the amount of LC3-II is correlated with the extent of autophagosome formation.26 Both LC3-I and LC3-II could be detected in normal control brains, more pronounced in the immature brains, and both forms were significantly lower in normal adult brains (Figure 12a). After HI, LC3-II increased in the ipsilateral hemisphere, and this process appeared to peak 24–72 h after HI (data not shown). The relative increase of LC3-II in the ipsilateral hemisphere was more pronounced in the adult than the immature brain, approximately three-fold higher compared with normal controls, somewhat less compared with the contralateral hemispheres (Figure 12b).
Discussion
The influence of age on HI brain injury
The developing brain has been reported to be more resistant to certain insults than its adult counterparts.1, 3 The reason for increased susceptibility to injurious stimuli in older brains is often attributed to increased metabolic requirements once connectivity is complete.39 Other experimental studies question these conclusions.4, 8, 9, 40 McDonald et al.8 injected NMDA into the striatum of 7-day- and 3-month-old rats, producing 21 times larger damage in the younger animals than in the adults,8 which reflects the higher density of NMDA receptors in the developing brain. Similarly, Ikonomidou et al.9 demonstrated that the vulnerability to HI peaked at P6, and diminished thereafter. Yager et al., using male rats exposed to identical HI insults, demonstrated that brain damage was most severe in 1- and 3-week-old animals, followed by those that were 6 months old. The 6- and 9-week-old animals had significantly less injury than the other age groups.4 Our results are consistent with the apprehension that immature brains are considerably less susceptible to HI injury than mature ones. The two independent methods used to evaluate brain injury in this study have been shown to correlate well with each other.41, 42, 43 Our results showed that longer hypoxia times were required to obtain a similar degree of brain injury in the immature brains than in the older ones. Furthermore, in the immature brain, extensive atrophy was observed, that is, in addition to the acute loss of dead tissue, there was secondary loss of tissue because the acutely lost tissue could not support the further growth of the surrounding brain tissue. Using the different durations of hypoxia, both the extent and distribution of brain injury was very similar, with a couple of exceptions. The NH was virtually resistant to HI injury in P60 mice, whereas in the immature brain, this area is one of the first to display signs of tissue damage, such as loss of MAP-2. The CA1 has earlier been reported to be relatively resistant to HI in the immature brain, and the selective vulnerability of this subfield developed between P13 and P21 in rats.3 In the present study, the CA1 was injured at all ages; however, the mechanisms involved appeared to change dramatically between P5 and P21, shifting from mainly AIF translocation, Cyt c release and caspase-3 activation at P5, to mainly calpain activation at P21 and P60. It is clear that the vulnerability of the brain is strongly influenced by age, although the mechanisms behind these developmental changes are only partly understood.2, 9, 22, 44
The influence of age on cell death mechanisms
Activation of caspase-3 appears to be a critical event in the execution of neuronal apoptosis in the brain during development and after acute injury.1, 21, 23, 24, 25 In this study, we examined caspase-3 during normal development and after HI. We demonstrated that caspase-3 decreased dramatically during normal development of the mouse brain as judged by the basal activity and by immunoblotting, consistent with our previous reports from the rat brain.16, 23, 32 This developmental downregulation of caspase-3, as well as downregulation of other elements involved in caspase-3 activation, such as Apaf-1 and bax, occurs in parallel with the decline of physiological programmed cell death and may serve as a supplementary mechanism protecting the mature brain from apoptosis.17, 18, 40 Accordingly, caspase-3 activity increased dramatically after HI in the immature brain but increased only slightly in the mature brain. Immunostaining of active caspase-3 showed very few positive cells in most regions of the adult brain, indicating that caspase-3-mediated neuronal death does not play a major role in the mature brain after HI, in accordance with earlier findings.1, 27 In support of our findings, Pohl et al.45 found a marked decrease with age in the extent of distant, apoptosis-related cell death after traumatic brain injury.
Cyt c is an essential component of the respiratory chain, an ATP-generating system in the inner mitochondrial membrane. We found that the relative content of Cyt c increased during brain development, in agreement with earlier findings.32, 46 This fits with the increased energy requirement in the mature brain needed to maintain the elaborate network of axons and dendrites. Release of Cyt c from mitochondria as a consequence of HI has been detected by immunoblotting and immunohistochemistry.32, 47 In some of the affected cells, the staining was associated with DNA fragmentation suggesting apoptosis.32, 48 Other studies showed that loss of mitochondrial Cyt c was correlated with an increased production of reactive oxygen species by mitochondria, which may contribute to cellular damage.49, 50 In this study, there were fewer cells displaying increased cytoplasmic Cyt c staining in most regions of the mature brains than in the immature brains, indicating that Cyt c-related, caspase-3-dependent apoptotic cell death in the mature brain is not as prevalent as in the immature brain.
Caspases have been recognized as important mediators of apoptotic cell death after HI brain injury.24 However, caspase inhibition has typically resulted in limited neuronal protection.32, 51 This indicates that additional or caspase-independent pathways of neuronal cell death exist. AIF was identified as a major player in caspase-independent cell death.52 Genetic targeting of AIF abolished the first wave of apoptosis that is indispensable for early embryonic morphogenesis.53 The expression of AIF in the normal rat brain was reported to decrease slightly with development. However, the protein expression in the cerebellum was markedly increased, distinctively different from the mRNA expression.54 In the normal rat brain, not including the cerebellum, we found no changes of total AIF protein during the normal brain development.32 In this study, similar results were found using the mouse brain. So, the constant levels of AIF and increasing levels of mitochondrial markers demonstrated a relative downregulation of AIF with age.32 Mitochondrial release and nuclear translocation of AIF correlating with neuronal apoptotic cell death have been demonstrated in different brain injury models.32, 33, 54, 55, 56, 57, 58 In this study, the total number of AIF-positive nuclei decreased in all brain regions and at all the time points with increasing age after HI, indicating that AIF plays a more important role in the early development of neuronal apoptosis. Blocking AIF function with neutralizing antibodies provided significant protection against neuronal cell death.59 Downregulation of AIF by RNA interference could inhibit UVA-induced cell death60 and oxygen/glucose deprivation-induced death of primary cultured neurons (authors' unpublished observations). AIF also has a potent oxidoreductase function61 and the Harlequin mouse, expressing 80% lower levels of AIF, displayed increased amounts of hydroperoxides in the brain, cerebellum and heart.62 In summary, accumulating evidence suggests that AIF plays an important role both in normal development and under pathological conditions.
Calpains represent a class of cytosolic cysteine proteases activated by elevated intracellular calcium concentrations. Under pathological conditions, calpains have been implicated in excitotoxic neuronal injury and HI brain injury.16, 31, 35, 36, 37, 63, 64 Calpains are activated early in situations of energy depletion and increased calcium influx, triggering other downstream events leading to neurodegeneration. Calpains are generally considered to be activated during excitotoxic and other necrosis-related conditions.65 Fodrin is a well-known calpain substrate and detection of specific FBDP has been widely used to detect calpain activity.16, 36, 37, 63, 66, 67 In this study, FBDP-positive cells increased and reached a peak 3 h post-HI in the cortex, striatum and nucleus habenularis in the immature brain, probably indicating early, necrosis-related cell death. However, in the mature brain, the activation of calpains occurred later, as judged by the later-appearing FBDP, and remained on a high level even at 72 h postinsult, a time point by which there were almost no FBDP-positive cells left in any region of the immature brain. This may indicate sustained calpain activation resulting in lysosomal rupture, causing neuronal necrosis.68
Nitric oxide (NO) is produced by three isoforms of nitric oxide synthase (NOS). Inducible and neuronal NOS (iNOS and nNOS, respectively) activities have been demonstrated to increase in models of HI in the immature brain.69, 70, 71 Excessive NO produced after HI combines rapidly with superoxide to form the powerful oxidizing agent peroxynitrite (ONOO−). The ONOO− adduct is freely diffusible in its protonated form, oxidizes thiol groups, damages mitochondrial respiration and induces protein nitrosylation. Nitrosylation of tyrosine residues in proteins yields the compound 3-nitrotyrosine, and immunohistochemical detection of nitrotyrosine can be used as an indicator of peroxynitrite formation after HI.38 Pharmacological inhibition nNOS and iNOS reduced nitrotyrosine formation38 and was demonstrated to be neuroprotective.72 Oxidative stress, including production of NO and peroxynitrite, is considered to induce mainly necrotic cell death but may also be involved in apoptosis.73 The developing brain may be particularly vulnerable to oxidative damage because of its high concentrations of unsaturated fatty acids, high rate of oxygen consumption, low concentrations of antioxidants, and increased availability of ‘free’ redox-active iron.74 In this study, however, the extent of nitrotyrosine formation after HI was similar at all ages, despite downregulation of both nNOS and iNOS protein during development. Notably, the levels of iNOS were constitutively high in the immature brain even in naïve control animals.
Autophagy is a process responsible for the bulk degradation of intracellular material in double or multiple-membrane autophagic vesicles, and their delivery to and subsequent degradation by the cell's own lysosomal system. Just like the genetically controlled, physiological programmed cell death, autophagy was demonstrated to be more pronounced during embryonic development and tissue remodeling.75 One study suggests that autophagy is a caspase-independent, genetically controlled cell death.76 Visualization of autophagic vesicles by electron microscopy is still the golden standard to demonstrate that autophagy is taking place. The electrophoretic mobility change of LC3 from the nonautophagic, cytosolic form (LC3-I; 16 kDa) to the autophagic, membrane-recruited form (LC3-II; 14 kDa) provides the first molecular marker-based method for detection of autophagic activity.26, 77, 78, 79 The notion that autophagy is involved in tissue remodeling is in agreement with our finding that the basal levels of LC3-II in normal control animals was 2.5 times higher in the immature than in the adult brains. After HI, increased LC3-II levels were detected as early as 8 h, much more pronounced after 24 and 72 h. This indicates that autophagy is involved in delayed cell death. Notably, a recent EM study demonstrated numerous vacuoles in degenerating neurons after neonatal HI.80 Even though the basal levels of LC3-II were higher in the immature brains, the increase after HI was more pronounced in the adult brains. After HI, LC3-II levels increased about 2.5 times more in P60 animals than in P5 mice, comparing the ipsi- and contralateral hemispheres. The increase was even higher (more than three times) when comparing with the control brains instead of the contralateral hemispheres. Our results show for the first time that autophagy is involved in cell death after cerebral ischemia, and that the activation, as judged by the recruitment of LC3-II, was three times more pronounced in the adult brains compared with the immature brains.
In summary, the sensitivity of neurons, and various brain regions, to injury varies with the animal's age and level of brain development. By adjusting the duration of HI in different age groups, we could produce a similar extent of overall brain damage. The most obvious developmental difference in the response to HI was that apoptotic mechanisms, both caspase-dependent and caspase-independent, were activated to a much greater extent in the immature brains compared with the juvenile and adult brains. Despite the constant levels of AIF during brain development, mitochondrial release and nuclear translocation of AIF was much more pronounced in the immature than the juvenile and adult brains. To our knowledge, this is the first report of developmental differences in AIF activation in a model of brain injury. AIF, Cyt c and caspase-3 are more important in the immature brain than in older animals. Calpains and NO are both important in necrotic, and to some degree, apoptotic cell death, but displayed no obvious developmental differences. Autophagy, as judged by the recruitment of LC3-II, after HI was more pronounced in the adult than in the immature brain. Taken together, our findings offer additional support for the fact that prevention and treatment of brain injury need to be adjusted to the developmental level.
Materials and Methods
Induction of HI
Unilateral HI was induced in C57/BL6 male mice on postnatal day 5 (P5), P9, P21 and P60 essentially according to the Rice–Vannucci model.7, 81 Mice were anesthetized with halothane (3.0% for induction and 1.0–1.5% for maintenance) in a mixture of nitrous oxide and oxygen (1 : 1), and the duration of anesthesia was <5 min. The left common carotid artery was cut between double ligatures of prolene sutures (6-0). After surgery, the wounds were infiltrated with a local anesthetic, and the pups were allowed to recover for 1–1.5 h. The litters were placed in a chamber perfused with a humidified gas mixture (10% oxygen in nitrogen) for 65 min (P5), 60 min (P9), 50 min (P21) or 40 min (P60). The temperature in the incubator, and the temperature of the water used to humidify the gas mixture, was kept at 36°C. After hypoxic exposure, the pups were returned to their biological dams and were allowed to recover for 3, 8, 24 or 72 h. The injury was evaluated at 72 h post-HI through neuropathological scoring and measurement of tissue volume loss. Control pups, subjected to neither ligation nor hypoxia, were killed at postnatal day 5, 9, 21 or 60. All animal experimentation was approved by the Ethical Committee of Göteborg (94-2003).
Sample preparation for immunoblotting and activity assay
Animals were killed by decapitation 24 h after HI (n=5 for each age). Control animals were killed on postnatal day 6, 10, 22 or 61 (n=5 for each age). The brains were rapidly dissected out on a bed of ice. Parietal cortex was dissected out by first removing the frontal and occipital poles (approx. 2–3 mm) of the brain, and second, after positioning the brain with the occipital pole face down on the dissection tray, removing the diencephalon, the medial cortex and the ventrolateral (piriform) cortex, leaving an approximately 50 mg piece of parietal cortex. This piece was dissected out from each hemisphere and 9 volumes of ice-cold homogenization buffer was added (15 mM Tris-HCl, pH 7.6, 320 mM sucrose, 1 mM dithiothretitol, 1 mM MgCl2, 0.5% protease inhibitor cocktail (P8340, Sigma) and 3 mM EDTA-K). Homogenization was performed gently by hand in a 2-ml glass/glass homogenizer. Half of the homogenate was sonicated and used for Western blotting. The other half of the homogenate was centrifuged at 800 × g for 10 min at 4°C. The supernatant was then centrifuged at 9200 × g for 15 min at 4°C, producing a crude cytosolic fraction in the supernatant (S2), subsequently used for the caspase-3 activity assay. The pellet (P2), enriched in mitochondria, was washed, recentrifuged and used for Western blotting.
Immunohistochemistry
Mice were deeply anesthetized with 50 mg/ml phenobarbital and their brains were perfusion-fixed with 5% formaldehyde in 0.1 M phosphate buffer through the ascending aorta for 5 min. The brains were rapidly removed and immersion-fixed at 4°C for 24 h. The brains were dehydrated with xylene and graded ethanol, paraffin-embedded, serial-cut into 5 μm sections and mounted on glass slides. Antigen retrieval was performed by boiling deparaffinized sections in 10 mM sodium citrate buffer (pH 6.0) for 10 min. Nonspecific binding was blocked for 30 min with 4% horse serum (for MAP-2, Cyt c and AIF) or goat serum (for active caspase-3, fodrin breakdown product (FBDP) and nitrotyrosine) in phosphate-buffered saline (PBS). Anti-MAP-2 (clone HM-2, Sigma), diluted 1 : 2000 (4 μg/ml) in PBS, anti-Cyt c (clone 7H8.2C12, Pharmingen, San Diego, CA, USA), diluted 1 : 500 (2 μg/ml) in PBS, anti-AIF (sc-9416, from Santa Cruz Biotechnology, Santa Cruz, CA, USA), diluted 1 : 100 (2 μg/ml), antiactive caspase-3 (67342A, Pharmingen, San Diego, CA, USA), diluted 1 : 50 (10 μg/ml) in PBS, anti-FBDP82(1 : 50) and anti-nitrotyrosine (A-21285, Molecular probes, Eugene, OR, USA), diluted 1 : 100 (10 μg/ml) in PBS were incubated for 60 min at room temperature, followed by another 60 min with a biotinylated horse anti-mouse IgG (2 μg/ml) or horse anti-goat IgG (2 μg/ml) or goat anti-rabbit IgG (2 μg/ml) diluted in PBS. Endogenous peroxidase activity was blocked with 3% H2O2 in PBS for 5 min. Visualization was performed using Vectastain ABC Elite with 0.5 mg/ml 3,3′-diaminobenzidine (DAB) enhanced with 15 mg/ml ammonium nickel sulfate, 2 mg/ml beta-D-glucose, 0.4 mg/ml ammonium chloride and 0.01 mg/ml beta-glucose oxidase (Sigma).
Immunoblotting
The protein concentration was determined according to Whitaker and Granum83 adapted for microplates, using a Spectramax Plus plate reader (Molecular Devices, Sunnyvale, CA, USA). The samples were mixed with an equal volume of concentrated (3 ×) SDS-PAGE buffer and heated (96°C) for 5 min. Homogenates (50 μg protein) were run on 4–20% Tris-Glycine gels (Novex) and transferred to reinforced nitrocellulose (Schleicher & Schuell) membranes. The membranes were blocked in 30 mM Tris-HCl (pH 7.5), 100 mM NaCl and 0.1% Tween 20 (TBS-T) containing 5% fat-free milk powder for 60 min at room temperature. After washing in TBS-T, the membranes were incubated with anti-AIF (sc-9416, 1 : 1000, 0.2 μg/ml, goat polyclonal antibody, Santa Cruz, CA, USA), anti-caspase-3 (H-277, 1 : 1000, Santa Cruz, CA, USA), anti- Cyt c (1 : 500, clone 7H8.2C12, Pharmingen, San Diego, CA, USA), anti-calpain 1 (also called μ-calpain) (1 : 1000, 1 μg/ml, rabbit polyclonal antibody, RP1-calpain-1, Triple Point Biologics, Forest Grove, OR, USA), anti-calpain 2 (also called m-calpain) (1:1000, 1 μg/ml, rabbit polyclonal antibody, RP1-calpain-2, Triple Point Biologics, Forest Grove, OR,USA), anti-alpha-fodrin (FG6090,1 : 500, Affiniti Research Product Ltd, Mamhead, UK), anti-nNOS (clone 16, 1 : 1000, 0.25 μg/ml, BD Biosciences, San Jose, CA, USA), anti-iNOS (sc-650, 1 : 1000, 0.2 μg/ml, rabbit polyclonal antibody, Santa Cruz, CA, USA) anti-LC3 (1 : 800)79 and anti-actin (A2066, 1 : 200, Sigma, Stockholm, Sweden) at 4°C overnight. After washing, the membranes were incubated with a peroxidase-labeled secondary antibody for 30 min at room temperature (goat anti-rabbit, 1 : 2000, horse anti-goat, 1 : 2000, or horse anti-mouse 1 : 4000). Immunoreactive species were visualized using the Super Signal Western Dura substrate (Pierce, Rockford, IL, USA) and a LAS 1000 cooled CCD camera (Fujifilm, Tokyo, Japan). Immunoreative bands were quantified using the Image Gauge software (Fujifilm, Tokyo, Japan).
Caspase activity assays
The protein concentrations were determined as above. Samples of crude cytosolic fractions (S2) (25 μl) were mixed with 75 μl of extraction buffer as described earlier.23 Cleavage of Ac-DEVD-AMC (Peptide Institute, Osaka, Japan) was measured with an excitation wavelength of 380 nm and an emission wavelength of 460 nm, and expressed as pmol AMC released per mg protein and minute.
Injury evaluation
Neuropathological scoring
Brain injury in different regions was evaluated using a semiquantitative neuropathological scoring system as described earlier.84 Briefly, sections were stained with thionin/acid fuchsin and scored by an observer blinded to the animals. The cortical injury was graded from 0 to 4, 0 being no observable injury and 4 confluent infarction encompassing most of the cerebral cortex. The damage in the hippocampus, striatum and thalamus was assessed both with respect to hypotrophy (shrinkage) (0–3) and observable cell injury/infraction (0–3) resulting in a neuropathological score for each brain region (0–6). The total score (0–22) was the sum of the scores for all four regions.
Tissue volume
The volumes of tissue loss were measured 3 days post-HI by sectioning the entire brains into 5 μm sections and staining every 100th section for MAP-2. The areas in the cortex, striatum, thalamus and hypothalamus displaying MAP-2 staining were measured in both hemispheres using Micro Image (Olympus, Japan) and the volumes calculated according to the Cavalieri Principle using the following formula: V=∑APT, where V=total volume, ∑A is the sum of the areas measured, P=the inverse of the sampling fraction and T is the section thickness.85 The ratio of tissue loss=(contralateral volume−ipsilateral volume)/contralateral volume.
Cell counting
Cell counting was performed in the cortex, hippocampus, striatum and thalamus (NH) in the similar level for different ages (according to Bregma: −1.64 mm of P60, Franklin and Paxinos). The hippocampus was divided into the CA1, CA3 and DG subfields. Positive cells were counted at × 400 magnification (one visual field=0.196 mm2). In the cortex, three visual fields within an area displaying loss of MAP-2 (if any) were counted and expressed as average number per visual field. Parallel sections were used for all different staining. The counting results were corrected for possible differences in cellular density at different ages by expressing the results as number of immunopositive cells per total number of cells in the visual field or area counted.
Statistics
The Mann–Whitney U-test with Bonferroni correction, preceded by a Kruskal–Wallis test when comparing more than two groups, was used when comparing injury scores and tissue loss. ANOVA with Fisher's post hoc test was used when comparing quantification of Western blots and activity assay. Significance level was assigned at P<0.05.
Abbreviations
- ABC:
-
avidin–biotin peroxidase complex
- AMC:
-
aminomethylcoumarin
- AIF:
-
apoptosis-inducing factor
- Cyt c:
-
cytochrome c
- DTT:
-
dithiothretitol
- FBDP:
-
alpha-fodrin breakdown product
- HI:
-
hypoxia–ischemia
- LC3:
-
microtubule-associated protein 1 light chain 3
- MAP-2:
-
microtubule-associated protein-2
- NOS:
-
nitric oxide synthase
- NO:
-
nitric oxide
- P:
-
postnatal day
- PBS:
-
phosphate-buffered saline
- TBS:
-
tris-buffered saline.
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Acknowledgements
This work was supported by the Swedish Research Council (to HH and KB), the Swedish Child Cancer Foundation (Barncancerfonden) (to KB), the Göteborg Medical Society, the Åhlén Foundation, the Swedish Society of Medicine, the Wilhelm and Martina Lundgren Foundation, the Sven Jerring Foundation, the Frimurare Barnhus Foundation, the Magnus Bergvall Foundation, the National Natural Science Foundation of China (to CZ, 30470598), the Bureau of Science and Technology of Henan Province, the Department of Education of Henan Province.
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Zhu, C., Wang, X., Xu, F. et al. The influence of age on apoptotic and other mechanisms of cell death after cerebral hypoxia–ischemia. Cell Death Differ 12, 162–176 (2005). https://doi.org/10.1038/sj.cdd.4401545
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DOI: https://doi.org/10.1038/sj.cdd.4401545
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