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The Journal of Neuroscience, July 2, 2003, 23(13):5416-5424
Previous Article | Next Article
Glial Reactivity in Ciliary Neurotrophic Factor-Deficient Mice after Optic Nerve Lesion
Aliki Martin, Hans-Dieter Hofmann, andMatthias Kirsch Institute of Anatomy, University of Freiburg, D-79001 Freiburg, Germany
Abstract
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Abstract
Introduction
There is evidence that ciliary neurotrophic factor (CNTF), in addition to its neurotrophic activity, positively regulates astrogliosis after CNS injury. CNTF and its receptor, CNTFR, are strongly upregulated in activated astrocytes. Application of CNTF upregulates GFAP expression in cultured astrocytes and induces various aspects of gliosis in the intact brain. Here we examined whether inactivation of the CNTF gene results in the expected changes in glial reactivity by analyzing gliosis in the superior colliculus (SC) after optic nerve crush.
Basal expression levels of GFAP and vimentin in unlesioned CNTF-deficient mice were reduced by 66 and 37%, respectively. Absolute numbers of astrocytes were found not to be different. Surprisingly, however, lesion induced robust activation of astrocytes in CNTF-deficient mice; the time course of activation was even accelerated as compared with wild-type animals. At later time points, activation reached the same level. With respect to microglial cells, basal expression of microglial markers was unaltered in CNTF–knock-out animals. Lesion-induced upregulation of Iba-1, ICAM-1, and F4/80 in microglial cells was unaffected in CNTF-deficient animals. Differences were observed with respect to the time course of microglial activation, different markers being affected differentially. We further demonstrate that lesion induces upregulation of CNTF-related cytokines (LIF, NNT-1) and, interestingly, a more pronounced upregulation of cytokine receptor components (LIF receptor
, gp130) and TGF
Key words: gliosis; astrocytes; GFAP; microglia; ciliary neurotrophic factor; leukemia inhibitory factor
Introduction
There is increasing evidence that ciliary neurotrophic factor (CNTF) is of particular importance as a regulator of reactive processes after lesion in the PNS and CNS. CNTF and its specific receptor component, CNTFR; Rudge et al., 1994
A large number of other cytokines and growth factors have been shown to be involved in mediating astroglial or microglial activation. Interleukin (IL)-1, IL-2,
-interferon, TGF-
In the experiments reported here, we have examined the role of CNTF in regulating glial reactivity by using CNTF–knock-out animals, for which no lesion-associated phenotype has been described so far. In the optic nerve lesion model, the results of lesioning can be monitored in the target area of retinal ganglion cells, the superior colliculus, which is at some distance from the actual lesion site, thereby minimizing the direct effects of breaching the blood–brain barrier.
We demonstrate that in the absence of CNTF, the glial reaction to lesion in principle is unimpaired. Morphological analyses, however, suggest that at early time points after lesion (3 dpl), astrocyte activation has progressed further in CNTF–knock-out animals. This is accompanied by increased mRNA expression of key components of its receptor system, namely gp130 and LIFR
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Materials and Methods
Animals. Adult male animals were used in all experiments. CNTF–/– breeding animals (Masu et al., 1993Optic nerve lesions. Animals were anesthetized with a mixture of 25% Ketavet (Parke-Davis; 100 mg/ml), 6% Rompun (Bayer; 20 mg/ml), and 2.5% Ventranquil (Albrecht; 10 mg/ml) in physiological saline at a dose of 2.5 ml/kg body weight. Access to the orbita was gained by lateral canthotomy. The optic nerve was exposed by cutting the lateral rectus muscle and by blunt dissection of the tissue surrounding the optic nerve. The meninges were left intact. Crush lesioning was performed with forceps of 1 mm tip width for 30 sec. Immediately after the crush, retinal circulation was checked ophthalmoscopically. Only animals that showed unimpaired circulation within 2 min after the nerve was lesioned were included in this study. The eyelid was closed by a suture to prevent drying of the cornea.
Morphological analysis. After various survival times, animals were transcardially perfused first with 0.9% NaCl in 20 mM phosphate buffer (PB), pH 7.2, followed by 4% paraformaldehyde in 0.1 M PB for 10 min. The brains were removed and postfixed in the same fixative for 3 hr at 4°C followed by cryoprotection in 20% sucrose in 0.1 M PB, pH 7.2, at 4°C overnight. Cryostat sections (30 µm, coronal plane) were cut in series through the midbrain at the level of the superior colliculus. Series consisting of five to six sections covering the whole rostrocaudal extent of the superior colliculus were collected into individual wells of a multiwell plate. Sections from wild-type and knock-out animals were marked by needle punches to enable their identification, and one series of sections from a wild-type and a CNTF–knock-out animal was processed free-floating for immunocytochemistry after placing them together into a single well of a 12-well tissue culture plate to ensure equal staining conditions. Immuncytochemical staining was performed with the following antibodies at the dilutions given: anti-S100 (1:10,000; Swant, Bellinzona, Switzerland), anti-GFAP (1:500; Dako, Glostrup, Denmark), anti-F4/80 (1:50), anti-CD11b (1:50; all from Serotec/Biozol, Eching, Germany), anti-Iba-1 (1:2000; a kind gift of Dr. Y. Imai, National Institute of Neuroscience, Tokyo, Japan). All incubations were performed at room temperature (RT) unless noted otherwise. Sections were first treated at RT with methanol containing 0.3% H2O2 to quench endogenous peroxidase activity for 30 min. After one brief washing step in 0.1 M PB, unspecific binding sites were blocked by incubation with 10% normal serum (normal rabbit or normal goat serum, depending on the secondary antibody used; Biotrend, Köln, Germany), 1% Triton X-100 in 0.1 M PB for 1 hr. Incubation with the primary antibodies was performed overnight at 4°C in 0.1 M PB containing 10% blocking solution. After three washes (15 min each) with PB, sections were incubated with biotinylated secondary antibody (Vector Laboratories, Burlingame, CA) diluted 1:250 in PB containing 2% horse serum for 60 min at room temperature. Bound antibodies were detected by the indirect immunoperoxidase method using the ABC-Elite kit (Vector Laboratories) and DAB/H2O2 following the manufacturer's recommendations. Sections were mounted onto glass slides, air dried, and coverslipped in Hyper-Mount (Shandon, Frankfurt, Germany) after dehydration in a graded series of ethanol and toluene.
To quantitate staining intensity, digital images of the stained sections were obtained with an Olympus PD-11 digital camera using standardized illumination conditions. Images obtained in this way were then analyzed with an image analysis program (Scion-Image, Scion Corporation). Mean gray levels and optical density (sum of the gray values in the selection, with background subtracted) on the ipsilateral and contralateral side were measured in 10 circular measuring fields
100 µm in diameter placed randomly over the stratum opticum and stratum griseum superficiale of the superior colliculus. Measurements were done in three to six sections of a minimum of three animals of each genotype per time point analyzed. All measurements from one animal were averaged and treated as an independent data point in the subsequent statistical analysis. For evaluating Iba-1 staining, the optical density ratio between the contralateral and ipsilateral side was chosen as a measuring parameter. For evaluation of F4/80 and GFAP staining, a mean gray value (sum of gray values of all pixels in the selection divided by number of pixels) was calculated by subtracting the mean gray value of the ipsilateral from that obtained on the contralateral side. For these markers, calculation of the optical density ratio was not possible because of the absence of stained cells on the ipsilateral side. Statistical analysis was performed by two-tailed t tests or two-way ANOVA using GraphPad Prism (GraphPad Software, San Diego, CA) and the post-test calculators provided at http://www.graphpad.com. Details are given in respective figure legends.
Real-time quantitative RT-PCR. Tissue for PCR analysis of mRNA expression was dissected from brains frozen immediately after dissection. Purification of total RNA was performed by sonication (Branson Sonifier, Danbury, CT) in 1 ml Trizol (Invitrogen, Karlsruhe, Germany) according to the manufacturer's suggestions. After the RNA pellet was dried and redissolved in RNAase-free water, concentration was determined spectrophotometrically. Total RNA (1–2 µg) was then subjected to DNAase I treatment (Invitrogen) and reverse transcribed with oligo-dT as a primer and Moloney murine leukemia virus-reverse transcriptase (Promega, Mannheim, Germany) for 1 hr at 42°C.
Aliquots of cDNA corresponding to
3' direction.
The primers were used at a concentration of 250 nM in the PCR reaction. Cycling conditions were as follows: 10 min at 95°C (to activate the hot-start Taq-polymerase supplied with the SybrGreen detection kit), followed by 40 cycles of 1 min at 95°C and 1 min at 60°C (two-step PCR). During amplification, the fluorescence signal, which is proportional to the amount of double-stranded product produced, was monitored. In this way a complete amplification profile for each of the 96 wells of a PCR plate was obtained, which was used for the analysis. At the end of the PCR run, melting curves of the amplified products were obtained, which were used to control specificity of the amplification reaction. Pilot experiments, in which aliquots of the amplified products were separated on agarose gels, were performed to ensure amplification of specific products of the predicted length.
From the amplification curves obtained in this way, a threshold cycle number (Ct) was calculated. Ct corresponds to the cycle number at which the amplification curve reaches a fluorescent signal of a user-defined magnitude. Thresholds were selected so that Ct values lay at the beginning of the linear phase of amplification. Expression levels were normalized to those obtained for the housekeeping gene glyceraldehyde-3-phosphate dehydrogenase. Values from triplicate measurements of each experimental animal were averaged and treated as independent data points in the subsequent statistical analysis by two-tailed, unpaired t tests. Details of relative quantification of gene expression using this method can be found in User Bulletin 2, which can be found by searching for the phrase "relative quantitation of gene expression" at the following site: http://docs.appliedbiosystems.com/search.taf.
Results
Five days after crush lesioning of the optic nerve in mice, astrocytes and microglial cells are activated in the deafferented SC contralateral to the lesion side (Fig. 1a–c). Glial activation is restricted to the contralateral side and to the superficial layers of the SC where retinal ganglion cell axons terminate. Activation of astrocytes on the contralateral side could be readily detected by staining with antibodies against GFAP, and no detectable staining was observed ipsilateral to the lesion side and in unlesioned control mice. GFAP-stained cells show the typical morphology of activated astrocytes with numerous thick processes and hypertrophied somata (Fig. 1a, inset). Microglial cells can be stained with various markers; some of them, like Iba-1, stain both resting and activated microglial cells (Fig. 1b), and others, like F4/80, stain only activated microglial cells (Fig. 1c). Staining of midbrain sections with antibodies against Iba-1 shows a regular distribution of ramified microglial cells. After lesion, microglial cells in the contralateral SC are stained more intensely and show the typical activated morphology with decreased ramification and hypertrophy of the soma region (Fig. 1b, inset). Activation of astrocytes and microglial cells in the deafferented superior colliculus as evidenced by staining for these markers first becomes detectable 2 d after lesion (data not shown). This is in contrast to the situation in areas directly affected by a lesion in other lesion paradigms such as stab wounds or ischemia, where glial activation becomes apparent within hours after lesion (Raivich et al., 1999
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Figure 1. Astroglial and microglial activation after optic nerve lesion in the mouse. Five days after a crush lesion of the left optic nerve, cryosections through the midbrain at the level of the superior colliculus were immunostained with antibodies against GFAP (a) to detect activated astrocytes and Iba-1 (b) or F4/80 (c), both specifically staining microglial cells. For all markers used, immunoreactivity on the contralateral (right) side is stronger than on the ipsilateral side. Insets show details of the superficial layer of the superior colliculus at higher magnification. Scale bar: a, 200 µm; inset, 50 µm.
When comparing GFAP-stained sections of CNTF-deficient and wild-type animals 3 d after an intraorbital crush of the optic nerve (3 dpl) (Fig. 2), increased staining in the CNTF–knock-out animals (Fig. 2b) is apparent as compared with wild-type animals (Fig. 2a). Astrocyte activation in wild-type animals exhibits the characteristics of the early activation response described by Raivich et al. (1999
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Figure 2. Astrocytes are more strongly activated at 3 dpl in CNTF–/– animals. a–d, GFAP immunostaining of cryosections through the right (contralateral) superior colliculus 3 d (a, b) and 14 d (c, d) after lesion in wild-type (a, c) and CNTF–knock-out animals (b, d). At 3 dpl astrocytes in CNTF–/–-animals (b) are more strongly stained than in wild-type animals (a). Astroglial reactivity has reached similar levels at 14 dpl (c, d). Scale bars: b, d, 50 µm. e, Densitometric analysis of GFAP-immunostained sections 3 and 14 dpl. Staining intensity was quantified by densitometric analysis as detailed in Materials and Methods (Morphological analysis). Values are means ± SD. Asterisk indicates a significant increase in staining intensity as compared with wild-type animals; p < 0.05; two-way ANOVA with post-test using the Bonferroni correction: residual df = 10; residual mean square 13.31.
With respect to activation of microglial cells, no differences could be demonstrated by immunocytochemistry between unoperated wild-type and knock-out animals with the markers used (Iba-1, F4/80, CD11b). These markers have been widely used to detect activated microglial cells after lesion (for review, see Raivich et al., 1999
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Figure 3. Microglial cells are more strongly activated in CNTF–/– animals. Maximal differences in microglial reactivity as shown by different activation markers could be observed at different time points after lesion. a–f, Immunostaining with antibodies against the microglial markers F4/80 (5 dpl; a, b), CD11b (14 dpl; b, c), and Iba-1 (8 dpl; e, f) in wild-type (a, c, e) and CNTF–knock-out animals (b, d, f). Scale bar: (in f) a–f, 50 µm.
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Figure 4. Densitometric analysis of Iba-1 and F4/80 staining shows stronger activation of microglial cells in CNTF–/– animals (hatched bars) as compared with wild-type animals (filled bars). Staining intensity was quantified by densitometric analysis as detailed in Materials and Methods (Morphological analysis). Results for Iba-1 (a) staining are given as optical density ratio (±SEM) between staining on the contralateral and ipsilateral sides; those for F4/80 staining (b) are expressed as the mean gray level (±SEM) on the contralateral side obtained by subtracting the mean gray level determined on the ipsilateral side from that measured on the contralateral side. Asterisk indicates significant differences in staining intensity; p < 0.05 (**p < 0.01); two-way ANOVA with post-test using the Bonferroni correction. a, Residual df = 19; residual mean square 0.02365; b, residual df = 28; residual mean square 11.06.
To determine differences in glial activation on the mRNA level, we performed a quantitative RT-PCR analysis for astroglial and microglial markers (Figs. 5, 6). Analysis of GFAP mRNA expression in unlesioned control animals revealed reduced basal expression in CNTF–knock-out as compared with wild-type animals (33.5%) (Fig. 5a). However, 1 d after optic nerve lesion, GFAP expression has increased 1.8-fold in knock-out animals as compared with 1.2-fold in wild-type animals (Fig. 5b). Statistical analysis (two-tailed, unpaired t test) showed that at this time point, GFAP expression in knock-out animals is already significantly increased (p < 0.05), whereas the increase in wild-type animals has not reached statistical significance. Thus astroglial activation has only been initiated measurably in CNTF-deficient animals at this time point. Three days after lesion, expression of GFAP mRNA has increased 8.9-fold in the knock-out animals and only 3.1-fold in the wild-type animals (Fig. 5b). On the basis of the observed reduced basal GFAP mRNA expression in knock-out animals, this results in similar absolute levels of GFAP mRNA at 3 dpl.
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Figure 5. Basal expression of GFAP and vimentin mRNA is reduced (a), and relative increase in expression induced by optic nerve lesion is stronger in CNTF–knock-out animals 3 dpl (b). a, b, Results from quantitation of mRNA expression by real-time quantitative PCR. Basal expression of GFAP and vimentin (a) in the superior colliculus of unoperated CNTF–/– animals (n = 4) is expressed as percentage (±SD) of the expression level determined in unoperated wild-type animals (n = 3). Lesion-induced upregulation of marker expression (b) is given as fold induction versus unoperated controls. All values are mean values (±SD) from n = 3–4 animals. Solid bars represent values from wild-type animals; hatched bars represent values from CNTF–/– animals. a, Values for GFAP and vimentin in CNTF–knock-out animals are significantly different from those obtained from wild-type animals with p < 0.01; unpaired t test, two-tailed. b, *** indicates significant differences in staining intensity between CNTF–/– and wild-type animals; p < 0.001, two-way ANOVA with post-test using the Bonferroni correction. GFAP, Residual df = 10; residual mean square 0.7089; vimentin, residual df = 10; residual mean square 0.330. c, Western blotting of protein extracts from the superior colliculus of wild-type (WT) and CNTF–/– animals (KO). Tissue samples were separated by SDS-PAGE, immunoblotted, and sequentially probed with antibodies against the indicated proteins. Bound antibodies were detected by chemiluminescence and exposure to x-ray film (Kodak-X-OMAT). d, e, Immunostaining of cryosections through the right (contralateral) superior colliculus with antibodies against the astroglial marker S100
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Figure 6. Lesion-induced upregulation of microglial marker mRNAs (a) and LIFR
Another astroglial marker, vimentin, showed a similar expression pattern. Basal expression of vimentin mRNA is reduced to 62.7% in knock-out animals (Fig. 5a). Vimentin expression at 3 dpl is upregulated 4.9-fold in knock-out animals and twofold in wild-type animals. As for GFAP, increased lesion-induced up-regulation of vimentin expression is also already apparent at 1 dpl, with knock-out animals showing higher expression than wild-type animals (Fig. 5b). Differences in basal expression of GFAP could also be detected by immunoblotting (Fig. 5c). To test whether reduced basal expression of GFAP in the knock-out animals results from a reduction in astrocyte numbers, immunocytochemical staining and immunoblotting with antibodies against another astroglial marker protein, S-100
Quantitative analysis of the expression of microglial markers 3 dpl showed that expression of all markers studied is upregulated after lesion (Fig. 6a). All markers showed a consistently stronger lesion-induced upregulation in the CNTF-deficient animals (Fig. 6a, hatched bars) as compared with wild-type animals (Fig. 6a, solid bars), although statistical analysis of the data showed that only values for Iba-1 and ICAM-1 reached statistical significance. None of the microglial markers examined showed differences in basal expression between wild-type and knock-out animals (data not shown), indicating that the observed differences in lesion-induced upregulation indeed reflect stronger activation of microglial cells in the CNTF-deficient animals. This is in agreement with the immunocytochemical observations for Iba-1, CD11b, and F4/80 (Figs. 3, 4a).
Taken together, our results would indicate that activation of astrocytes and microglial cells in the knock-out animals is not only unimpaired, but may even be accelerated. To examine whether changes in the regulation of receptor components for CNTF and related cytokines is different in CNTF–knock-out animals or if other factors that have been shown to be involved in inducing gliosis are differentially regulated, we studied expression of candidate molecules by quantitative PCR. Figure 6b summarizes these results. All expression levels are expressed as fold upregulation relative to unoperated control animals, because none of the examined genes showed differences in basal expression levels. First, we found lesion induced upregulation of two other members of the IL-6 family of cytokines, namely LIF and the recently described family member NNT-1/cardiotrophin-like cytokine. However, 3 dpl expression of both factors is upregulated to the same extent. On the other hand, expression of two of the three receptor components of the CNTF/LIF system, LIFR
Discussion
Previous studies had suggested a role for CNTF as a positive regulator of gliosis after lesions in the CNS. By analyzing glial activation in the SC of CNTF-deficient mice after optic nerve lesion, we show that astroglial and microglial activation are remarkably unaffected by the absence of CNTF and that differences between wild-type and knock-out animals are mainly reflected in an altered time course of activation. Specifically, we show that certain markers of glial activation are upregulated earlier in CNTF–knock-out animals. Increased lesion-induced upregulation of LIFRGlial reactivity in the superior colliculus after optic nerve lesion
In unoperated animals, astrocytes in the SC are GFAP negative. Optic nerve lesion, however, leads to the appearance of strongly GFAP-stained astrocytes in the SC that exhibit the characteristics of activated cells (Fawcett and Asher, 1999In agreement with previous studies, glial activation was undetectable morphologically earlier than 2–3 dpl (Schmidt-Kastner et al., 1993
Basal expression of astroglial markers is reduced in the absence of CNTF
CNTF and LIF can control GFAP expression in cultured astrocytes and during development (Bugga et al., 1998None of the microglial markers examined showed differences in basal expression levels (data not shown), suggesting that unlike the situation for astrocytes, microglial cells in the unlesioned brain are not affected by the absence of CNTF.
Glial activation in CNTF–/– mice
We reasoned that elimination of CNTF would lead to reduced glial activation after lesion, thus directly proving its suggested contribution in inducing gliosis. Unexpectedly, however, glial responses, and that of astrocytes in particular, are not impaired at all in CNTF–knock-out animals. Rather, lesion-induced upregulation of the astrocytic activation markers GFAP and vimentin could be detected earlier in CNTF-deficient animals. Starting at lower basal levels, upregulation of GFAP mRNA is detectable at 1 dpl only in the mutants. At later time points, mRNAs for GFAP as well as vimentin reach the same expression levels as in wild-type mice at 3 dpl, suggesting that the absence of CNTF affects only the initial phase of activation. This was also observed morphologically by immunostaining for GFAP, which showed that at 3 dpl fully activated astrocytes were more abundant in CNTF-deficient animals. At later time points activation was indistinguishable from that in wild-type mice, indicating that the lack of CNTF, rather than leading to reduced activation, results in a subtle change of its time course.With respect to microglial cells, CNTF elimination affected microglial markers differentially. For F4/80 staining, maximal differences were found at 5 dpl, whereas Iba-1 and CD11b staining were maximally different at 8–14 dpl. Because different activation markers probably characterize different functional states of microglial cells (for review, see Raivich et al., 1999
Because it is assumed that microglial cells are first to detect damage (Kreutzberg, 1996
Increased expression of CNTFR
Expression of gp130 and LIFRWe observed a significant difference in lesion-induced up-regulation of TGF-
Footnotes
Received Aug. 20, 2002; revised Apr. 29, 2003; accepted May. 1, 2003.This work was supported by Deutsche Forschungsgemeinschaft Grant KI 419/2-1, 2-2 (M.K.). We thank Birgit Egle and G. Kaiser for excellent technical assistance. We are indebted to Dr. M. Sendtner for the CNTF–knock-out animals.
Correspondence should be addressed to Matthias Kirsch, Institute of Anatomy I, University of Freiburg, Albertstrasse 23, D-79104 Freiburg, Germany. E-mail: matthias.kirsch{at}zfn.uni-freiburg.de.
Copyright © 2003 Society for Neuroscience 0270-6474/03/235416-09$15.00/0
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