- Research article
- Open Access
The neurotrophin receptor p75NTR mediates early anti-inflammatory effects of estrogen in the forebrain of young adult rats
BMC Neuroscience volume 6, Article number: 58 (2005)
Estrogen suppresses microglial activation and extravasation of circulating monocytes in young animals, supporting an anti-inflammatory role for this hormone. However, the mechanisms underlying estrogen's anti-inflammatory effects, especially in vivo, are not well understood. The present study tests the hypothesis that anti-inflammatory effects of estrogen are mediated by the pan-neurotrophin receptor p75NTR. Previously, we reported that estrogen attenuated local increases of interleukin(IL)-1β in the NMDA-lesioned olfactory bulb, while further increasing NGF expression.
The present studies show that this lesion enhances expression of the neurotrophin receptor p75NTR at the lesion site, and p75NTR expression is further enhanced by estrogen treatment to lesioned animals. Specifically, estrogen stimulates p75NTR expression in cells of microvessels adjacent to the lesion site. To determine the role of this receptor in mediating estrogen's anti-inflammatory effects, a p75NTR neutralizing antibody was administered at the same time the lesion was created (by stereotaxic injections of NMDA) and specific markers of the inflammatory cascade were measured. Olfactory bulb injections of NMDA+vehicle (preimmune serum) increased IL-1β and activated the signaling molecule c-jun terminal kinase (JNK)-2 at 6 h. At 24 h, the lesion significantly increased matrix metalloproteinase (MMP)-9 and prostaglandin (PG)E2, a COX-2 mediated metabolite of arachadonic acid. All of these markers were significantly attenuated by estrogen in a time-dependent manner. However, estrogen's effects on all these markers were abolished in animals that received anti-p75NTR.
These data support the hypothesis that estrogen's anti-inflammatory effects may be, in part, mediated by this neurotrophin receptor. In view of the novel estrogen-dependent expression of p75NTR in cells associated with microvessels, these data also suggest that the blood brain barrier is a critical locus of estrogen's neuro-immune effects.
Estrogen replacement in adult female rats is neuroprotective for a variety of experimentally induced neural injury models, such as ischemia [1–3], toxins [4–6], and forebrain transections . Estrogen is an important modulator of the neural inflammatory response, principally via its actions on microglia, the brain-resident immune cell. In primary cultures of microglia or in glial cell lines, estrogen pretreatment attenuates lipopolysaccharide (LPS)-induced superoxide release, phagocytic activity  and inducible nitric oxide synthase (iNOS) [8–11]. In vivo, estrogen treatment prevents the activation of microglia and recruitment of monocytes following injections of LPS , and attenuates expression of the inflammatory cytokine interleukin (IL)-1β following excitotoxic lesions .
The mechanisms by which estrogen exerts an anti-inflammatory effect, especially in vivo, remain poorly understood. In this report, we test the hypothesis that estrogen's anti-inflammatory effects are mediated via the neurotrophin family of growth factors and receptors. Members of this family include nerve growth factor (NGF), brain-derived neurotrophic factor (BDNF) and neurotrophins (NT)-3 and 4/5. Although first identified by their potent effects on neuronal survival and differentiation, NGF and BDNF are widely distributed and have a broad range of effects. BDNF, for example, is widely synthesized in the vascular system [12–15] and NGF is synthesized in immune cells (for review see ). Local NGF expression increases dramatically following a variety of injurious stimuli [17–19] and may prevent toxic effects of other inflammatory cytokines .
P75NTR, the pan neurotrophin receptor which binds NGF and all the known neurotrophins, also increases following neuronal injury [21, 22]. This increase may be associated with glia  and endothelial cells . Several studies have shown that NGF, when bound to p75NTR, initiates apoptosis in several cell types (reviewed in ) and recent evidence suggests that pro-NGF may preferentially bind p75NTR and initiate apoptosis [26, 27]. P75NTR-NGF interactions have also been implicated in suppressing the immune response by inhibiting the induction of major histocompatibility complex (MHC) class II proteins  and by suppressing the transmigration of circulating immune cells to the brain [24, 29].
Although classified as a neurotrophin receptor, p75NTR may also be considered a member of the tumor necrosis factor receptor (TNFR) family, due to the presence of specific domains called TRAF-interacting motifs or TIMs . TRAF's are TNFR-associated factors, and recruitment of these factors by TIM-containing members of the TNFR family results in the activation of multiple signaling pathways such as NFkB, JNK, ERK and PI-3K, which lead to immune and inflammatory responses as well as cell survival and differentiation (for review see ). P75NTR has been shown to bind recruitment molecules such as the interleukin-receptor associated kinase (IRAK) , which are typically recruited by IL ligand-receptor complexes to activate NFkB and to initiate a pro-inflammatory cascade. Although the downstream consequences of p75NTR-IRAK interactions are not well known, one possibility is that p75NTR competes with IL-1β for this molecule, and may thus attenuate the inflammatory cascade initiated by the interleukins.
The present study was designed to determine the mechanism of estrogen's anti-inflammatory effect in lesioned forebrain of young adult females. Specifically, we examined whether estrogen interacted with the pan-neurotrophin receptor p75NTR to suppress the inflammatory cascade. Following brain injury, there is a rapid synthesis and release of inflammatory cytokines such as IL-1β. These cytokines activate signaling intermediaries such as NFkB and JNK to initiate the transcription of downstream inflammatory genes. We tested the effects of bulb lesions on key portions of this cascade (IL-1β expression, JNK activation, PGE2 and MMP-9 expression) in animals that were given either estrogen or control pellets. The role of p75NTR was evaluated by using a neutralizing antibody to this receptor, injected into the lesion site. In the present study, we used NMDA-induced olfactory bulb lesions, which we have previously shown results in an inflammatory response as indicated by microglial activation and increases in IL-1β . Here we report that olfactory bulb lesions to ovariectomized females increase p75NTR expression, and receptor expression is further enhanced in females that received estrogen treatment. Specifically, estrogen treatment stimulates p75NTR expression in cells associated with microvessels. Antibody experiments reveal that while estrogen treatment suppresses the inflammatory cascade resulting from bulb lesions, blocking the p75NTR receptor completely abolishes estrogen's effects on the early and late markers of the inflammatory cascade, but has no effect on these markers in controls (non-estrogen treated animals). These data support the hypothesis that estrogen's anti-inflammatory effects are mediated through p75NTR. In view of our recent studies that estrogen reduces extravasation of dye from circulation to brain tissue  and the current evidence that estrogen stimulates p75NTR expression in the wall of microvessels, we propose that early in the course of brain injury, estrogen pretreatment suppresses the inflammatory cascade by affecting the blood brain barrier.
Confirmation of estrogen treatment
Plasma estradiol levels were measured from trunk blood collected at termination (approximately three weeks after pellet implantation). Ovariectomized animals replaced with an estrogen-containing pellet (E2) had average plasma estradiol levels of 51.66 ± 4.19 pg/ml, typical of levels seen at proestrus in this animal. The average weight gain as a result of estrogen treatment was -6.24 ± 2.1 g. In contrast, ovariectomized, control pellet-replaced animals (OVX) had low estradiol levels (9.1 ± 0.49 pg/ml) with a corresponding weight gain of 57.5 ± 2.76 g.
Confirmation of anti-p75NTR antibody treatment
In the present studies, the effectiveness of anti-p75NTR antibodies was tested in vivo by measuring caspase-3 activity. Caspase-3, an effector caspase that is proximal to the apoptotic cell death cascade , was used as a marker since p75NTR has been implicated in apoptotic cell death. Caspase-3 activity was significantly reduced (by 40%, p < 0.05) in animals that received NMDA+anti-p75NTR antibody (0.73 ± 0.06 pmol AMC liberated/min at 37°C/mg protein) as compared to animals that received NMDA+preimmune serum (1.23 ± 0.04 pmol AMC liberated/min at 37°C/mg protein).
Specificity of the actions of the p75NTR antibody was not tested directly, by the use of non-specific antibody or antibody to an unrelated protein. However, as described below, the actions of the antibody were seen only in estrogen-treated animals and not in control-treated animals. Furthermore, the actions of the antibody reversed estrogen's actions on inflammatory markers (see Figures 3, 5, 6 and 7), but did not reverse estrogen's effects on the neurotrophin NGF (see Figure 8).
P75NTR regulation following olfactory bulb lesions
P75NTR expression in olfactory bulb lysates was determined by Western blot assay (Figure 1A), and the quantitated signal, normalized to JNK, is shown in a histogram in Figure 1B. P75NTR expression increased 3-4 fold in lesioned animals as compared to sham-injected animals (F1,20: 12.2; p < 0.05). Estrogen treatment further enhanced the level of lesion-induced p75NTR (F1,20: 4.99, p < 0.05). As reported before, this is the group where expression of the inflammatory cytokine IL-1β is attenuated by estrogen . The p75NTR antibody used in Western blot assays recognized a size-appropriate band in olfactory bulb tissue and PC12 cells, a prototypic p75NTR positive cell line.
P75NTR expression in the olfactory bulb of sham and lesioned animals was determined by immunofluorescence (Figure 2), using the same antibody that was used for Western blot analysis. A few sections were also probed with the neutralizing p75NTR antibody. Figure 2a shows the cellular architecture of the olfactory bulb in a section stained with a nuclear dye (DAPI). With either p75NTR antibody, prominent staining was noted in the fibers of the glomerular layer of lesion and sham-injected animals (Figure 2b; taken from region indicated by solid-line box in 2a), similar to that reported by others . While the central portion of the bulb was poorly immunoreactive for p75NTR in the sham-lesion animals (Figure 2c), NMDA injections resulted in bright staining in fibers and cells surrounding the lesion site (Figure 2d). Although the type of cell and fibers is not known currently, the pattern of staining did not appear to be any different in the estrogen-replaced and estrogen-deprived animals. This diffuse staining pattern likely accounts for the bulk of p75 expression observed following lesions in the Western blot analysis. The only location where p75NTR expression differed in estrogen- and control-treated lesioned animals was associated with blood vessels. P75NTR-positive staining was visible in cells lining microvessels near the lesion site in estrogen-treated animals (Figure 2e and 2g). Typically, these vessels contained one or two curved nuclei, characteristic of endothelial cells (visualized by DAPI, Figure 2f and 2h), indicating that these vessels were either capillaries or postcapillary venules. A high magnification image from a section of an estrogen-treated animal photographed under both UV and fluorescein illumination, shown in Figure 2i, depicts p75NTR (in green) localized to a cell lining the vessel wall, identified by its curved nucleus (in blue). While microvessel staining was easily seen in the estrogen-treated animals, there was virtually no p75NTR staining seen in microvessels in the control pellet replaced animals (Figure 2j; nuclear stain in 2k) and in control sections from lesioned, estrogen-replaced animals where the primary antibody was not applied (Figure 2l; nuclear stain in 2m). Photomicrographs (e) through (m) were obtained from the region indicated by the hatched box shown in 2a.
Markers of inflammation
To test if p75NTR mediates the anti-inflammatory effects of estrogen, control and estrogen-pellet replaced animals were injected with NMDA+anti-p75NTR, and compared to sham lesioned controls and controls that received NMDA+preimmune serum. Animals were either terminated 6 or 24 h after the lesion, and olfactory bulb protein lysates were used to measure several proteins associated with the inflammatory cascade.
Local levels of IL-1β, measured by ELISA assay, increased dramatically at 6 h (F 2,30 : 51.61, p < 0.05) and 24 h (F 2,30 : 39.31, p < 0.05) after NMDA injections (Figure 3). At 6 h after lesion, estrogen treated groups had slightly lower levels of IL-1β as compared to placebo groups (F 1,30 : 5.72, p < 0.05). At 24 hours after lesion, estrogen replacement (OVX+E) clearly blunted the injury-related increase in IL-1β (F 2,30 : 4.99, p < 0.05). However, neutralizing p75NTR antibodies completely abolished estrogen's effects, causing IL-1β levels to be no different from those seen in the control-pellet (OVX) replaced NMDA-lesioned group. Note that anti-p75NTR treatment had no effect on the control-replaced group.
Regulation of IL-1β mRNA and ICE activity
To determine the locus of hormone action on this cytokine, IL-1β mRNA levels and the activity of the interleukin-converting enzyme (ICE or Caspase-1) was measured. As shown in Figure 4A, RT-PCR analysis indicated that the lesion substantially increased IL-1β mRNA (F1,12: 146.85; p < 0.05) at 24 h, however, estrogen pretreatment did not affect mRNA expression (F1,12: 0.01, p > 0.05). Furthermore, activity levels of caspase-1, which cleaves the pro-peptide to mature IL-1β, were not regulated by lesion or estrogen treatment (F5,30: 0.99; p > 0.05) at 24 h, (Figure 4B), suggesting that this pathway is not initially responsible for the increase in activated IL-1β.
C-jun kinase activation was determined using antibodies specific for the phosphorylated form of the protein (pJNK) and normalized to total JNK protein (Figure 5). Histogram shows the ratio of pJNK2/JNK at 6 and 24 hours post injury (hpi). JNK is one of the signaling molecules activated by IL-1β when the latter is bound to its receptor. As shown in Figure 5, pJNK2, but not pJNK1, was increased by lesion at 6 h (F2,30: 19.22, p < 0.05) and remained activated at 24 h (F2,30: 19.9, p < 0.05). pJNK1, on the other hand, was constitutively active, which is typical for this isoform. JNK2 has a higher affinity for c-jun , and activated JNK2 translocates to the nucleus, while pJNK1 generally remains in the cytoplasmic compartment . Post hoc analysis indicated that estrogen treatment (OVX+E) attenuated pJNK2 activation in lesioned animals at 24 h as compared to control replaced animals. However, concurrent injection of NMDA+antip75NTR abolished estrogen's effects on pJNK2 at 24 h, such that the relative activation of this molecule was no different from that of control-treated (OVX) animals.
Prostaglandin E2 (PGE2) levels
At 6 h after the lesion, PGE2 levels in the olfactory bulb were no different from sham controls (F2,30: 0.21, p > 0.05; Figure 6), indicating that this marker occurs later in the inflammatory cascade. At 24 hours post injury, there was a 2-fold increase in PGE2 levels in lesioned animals that were deprived of estrogen, while estrogen treatment completely attenuated this increase in PGE2. Anti-p75NTR antibodies completely eliminated estrogen's effects, causing PGE2 levels to rise similar to those seen in the control-replaced (OVX) animals. Note that as with IL-1β, anti-p75NTR treatment had no effect on PGE2 levels in the control-replaced group.
The 96 kD metalloproteinase MMP-9 is secreted by several cell types and is activated by cytokines via the JNK/NFkB pathways. To test whether the lesion influenced expression of MMP-9, both mRNA expression of this gene and functional activation of its protein were analyzed by RT-PCR (Figure 7A) and gelatin zymography (Figure 7B), respectively. While MMP-9 mRNA expression was increased in olfactory bulb lysates 24 h after the lesion (F1,12: 200.32; p < 0.05; Figure 7A), estrogen treatment resulted in a small but signifcant reduction of MMP-9 mRNA (F1,12: 12.4; p < 0.05, main effect of hormone). Lesion-induced increases in MMP-9 mRNA were paralleled by increased MMP-9 activity at 24, but not 6 hours post injury (data not shown), as assayed by gelatin zymography. At 24 hpi, there was a significant increase in MMP-9 gelatinolytic activity as a result of the lesion (F2,30: 10.12, p < 0.05), and estrogen treatment attenuated MMP-9 activity in lesioned animals (F1,30: 21.15, p < 0.05). As with other markers of inflammation measured here, post-hoc analysis indicated that estrogen's effect on MMP-9 activity was reversed in estrogen-treated animals that received anti-p75NTR treatment (F2,30: 3.84, p < 0.05; Figure 7B).
NGF expression in olfactory bulb lysates was measured by an ELISA assay and normalized to total protein. NGF is synthesized by a variety of cell types in the nervous and immune system and one of its principal actions in the brain is to promote growth and regeneration. As shown in Figure 8, olfactory bulb lesions increased NGF levels when measured at 24 h post lesion (F2,30: 24.154, p < 0.05) and estrogen treatment also increased constitutive and lesioned-induced expression of this growth factor (F2,30: 9.41, p < 0.05). However, anti-p75 antibodies did not attenuate the lesion-induced increase in NGF expression in either control or estrogen-treated animals, suggesting that the anti-p75NTR specifically targets the inflammatory cascade (IL-1β, PGE2, MMP-9) rather than repair pathways.
In previous studies, we have shown that the mechanical and excitotoxic damage caused by an NMDA injection to the olfactory bulb results in cell loss, astrocytosis and loss of cholinergic function , as well as microglial activation and a concomitant increase in the inflammatory cytokine IL-1β . The present studies confirm our earlier observations that the inflammatory response in the forebrain of ovariectomized young adult rats is attenuated in animals that were replaced with estrogen as compared to animals that received a control (non-estrogen) pellet . This report also shows that estrogen treatment further stimulates p75NTR expression, and that antibodies to p75NTR, administered concurrently with the lesion, completely abolish estrogen's anti-inflammatory effects. This study supports the hypothesis that estrogen's anti-inflammatory effects in the early portion of neural injury are mediated via the p75NTR. Since anti-p75NTR treatment had no effect on control replaced lesioned animals, these data further suggest that p75NTR expression in cells associated with the microvessel wall, which estrogen stimulates in lesioned animals only, may be a key cellular target of estrogen's anti-inflammatory effects.
The inflammatory cascade contains several protein and proteolipid mediators designed to contain the infectious agent and to phagocytize injured and dead cells. Mature IL-1β binds to its receptor and recruits the interleukin receptor associated kinase (IRAK), and this complex subsequently activates NFkB by association with TRAF-6, a member of the TNF receptor associated factor family [38, 39]. Activation of signaling molecules, such as NFkB and JNK, result in the coordinate transcriptional expression of several downstream inflammatory mediators such as IL-6, IL-10, MMP-9 and cyclooxygenase-2 (COX-2), all of which contain motifs for NFkB or AP-1 in their promoter regions. The present study focused on a few key mediators, representing the early and later points of the inflammatory cascade. IL-1β, which is secreted by activated microglia/macrophages, is an early indicator of inflammation, and is known to activate JNK . Both JNK and NFkB regulate MMP-9  and COX-2 (the synthesizing enzyme for PGE2) . In the present study, the lesion resulted in an early increase in IL-1β, JNK, and MMP-9 and a delayed increase in PGE2. All these indicators were attenuated in lesioned animals that received estrogen, and estrogen's actions were abrogated by anti-p75NTR antibodies. These data strongly support the hypothesis that p75NTR is an important mediator of estrogen's anti-inflammatory effects. While the mechanism of p75NTR anti-immune action is not yet known, one possibility is that p75NTR may interfere with IL-1β signaling pathways by competing for a limited pool of IRAK. NGF/p75NTR complexes are also capable of recruiting IRAK , and may therefore reduce the ability of interleukin receptor ligand complexes to activate NFkB or JNK, and consequently, hamper transcription of inflammation-related genes.
Identified as the first neurotrophin receptor [43, 44], p75NTR has been implicated in both survival and apoptotic pathways . While p75NTR interacts with the receptor tyrosine kinases, or trks, it has independent signaling activities mediated through the ceramide and JNK pathways as well . P75NTR also has significant homology with a family of cell death molecules, such as TNFr and Fas (see [45, 47] for reviews) and has been shown to promote apoptotic cell death in PC12 cells , retinal cells , oligodendrocytes , Schwann cells  and otic vesicles . P75NTR expression also increases following injury, such as spinal cord injury [27, 53]. More recently, studies have implicated p75NTR in the regulation of the inflammatory response, ranging from suppression of MHC molecules to preventing the transmigration of leukocytes. In hippocampal explant cultures, endogenous neurotrophins produced by neurons appear to control the antigen presenting ability of microglia, and neurotrophins, via p75NTR, suppress MHC II molecules . P75NTR has also been localized to peripheral monocytes, and NGF, via p75NTR, prevents monocyte transmigration through the blood brain barrier . In p75 knock-out animals, the severity of inflammation caused by a cranial nerve injury  or experimental allergic encephalomyelitis  is significantly greater as compared to wildtype controls. The p75NTR null animals had increased staining of activated microglia, and a massive recruitment of T-lymphocytes at the lesion site, indicative of increased permeability of the blood brain barrier . The blood brain barrier serves to exclude peripheral cells, specific proteins and molecules from the brain, and p75NTR induction in endothelial cells following experimental allergic encephalomyelitis  suggests that this receptor may serve to maintain the integrity of the blood brain barrier. The present study indicates that estrogen exploits p75NTR-dependent anti-inflammatory mechanisms, and that this action may also occur at the blood brain barrier. In fact, estrogen itself is known to reduce transport across the blood brain barrier in injured [55, 56] and non-injured animals  and reduces monocyte migration into the brain following ischemia .
Local levels of inflammatory cytokines such as IL-1β after traumatic neural injury are derived from two sources: initially from the activation of local microglia and eventually from the influx of circulating macrophages (and their products) that enter the brain due to progressive changes in the blood brain barrier. At 6 h after injury, estrogen treatment has a very modest effect on the IL-1β levels, and consequently, has little or no effect on JNK2 activation, which is activated by IL-1β/IL receptor complexes. At 24 h, however, estrogen markedly suppresses IL-1β levels and this is reflected in a pronounced decrease in JNK activation at this time point. This biphasic effect of estrogen on IL-1β suggests that estrogen may exert its effects not by acting on local microglia, but by reducing the pool of activated immune cells that are recruited to a central lesion site from circulatory sources, either by maintaining the integrity of the blood brain barrier, or by direct action on monocytes/macrophages. Our recent studies show that both possibilities are likely. For example, estrogen treatment suppresses cytokine production in circulating immune cells, but not microglia, when challenged ex vivo with LPS . Furthermore, estrogen treatment also reduces permeability of the blood brain barrier as measured by extravasation of Evan's blue dye . This latter hypothesis is also supported by the fact that estrogen fails to suppress IL-1β mRNA or the activity of caspase-1, which cleaves precursor IL-1β to its mature active form, at 24 hours post injury. This suggests that estrogen may not directly alter the availability of a local pool of IL-1β by canonical pathways but acts to gate the entry of cytokines from circulating immune cells or those produced by microvessel-associated cells.
Vascular permeability and leukocyte invasion can be increased by matrix remodelling resulting from the actions of the MMP family [58, 59]. MMP-9 increases following experimentally induced stroke, and the availability of this proteinase directly contributes to the size of the infarct . Several factors may control MMP-9 regulation and one report indicates that NGF associates with p75NTR to downregulate MMP-9 activity . Estrogen also has been shown to reduce MMP-9 mRNA [6, 62] which likely contributes to its neuroprotective actions. In the present study, estrogen-induced decreases in MMP-9 were reversed by anti-p75NTR. Although this study does not address the source of MMP-9 or its substrate, it may be the case that estrogen-induced reductions in MMP-9 provide the means for maintaining the integrity of the blood brain barrier in these animals.
The observation that estrogen treatment exacerbates p75NTR expression in lesioned animals is surprising in view of the many studies where estrogen has been shown to decrease p75NTR mRNA [63–65] and protein [66, 67] expression. However, these studies were performed in unlesioned animals (without neural trauma), and may therefore be representative of neuronal p75NTR, as has been shown in basal forebrain neurons . This was also the case in a more recent study where estrogen suppressed p75NTR expression in hippocampal neurons following ischemic injury in male gerbils . Moreover, the same study also reported that p75 expression in the hippocampus was first seen 48 h after injury. The present study, on the other hand, describes a very early event in the injury process. Furthermore, the only region where p75NTR expression was regulated differentially was in the microvasculature of estrogen-treated, lesioned animals. This specificity may explain why anti-p75NTR treatment abolished estrogen's effects on the inflammatory cascade but had no discernable effects on the placebo-replaced animals. We hypothesize that the early increase in microvascular p75NTR may play a significantly different role in inflammation as compared to the later expression of neuronal p75NTR.
The present study shows that estrogen replacement to ovariectomized young females suppresses the inflammatory response following neural injury; however, hormonal regulation of the inflammatory response is not always benign. While estrogen reduces experimentally induced inflammation in the anterior chamber of the eye , lungs  and the tibiotarsal joint in adjuvant-induced arthritis [71, 72], this hormone promotes inflammation in the prostate [73, 74], and stimulates edema , vascular permeability and influx of macrophages in the uterus [76–79]. Even in models of neurogenic inflammation, such as the present study, estrogen treatment is not uniformly neuroprotective. For example, a similar 3 wk regimen of estrogen to reproductive senescent females does not attenuate the production of IL-1β, and actually exacerbates it . Furthermore, in these senescent animals, estrogen fails to enhance p75NTR expression following a lesion (data not shown). While the reasons for estrogen's disparate actions on different tissues is not clear, the present study suggests that p75NTR may be one of the switches that predict whether estrogen will exert neuroprotective or neurotoxic effects. An important direction for this work would be to test this hypothesis in the p75 knock-out model or, preferably, a conditional p75NTR knock-out animal, which eliminates the compensatory changes that might occur as a result of developmental loss of p75.
Sprague Dawley females (~250 g, 4 months) were purchased from Harlan Laboratories (IN) and maintained in an AALAC-approved facility on a 12-h light: 12-h dark cycle with lights on at 06:00 h, with food and water available ad libitum. All procedures were in accordance with NIH and institutional guidelines governing animal welfare. Several sets of animals were prepared, each with internal controls. For convenience a chart is provided below. For the p75 expression studies (Westerns blot analysis and immunohistochemistry), we used tissue from four sets of animals that had been prepared for a previous study, and related data from these animals is published in . Briefly, young adult animals were ovariectomized and replaced with either control or estrogen pellets and 3 weeks later were assigned to either sham lesion or NMDA lesion groups. Twenty four hours later, animals were sacrificed and the olfactory bulbs were dissected and later harvested for proteins. A second set was prepared as above for histological analysis, where animals were perfused following anesthetic overdose and the brains recovered for histological processing (described later).
For p75NTR antibody studies, two sets of animals were prepared: placebo or estrogen-replaced animals were assigned to one of three groups: sham lesion, NMDA+vehicle control (preimmune rabbit serum) or NMDA+anti-p75NTR antibodies (made in rabbit). One set of animals was sacrificed at 6 h after the lesion, and the second set at 24 h after the lesion. In all sets, each treatment group consisted of 5-6 animals per group (See Table 1). Specific surgical procedures are detailed below.
Animals were also used for pilot studies to (a) determine the most effective concentration of anti-p75NTR antibodies (n = 12) and (b) to ensure that there were no differences between animals injected with NMDA and NMDA+preimmune serum (the vehicle for the anti-p75NTR antibody) (n = 6).
Ovariectomies: As previously described [4, 66, 80, 81], animals were anesthetized with ketamine (87 mg/kg)/xylazine (13 mg/kg) and bilateral ovariectomies were performed using a dorsal midline incision inferior to the palpated rib cage and kidneys. Ovaries and surrounding tissue were removed and 60-day time-release 17β estradiol pellets (1.0 mg) or control pellets (Innovative Research, FL) were inserted subcutaneously (s.c.) prior to closing the incision. These pellets have been used extensively in our work and have resulted in physiological levels of plasma estradiol for periods of 3 to 6 weeks [4, 5, 66].
After 3 weeks of estrogen or control treatment, all animals were anesthetized with ketamine (87 mg/kg)/xylazine (13 mg/kg) and placed in a rodent stereotaxic apparatus. Skin and cranial fascia were resected and the skull exposed. Two small craniotomies were made in all rats assigned to lesion groups, to expose the olfactory bulbs at the following coordinates: 7.6 mm anterior to bregma and 1.0 mm lateral to the sagittal suture. The tip of a Hamilton syringe needle was briefly lowered to a depth of 3.4 mm, and immediately raised by 0.2 mm to create a trough. A total of 2 μl (1 μl per side) of 50 nM NMDA was injected at a rate of 0.2 μl/30 s. For anti-p75NTR experiments, 1 μL of 50 nM NMDA + 2 μL preimmune rabbit serum (L groups) or 1 μL 50 nM NMDA + 1.5 μL preimmune rabbit serum + 0.5 μL ap75NTR (P groups) was injected in each bulb at a rate of 0.5 μL/30 s. After injections, the needle was raised slowly, craniotomies filled with gel-foam, and scalp sutured with wound clips. Surgical controls were anesthetized, restrained in the stereotaxic apparatus and their scalp and cranial fascia resected and reclipped. Other reports  and our previous studies  indicate that at 24 h post injury a saline injection is not an appropriate control since the injection itself results in injury.
The anti-p75NTR antibody used here (Chemicon, CA, AB1554) recognizes the extracellular domain of the p75NTR and has been shown to block NGF/p75NTR interactions [83–85]. This antibody is not recommended for Western blots (hence a different antibody was used for the Western blot assays), but can be used for immunohistochemistry. Both the neutralizing antibody used here and the antibody used for Westerns revealed similar staining patterns in the olfactory bulb when used for immunohistochemistry.
Animals were sacrificed at 6 h and 24 h after stereotaxic surgery by rapid decapitation and trunk blood was collected for estimation of estradiol content by radioimmunoassay (Diagnostic Systems Laboratories, TX). Olfactory bulbs were rapidly removed and stored at -80°C. Proteins were isolated from the entire olfactory bulb using previously established procedures [4, 80, 81] and total protein concentrations were determined using the BCA protein assay kit (Pierce, IL). In some cases, bulbs were processed for RNA extraction described below.
Western blot analysis
Equal amounts of total protein from tissue lysates were size-fractionated on a polyacrylamide gel, transferred to a nylon membrane (Hybond C-Super, Amersham, NJ) and analyzed for p75NTR and pJNK. Blots were also probed for total JNK expression as a loading control, since this protein did not vary with lesion or estrogen treatment . Membranes were blocked with 5% milk in 1 × Tris Buffered Saline + 0.05% Tween (TTBS) solution for 1 h, followed by incubation with the primary antibody in milk-TTBS (1/ 1500 Ms × NGF Receptor (p75NTR; MAB365), Chemicon, CA; 1/2500 anti-active JNK, Promega, WI; 1/2000 JNK, Santa Cruz, CA) for 1 h at room temperature (p75NTR) or overnight at 4°C (pJNK, JNK). Blots were washed with TTBS (3 × 10 min) and primary antibody was detected using an HRP-conjugated secondary antibody in milk-TTBS (anti-mouse IgG 1/3000 for p75NTR, Transduction Laboratories, KY; 1/6000 anti-rabbit IgG for pJNK, Promega, WI; 1/2000 anti-rabbit IgG for JNK, Santa Cruz, CA). All incubations were performed at room temperature with gentle shaking. After the last wash step, an enzyme-catalyzed chemiluminescent reagent (Renaissance NEN, MA) was used for immunodetection. Signals were detected using X-ray film and bands quantified by densitometric analysis (Molecular Analyst, Bio-Rad, CA) and normalized to JNK expression.
Immunohistochemistry for p75NTR
Immunohistochemistry was performed on olfactory bulb sections of placebo- or estrogenreplaced ovariectomized young-adult animals that were subject to olfactory bulb lesions as outlined above and sacrificed 24 h later. Sections were prepared using the NeuroScience Associates Multibrain technology and some sections from this set were used in previous assays to detect activated microglia . Briefly, animals were anesthetized with 0.6 mL pentobarbital solution (50 μg/mL pentobarbital, 10% ethanol, 40% propylene glycol) and perfused transcardially with PBS followed by 4% paraformaldehyde. Brains were removed from the skull and post-fixed in 4% paraformaldehyde (2 h). Brains were then shipped to NeuroScience Associates (Knoxville, TN), where they were treated with 20% glycerol and 2% dimethylsulfoxide to prevent freeze artifacts, and then embedded coronally in groups of 14-16 per block in a gelatin matrix. 40 μm freeze-cut sections through the entire olfactory bulbs were obtained with an AO 860 sliding microtome and collected in 4 × 6 array of containers filled with 10% phosphate-buffered formaldehyde. After 24 h, sections were rinsed and transferred into Antigen Preserve solution (50% PBS pH 7.0, 50% Ethylene glycol, 1% PVP) for storage and shipping. Prior to use in immunohistochemistry, sections were rinsed in PBS and mounted on gelatin coated glass slides. P75NTR was detected by fluorescence-labeled secondary. Sections were incubated with block solution and followed by overnight incubation with the primary antibody (1/200; mouse anti-NGFR; Chemicon, CA) diluted in PBS with 3% goat serum and 0.4% Triton. Controls were incubated with diluent only. Following washes, sections were incubated with a rat-adsorbed FITC-conjugated Fab specific secondary antibody (1/160 goat anti-mouse, Vector Labs, CA)or AlexaFluor 488 (1:2000 for goat anti-mouse, Invitrogen, CA) for 45 min at room temperature. Sections were then washed and coverslipped using a fluorescence-compatible mounting media which contained DAPI, a nuclear dye. The presence of glomerular staining in the bulb was also used as a positive control. Sections from the midpoint of the bulb (around the injection site) were examined under fluorescence illumination for FITC for the presence of p75NTR immunostaining. Five sections were examined from each animal and 5-6 animals were examined per treatment group.
Caspase-1 and Caspase-3 assays
A commercial kit was used to determine Caspase-1 (interleukin-1 converting enzyme) and Caspase-3 activity (Promega, WI) as before , using manufacturer's recommended procedures. Briefly, blanks, samples and negative controls were pipetted into a flat-bottom, black 96-well plate and incubated at 30°C for 30 minutes. Plates were then incubated with Caspase-1 (ICE) or CCP32 substrate (Ac-YVAD-AMC and Ac-DEVD-AMC, respectively) at 30°C for 60 minutes. A standard curve was prepared just prior to reading at 360 nm (excitation) and 460 nm (emission) in a fluorescence microplate reader (BioTek, VT). Measurement of liberated AMC, interpolated from standard curves, was normalized to protein per unit time (min).
Enzyme-linked immunosorbent assay (ELISA)
Commercial kits for IL-1β (R&D Systems, MN) and PGE2 (Cayman Chemical, MI) were used to determine cytokine and prostaglandin levels in tissue lysates, using procedures recommended by the manufacturers . Briefly, standards, controls, samples and a biotinylated (IL-1β) or acetylcholinesterase-linked (PGE2) secondary antibody were pipetted into 96-well plates pre-coated with antibodies specific for rat IL-1β and PGE2, and incubated at RT for 2 h (IL-1β) or 4°C overnight (PGE2). Following washes, plates were sequentially incubated with streptavidin peroxidase (IL-1β: 2 h) or Ellman's reagent (PGE2: 60-90 min) and substrate solution for 30 min (IL-1β). Plates were read at 450 nm (IL-1β) or 405 nm (PGE2) in a microplate reader (Bio-Tek, VT). Standard curves were established from optical densities of wells containing known dilutions of standard, using KC3 software (Bio-Tek, VT) and sample measurements were interpolated from standard curves.
Reverse transcription-polymerase chain reaction
IL-1β and MMP-9 gene expression was determined by semi-quantitative reverse transcription-polymerase chain reaction (RT-PCR). RNA was extracted using the TRIZOL® Reagent RNA extraction method , followed by further purification with the Qiagen RNeasy Kit (Qiagen, CA). The RNA concentration was determined using the RiboGreen® RNA Quantification Kit (Molecular Probes, OR). Reverse transcription of total RNA (2 μg) was performed with the Gibco Superscript™ First Strand Synthesis System. PCR of the newly synthesized cDNA (8 ng) was performed using PCR Supermix (Invitrogen, CA; primer conc. 0.25 μM; 200 μM dNTP; 1× PCR Buffer, 1.5 mM MgC12, 20 U recombinant Taq DNA polymerase). IL-1β (5'-3': IL-1β-For TTG AAT CTA TAC CTG TCC TGT GTG; IL-1β Rev TGA CTT GGC AGA GGA CAA AGG) PCR cycles were as follows: 95°C 2 min; 30 cycles of 95°C 30 sec, 60°C 1 min, 72°C 2 min. PCR reactions for MMP-9 were performed using previously published primers . PCR conditions were as follows: 95°C for 5 min followed by 40 cycles at 92°C for 1 min, 56°C for MMP-9 for 1 min, and 72°C for 1 min. Cyclophilin (5'-3': CPI-1, TGG TCA ACC CCA CCG TGT TCT TCG; CP1-2 TGC CAT CCA GCC ACT CAG TCT TGG) was used to normalize IL-1β and MMP-9 expression. The PCR cycles for cyclophilin are as follows: 95°C 2 min, 20 cycles of 95°C 30 sec, 62°C 1 min, 72°C 2 min. PCR reactions were performed on a Perkin-Elmer Thermal Cycler 480. Initial analyses were performed to ensure that IL-1β and cyclophilin were amplifying in the linear range. The PCR reaction was separated on a 1.5% agarose gel and quantified using Molecular Analyst™ (BioRad, CA). To avoid quantitation artifacts, only samples loaded on the same gel were analyzed. Hence, for each treatment group, 4 independent samples were analyzed. In every case, only a single band of the expected size was detected and bands amplified by each primer set was sequenced (Gene Technologies Laboratory, TAMU) and determined to be homologous to rat IL-1β and MMP-9 gene sequences.
Procedures used here are a modification of our previous protocol using culture media . Equal amounts of total protein were size fractionated on a 10% polyacrylamide gel containing 0.01% gelatin, along with prestained protein size markers. On some gels, a positive control was included (conditioned media from human umbilical vein endothelial cells; kind gift of G.E. Davis, TAMUS HSC). After electrophoresis, the gels were rinsed with MQ water and then incubated with renaturing buffer (2% Triton X-100 in MQ) at room temperature for 1 h with 3 buffer changes. Gels were then rinsed 3× with MQ water and incubated with developing buffer (50 mM Tris, 0.2 M NaCl, 5 mM CaCl2 0.02% Brij 35) overnight at 25°C with gentle shaking. After a brief rinse with MQ water, gels were stained with a 0.25% coomassie blue solution (50% methanol, 20% acetic acid) for 1 h and destained in 20% methanol: 10% acetic acid. Gels were dried at 50°C for 1 h, and later digitized. A standard densitometric program (Quantity One, BioRad, CA) was used to calculate the intensity of the lytic area.
Statistical analysis was performed using a statistical software package (SPSS Inc, IL), and group differences were considered significantly different at p < 0.05. Data was subject to a two-way analysis of variance (ANOVA) with hormone and lesion as independent variables. Planned post-hoc comparisons were performed for the lesion variable in those studies where there were three groups (sham, lesion+vehicle (preimmune serum) and lesion+anti-p75NTR).
Extracellular-signal regulated kinase
Interleukin-1 converting enzyme
Interleukin receptor-associated kinase
C-jun terminal kinase
Nerve Growth factor
P75 neurotrophin receptor
Prostaglandin E2, PI-3K: Phosphatidylinositol-3 kinase
Tumor necrosis factor receptor
TNFR associated factor
Hurn PD, Littleton-Kearney MT, Kirsch JR, Dharmarajan AM, Traystman RJ: Postischemic cerebral blood flow recovery in the female: effect of 17 beta-estradiol. J Cereb Blood Flow Metab. 1995, 15: 666-672.
Simpkins JW, Rajakumar G, Zhang YQ, Simpkins CE, Greenwald D, Yu CJ, Bodor N, Day AL: Estrogens may reduce mortality and ischemic damage caused by middle cerebral artery occlusion in the female rat. J Neurosurg. 1997, 87: 724-730.
Dubal DB, Kashon ML, Pettigrew LC, Ren JM, Finklestein SP, Rau SW, Wise PM: Estradiol protects against ischemic injury. J Cereb Blood Flow Metab. 1998, 18: 1253-1258. 10.1097/00004647-199811000-00012.
Sohrabji F, Peeples KW, Marroquin OA: Local and cortical effects of olfactory bulb lesions on trophic support and cholinergic function and their modulation by estrogen. J Neurobiol. 2000, 45: 61-74. 10.1002/1097-4695(20001105)45:2<61::AID-NEU1>3.0.CO;2-L.
Nordell VL, Scarborough MM, Buchanan AK, Sohrabji F: Differential effects of estrogen in the injured forebrain of young adult and reproductive senescent animals. Neurobiol Aging. 2003, 24: 733-743. 10.1016/S0197-4580(02)00193-8.
Vegeto E, Belcredito S, Etteri S, Ghisletti S, Brusadelli A, Meda C, Krust A, Dupont S, Ciana P, Chambon P, Maggi A: Estrogen receptor-alpha mediates the brain anti inflammatory activity of estradiol. Proc Natl Acad Sci U S A. 2003, 100: 9614-9619. 10.1073/pnas.1531957100.
Rabbani O, Panickar KS, Rajakumar G, King MA, Bodor N, Meyer EM, Simpkins JW: l7beta-estradiol attenuates fimbrial lesion-induced decline of ChAT-immunoreactive neurons in the rat medial septum. Exp Neurol. 1997, 146: 179-186. 10.1006/exnr.1997.6516.
Bruce-Keller AJ, Keelink JL, Keller JN, Huang FF, Camondola S, Mattson MP: Antiinflammatory effects of estrogen on microglial activation. Endocrinology. 2000, 41: 3646-3656. 10.1210/en.141.10.3646.
Drew PD, Chavis JA: Female sex steroids: effects upon microglial cell activation. Neuroimmunol. 2000, 111: 77-85. 10.1016/S0165-5728(00)00386-6.
Vegeto E, Pollio G, Ciana P, Maggi A: Estrogen blocks inducible nitric oxide synthase accumulation in LPS-activated microglia cells. Exp Gerontol. 2000, 35: 1309-1316. 10.1016/S0531-5565(00)00161-3.
Vegeto E, Bonincontro C, Pollio G, Sala A, Viappiani S, Nardi F, Brusadelli A, Viviani B, Ciana P, Maggi A: Estrogen prevents the lipopolysaccharide-induced inflammatory response in microglia. J Neurosci. 2001, 21: 1809-1818.
Donovan MJ, Miranda RC, Kraemer R, McCaffrey TA, Tessarollo L, Mahadeo D, Sharif S, Kaplan DR, Tsoulfas P, Parada L, et al: Neurotrophin and neurotrophin receptors in vascular smooth muscle cells. Regulation of expression in response to injury. Am J Pathol. 1995, 147: 309-324.
Nemoto K, Fukamachi K, Nemoto F, Miyata S, Hamada M, Nakamura Y, Senba E, Ueyama T: Gene expression of neurotrophins and their receptors in cultured rat vascular smooth muscle cells. Biochem Biophys Res Commun. 1998, 245: 284-288. 10.1006/bbrc.1998.8418.
Nakahashi T, Fujimura H, Altar CA, Li J, Kambayashi J, Tandon NN, Sun B: Vascular endothelial cells synthesize and secrete brain-derived neurotrophic factor. FEBS Lett. 2000, 470: 113-117. 10.1016/S0014-5793(00)01302-8.
Chaldakov GN, Fiore M, Stankulov IS, Manni L, Hristova MG, Antonelli A, Ghenev PI, Aloe L: Neurotrophin presence in human coronary atherosclerosis and metabolic syndrome: a role for NGF and BDNF in cardiovascular disease?. Prog Brain Res. 2004, 146: 279-289. 10.1016/S0079-6123(03)46018-4.
Tabakman R, Lecht S, Sephanova S, Arien-Zakay H, Lazarovici P: Interactions between the cells of the immune and nervous system neurotrophins as neuroprotection mediators in CNS injury. Prog Brain Res. 2004, 146: 387-401.
Crutcher KA, Collins F: Entorhinal lesions result in increased nerve growth factor-like growth-promoting activity in medium conditioned by hippocampal slices. Brain Res. 1986, 399: 383-389. 10.1016/0006-8993(86)91533-7.
Whittemore SR, Larkfors L, Ebendal T, Holets VR, Ericsson A, Persson H: Increased beta-nerve growth factor messenger RNA and protein levels in neonatal rat hippocampus following specific cholinergic lesions. J Neurosci. 1987, 7: 244-251.
Lorez H, Keller F, Ruess G, Otten U: Nerve growth factor increases in adult rat brain after hypoxic injury. Neurosci Lett. 1989, 98: 339-344. 10.1016/0304-3940(89)90425-4.
Hammarberg H, Lidman O, Lundberg C, Eltayeb SY, Gielen AW, Muhallab S, Svenningsson A, Linda H, van der Meide PH, Cullheim S, Olsson T, Piehl F: Neuroprotection by encephalomyelitis: Rescue of mechanically injured neurons and neurotrophin production by CNS-infiltrating T and natural killer cells. J Neurosci. 2000, 20: 5283-5291.
Taniuchi M, Clark HB, Schweitzer JB, Johnson EM: Expression of nerve growth factor receptors by Schwann cells of axotomized peripheral nerves: ultrastructural location, suppression by axonal contact, and binding properties. J Neurosci. 1988, 8: 664-681.
Gorio A, Vergani L, Ferro L, Prino G, Di Giulio AM: Glycosaininoglycans in nerve injury: II. Effects on transganglionic degeneration and on the expression of neurotrophic factors. J Neurosci Res. 1996, 46: 572-580. 10.1002/(SICI)1097-4547(19961201)46:5<572::AID-JNR6>3.0.CO;2-G.
Zhou XF, Rush RA, McLachlan EM: Differential expression of the p75 nerve growth factor receptor in glia and neurons of the rat dorsal root ganglia after peripheral nerve transection. J Neurosci. 1996, 16: 2901-2911.
Copray S, Kust B, Emmer B, Young Lin M, Liem R, Amor S, De Vries H, Floris S, Boddeke EJ: Deficient p75 low-affinity neurotrophin receptor expression exacerbates experimental allergic encephalomyelitis in C57/BL6 mice. J Neuroimmunol. 2004, 148: 41-53. 10.1016/j.jneuroim.2003.11.008.
Barrett GL: The p75 neurotrophin receptor and neuronal apoptosis. Prog Neurobiol. 2000, 61: 205-229. 10.1016/S0301-0082(99)00056-8.
Lee R, Kermani P, Teng KK, Hempstead BL: Regulation of cell survival by secreted proneurotrophins. Science. 2001, 294: 1945-1948. 10.1126/science.1065057.
Beattie MS, Hermann GE, Rogers RC, Bresnahan JC: Cell death in models of spinal cord injury. Prog Brain Res. 2002, 137: 37-47.
Neumann H, Misgeld T, Matsumuro K, Wekerle H: Neurotrophins inhibit major histocompatibility class II inducibility of microglia: involvement of the p75 neurotrophin receptor. Proc Natl Acad Sci U S A. 1998, 95: 5779-5784. 10.1073/pnas.95.10.5779.
Flugel A, Matsumuro K, Neumann H, Klinkert WE, Birnbacher R, Lassman H, Otten U, Wekerle H: Anti-inflammatory activity of nerve growth factor in experimental autoimmune encephalomyelitis: inhibition of monocyte transendothelial migration. Eur J Immunol. 2001, 31: 11-22. 10.1002/1521-4141(200101)31:1<11::AID-IMMU11>3.0.CO;2-G.
Ye X, Mehlen P, Rabizadeh S, VanArsdale T, Zhang H, Shin H, Wang JJ, Leo E, Zapata J, Hauser CA, Reed JC, Bredesen DE: TRAF family proteins interact with the common neurotrophin receptor and modulate apoptosis induction. J Biol Chem. 1999, 274: 30202-30208. 10.1074/jbc.274.42.30202.
Dempsey PW, Doyle SE, He JQ, Cheng G: The signaling adaptors and pathways activated by TNF superfamily. Cytokine Growth Factor Rev. 2003, 14: 193-209. 10.1016/S1359-6101(03)00021-2.
Mamidipudi V, Li X, Wooten MW: Identification of interleukin 1 receptor-associated kinase as a conserved component in the p75-neurotrophin receptor activation of nuclear factor-kappa B. J Biol Chem. 2002, 277: 28010-28018. 10.1074/jbc.M109730200.
Bake S, Sohrabji F: 17b-estradiol differentially regulates blood brain barrier permeability in young and aging female rats. Endocrinology. 2004, 145: 5471-5475. 10.1210/en.2004-0984.
Thornberry NA, Lazebnik Y: Caspases: enemies within. Science. 1998, 281: 1312-1316. 10.1126/science.281.5381.1312.
Turner CP, Perez-Polo JR: Regulation of the low affinity receptor for nerve growth factor, p75NGFR, in the olfactory system of neonatal and adult rat. Int J Dev Neurosci. 1992, 10: 343-359. 10.1016/0736-5748(92)90025-U.
Kallunki T, Su B, Tsigelny I, Sluss HK, Derijard B, Moore G, Davis R, Karin M: JNK2 contains a specificity-determining region responsible for efficient c-Jun binding and phosphorylation. Genes & Dev. 1994, 8: 2996-3007.
Coffey ET, Smiciene G, Hongisto V, Cao J, Brecht S, Herdegen T, Courtney MJ: c-Jun N-Terminal Protein Kinase (JNK) 2/3 Is specifically activated by stress, mediating c-Jun activation, in the presence of constitutive JNK1 activity in cerebellar neurons. J Neurosci. 2002, 22: 4335-4345.
Cao Z, Henzel WJ, Gao X: IRAK: a kinase associated with the interleukin-1 receptor. Science. 1996, 271: 1128-1131.
Cao Z, Xiong J, Takeuchi M, Kurama T, Goeddel DV: TRAF6 is a signal transducer for interleukin-1. Nature. 1996, 383: 443-446. 10.1038/383443a0.
Vereker E, O'Donnell E, Lynch MA: The inhibitory effect of interleukin-1beta on long-term potentiation is coupled with increased activity of stress-activated protein kinases. J Neurosci. 2000, 20: 6811-6819.
Moon SK, Cha BY, Kim CH: ERK1/2 mediates TNF-alpha-induced matrix metalloproteinase-9 expression in human vascular smooth muscle cells via the regulation of NF-kappaB and AP-1: involvement of the ras dependent pathway. J Cell Physiol. 2004, 198: 417-427. 10.1002/jcp.10435.
Plummer SM, Holloway KA, Manson MM, Munks RJ, Kaptein A, Farrow S, Howells L: Inhibition of cyclo-oxygenase 2 expression in colon cells by the chemopreventive agent curcumin involves inhibition of NF-kappaB activation via the NIK/IKK signalling complex. Oncogene. 1999, 18: 6013-6020. 10.1038/sj.onc.1202980.
Johnson D, Lanahan A, Buck CR, Sehgal A, Morgan C, Mercer E, Bothwell M, Chao M: Expression and structure of the human NGF receptor. Cell. 1986, 47: 545-554. 10.1016/0092-8674(86)90619-7.
Radeke MJ, Misko TP, Hsu C, Herzenberg LA, Shooter EM: Gene transfer and molecular cloning of the rat nerve growth factor receptor. Nature. 1987, 325: 593-597. 10.1038/325593a0.
Casaccia-Bonnefil P, Gu C, Khursigara G, Chao MV: p75 neurotrophin receptor as a modulator of survival and death decisions. Microsc Res Tech. 1999, 45: 217-224. 10.1002/(SICI)1097-0029(19990515/01)45:4/5<217::AID-JEMT5>3.0.CO;2-5.
Casaccia-Bonnefil P, Carter BD, Dobrowsky RT, Chao MV: Death of oligodendrocytes mediated by the interaction of nerve growth factor with its receptor p75. Nature. 1996, 383: 716-719. 10.1038/383716a0.
Frade JM, Barde YA: Nerve growth factor: two receptors, multiple functions. Bioessays. 1998, 20: 137-145. 10.1002/(SICI)1521-1878(199802)20:2<137::AID-BIES6>3.0.CO;2-Q.
Rabizadeh S, Oh J, Zhong LT, Yang J, Bitler CM, Butcher LL, Bredesen DE: Induction of apoptosis by the low-affinity NGF receptor. Science. 1993, 261: 345-348.
Frade JM, Rodriguez-Tebar A, Barde YA: Induction of cell death by endogenous nerve growth factor through its p75 receptor. Nature. 1996, 383: 166-168. 10.1038/383166a0.
Yoon SO, Casaccia-Bonnefil P, Carter B, Chao MV: Competitive signaling between TrkA and p75 nerve growth factor receptors determines cell survival. J Neurosci. 1998, 18: 3273-3281.
Soilu-Hanninen M, Ekert P, Bucci T, Syroid D, Bartlett PF, Kilpatrick TJ: Nerve growth factor signaling through p75 induces apoptosis in Schwann cells via a Bcl-2-independent pathway. J Neurosci. 1999, 19: 4828-4838.
Frago LM, Leon Y, de la Rosa EJ, Gomez-Munoz A, Varela-Nieto I: Nerve growth factor and ceramides modulate cell death in the early developing inner ear. J Cell Sci. 1998, 111: 549-556.
Dubreuil CI, Winton MJ, McKerracher L: Rho activation patterns after spinal cord injury and the role of activated Rho in apoptosis in the central nervous system. J Cell Biol. 2003, 162: 233-243. 10.1083/jcb.200301080.
Gschwendtner A, Liu Z, Hucho T, Bohatschek M, Kalla R, Dechant G, Raivich G: Regulation, cellular localization, and function of the p75 neurotrophin receptor (p75NTR) during the regeneration of facial motoneurons. Mol Cell Neurosci. 2003, 24: 307-322. 10.1016/S1044-7431(03)00167-2.
Chi OZ, Barsoum S, Wen Y, Liu X, Weiss HR: 17beta-estradiol prevents blood-brain barrier disruption induced by VEGF. Horm Metab Res. 2004, 36: 272-276. 10.1055/s-2004-814478.
Chi OZ, Liu X, Weiss HR: Effects of 17beta-estradiol on blood-brain barrier disruption during focal ischemia in rats. Horm Metab Res. 2002, 34: 530-534. 10.1055/s-2002-34794.
Johnson AB, Sohrabji F: Estrogen's anti-inflammatory effects on central and circulating immune cells vary with reproductive age. Neurobiol Aging. 2005.
Kraling BM, Wiederschain DG, Boehm T, Rehn M, Mulliken JB, Moses MA: The role of matrix metalloproteinase activity in the maturation of human capillary endothelial cells in vitro. J Cell Sci. 1999, 112: 1599-1609.
Puyraimond A, Fridinan R, Lemesle M, Arbeille B, Menashi S: MMP-2 colocalizes with caveolae on the surface of endothelial cells. Exp Cell Res. 2001, 262: 28-36. 10.1006/excr.2000.5069.
Romanic AM, White RF, Arleth AJ, Ohlstein EH, Barone FC: Matrix metalloproteinase expression increases after cerebral focal ischemia in rats: inhibition of matrix metalloproteinase-9 reduces infarct size. Stroke. 1998, 29: 1020-1030.
Herrmann JL, Menter DG, Hamada J, Marchetti D, Nakajima M, Nicolson GL: Mediation of NGF-stimulated extracellular matrix invasion by the human melanoma low-affinity p75 neurotrophin receptor: melanoma p75 functions independently of trkA. Mol Biol Cell. 1993, 4: 1205-1216.
Moalli PA, Klingensmith WL, Meyn LA, Zyczynski HM: Regulation of matrix metalloproteinase expression by estrogen in fibroblasts that are derived from the pelvic floor. Am J Obstet Gynecol. 2002, 187: 72-79. 10.1067/mob.2002.124845.
Sohrabji F, Greene LA, Miranda RC, Toran-Allerand CD: Reciprocal regulation of estrogen and NGF receptors by their ligands in PC12 cells. J Neurobiol. 1994, 25: 974-988. 10.1002/neu.480250807.
Sohrabji F, Miranda RC, Toran-Allerand CD: Estrogen differentially regulates estrogen and nerve growth factor mRNAs in adult sensory neurons. J Neurosci. 1994, 14: 459-471.
Gibbs RB: Effects of estrogen on basal forebrain cholinergic neurons vary as a function of dose and duration of treatment. Brain Res. 1997, 757: 10-16. 10.1016/S0006-8993(96)01432-1.
Jezierski MK, Sohrabji F: Neurotrophin expression in the reproductively senescent forebrain is refractory to estrogen stimulation. Neurobiol Aging. 2001, 22: 309-319. 10.1016/S0197-4580(00)00230-X.
Ping SE, Greferath U, Barrett GL: Estrogen treatment suppresses forebrain p75 neurotrophin receptor expression in aged, noncycling female rats. J Neurosci Res. 2002, 69: 51-60. 10.1002/jnr.10273.
Jover T, Tanaka H, Calderone A, Oguro K, Bennett MV, Etgen AM, Zukin RS: Estrogen protects against global ischemia-induced neuronal death and prevents activation of apoptotic signaling cascades in the hippocampal CA1. J Neurosci. 2002, 22: 2115-2124.
Miyamoto N, Mandai M, Suzuma I, Suzuma K, Kobayashi K, Honda Y: Estrogen protects against cellular infiltration by reducing the expressions of E-selectin and IL-6 in endotoxininduced uveitis. J Immunol. 1999, 163: 374-379.
Cuzzocrea S, Santagati S, Sautebin L, Mazzon E, Calabro G, Serraino 1, Caputi AP, Maggi A: 17beta-estradiol antiinflammatory activity in carrageenan-induced pleurisy. Endocrinology. 2000, 141: 1455-1463. 10.1210/en.141.4.1455.
Waksman Y, Hod I, Friedman A: Therapeutic effects of estradiol benzoate on development of collagen-induced arthritis (CIA) in the Lewis rat are mediated via suppression of the humoral response against denatured collagen type II (CII). Clin Exp Immunol. 1996, 103: 376-383.
Badger AM, Blake SM, Dodds RA, Griswold DE, Swift BA, Rieman DJ, Stroup GB, Hoffman SJ, Gowen M: Idoxifene, a novel selective estrogen receptor modulator, is effective in a rat model of adjuvant-induced arthritis. J Pharmacol Exp Ther. 1999, 291: 1380-1386.
Naslund MJ, Strandberg JD, Coffey DS: The role of androgens and estrogens in the pathogenesis of experimental nonbacterial prostatitis. J Urol. 1988, 140: 1049-1053.
Harris MT, Feldberg RS, Lau KM, Lazarus NH, Cochrane DE: Expression of proinflammatory genes during estrogen-induced inflammation of the rat prostate. Prostate. 2000, 44: 19-25. 10.1002/1097-0045(20000615)44:1<19::AID-PROS3>3.0.CO;2-S.
Tchernitchin AN, Galand P: Oestrogen levels in the blood, not in the uterus, determine uterine eosinophilia and oedema. J Endocrinol. 1983, 99: 123-130.
Quarmby VE, Korach KS: The influence of l7beta-estradiol on patterns of cell division in the uterus. Endocrinology. 1984, 114: 694-702.
De M, Wood GW: Influence of oestrogen and progesterone on macrophage distribution in the mouse uterus. J Endocrinol. 1990, 126: 417-424.
Kachkache M, Acker GM, Chaouat G, Noun A, Garabedian M: Hormonal and local factors control the immunohistochemical distribution of imrnunocytes in the rat uterus before conceptus implantation: effects of ovariectomy, fallopian tube section, and injection. Biol Reprod. 1991, 45: 860-868.
Kaushic C, Frauendorf E, Rossoll RM, Richardson JM, Wira CR: Influence of the estrous cycle on the presence and distribution of immune cells in the rat reproductive tract. Am J Reprod Immunol. 1998, 39: 209-216.
Jezierski MK, Sohrabji F: Region- and peptide-specific regulation of the neurotrophins by estrogen. Brain Res Mol Brain Res. 2000, 85: 77-84. 10.1016/S0169-328X(00)00244-8.
Jezierski MK, Sturm AK, Scarborough MM, Sohrabji F: NGF stimulation increases JNK2 phosphorylation and reduces caspase-3 activity in the olfactory bulb of estrogen-replaced animals. Endocrinology. 2001, 142: 2401-2404. 10.1210/en.142.6.2401.
Acarin L, Gonzalez B, Castellano B: Neuronal, astroglial and microglial cytokine expression after an excitotoxic lesion in the immature rat brain. Eur J Neurosci. 2000, 12: 3505-3520. 10.1046/j.1460-9568.2000.00226.x.
Mount HT, Elkabes S, Dreyfus CF, Black IB: Differential involvement of metabotropic and p75 neurotrophin receptors in effects of nerve growth factor and neurotrophin-3 on cultured Purkinje cell survival. J Neurochem. 1998, 70: 1045-1053.
Fiorentini C, Guerra N, Facchetti M, Finardi A, Tiberio L, Schiaffonati L, Spano P, Missale C: Nerve growth factor regulates dopamine D(2) receptor expression in prolactinoma cell lines via p75(NGFR)-mediated activation of nuclear factor-kappaB. Mol Endocrinol. 2002, 16: 353-366. 10.1210/me.16.2.353.
Pehar M, Cassina P, Vargas MR, Castellanos R, Viera L, Beckman JS, Estevez AG, Barbeito L: Astrocytic production of nerve growth factor in motor neuron apoptosis: implications for amyotrophic lateral sclerosis. J Neurochem. 2004, 89: 464-473.
Maier SE, Cramer JA, West JR, Sohrabji F: Alcohol exposure during the first two trimersters equivalent alters granule cell number and neurotrophin expression in the developing rat olfactory bulb. J Neurobiol. 1999, 41: 414-423. 10.1002/(SICI)1097-4695(19991115)41:3<414::AID-NEU9>3.0.CO;2-F.
The authors wish to thank Debbie Geevarghese, Najma Ahmed and Lynne O'Kelley for technical assistance. Supported by grants from the NIH (AG 19515) and the Alzheimer's Association to FS.
VLN performed almost all experiments and prepared most figures, DKL performed RT-PCR analyses and prepared the associated figures, SB participated in data analysis and interpretation, FS conceived the study, performed statistical analysis and photomicroscopy. All authors read and approved the final manuscript.
Authors’ original submitted files for images
Below are the links to the authors’ original submitted files for images.
About this article
Cite this article
Nordell, V.L., Lewis, D.K., Bake, S. et al. The neurotrophin receptor p75NTR mediates early anti-inflammatory effects of estrogen in the forebrain of young adult rats. BMC Neurosci 6, 58 (2005) doi:10.1186/1471-2202-6-58
- Nerve Growth Factor
- Olfactory Bulb
- Inflammatory Cascade
- Estrogen Treatment