Abnormal Reaction to Central Nervous System Injury in Mice Lacking Glial Fibrillary Acidic Protein and Vimentin

doi:10.1083/jcb.145.3.503

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© The Rockefeller University Press, 0021-9525/1999//503 $5.00
The Journal of Cell Biology, Volume 145, Number 3, , 1999 503-514

Regular Articles

Abnormal Reaction to Central Nervous System Injury in Mice Lacking Glial Fibrillary Acidic Protein and Vimentin

Milos Pekny^*, Clas B. Johansson^,||, Camilla Eliasson^*, Josefina Stakeberg^*, Åsa Wallén^¶, Thomas Perlmann^¶, Urban Lendahl, Christer Betsholtz^*, Claes-Henric Berthold, and Jonas Frisén

^* Department of Medical Biochemistry and Department of Anatomy and Cell Biology, Gothenburg University, SE-405 30 Gothenburg, Sweden; and Department of Cell and Molecular Biology, Medical Nobel Institute, ^|| Department of Neuroscience, Karolinska Institute and ^¶ Ludwig Institute for Cancer Research, Stockholm Branch, SE-17177 Stockholm, Sweden

In response to injury of the central nervous system, astrocytesbecome reactive and express high levels of the intermediatefilament (IF) proteins glial fibrillary acidic protein (GFAP),vimentin, and nestin. We have shown that astrocytes in micedeficient for both GFAP and vimentin (GFAP–/–vim–/–)cannot form IFs even when nestin is expressed and are thusdevoid of IFs in their reactive state. Here, we have studied the reaction to injury in the central nervous system in GFAP–/–,vimentin–/–, or GFAP–/–vim–/–mice. Glial scar formation appeared normal after spinal cord or brain lesions in GFAP–/– or vimentin–/–mice, but was impaired in GFAP–/–vim–/–mice that developed less dense scars frequently accompaniedby bleeding. These results show that GFAP and vimentin arerequired for proper glial scar formation in the injured centralnervous system and that some degree of functional overlap existsbetween these IF proteins.

Key Words: GFAP • nestin • injury • astrocyte • blood vessel

Abbreviations used in this paper: BrdU, bromodeoxyuridine; CNS, central nervous system; GFAP, glial fibrillary acidic protein; HE, hematoxylin and erythrosin/eosin; IF, intermediate filament; IR, immunoreactivity.

Address correspondence to Dr. Milos Pekny, Department of Medical Biochemistry, University of Gothenburg, Box 440, SE-405 30Gothenburg, Sweden. Tel.: 46 31 7733269. Fax: 46 31 416108.E-mail: milos.pekny @medkem.gu.se

Adense scar composed primarily of hypertrophic astrocytes formsrapidly at the site of a brain or spinal cord injury. Scar formationis thought to be important for recovering the tensile strengthof the tissue and to shield intact parts of the central nervoussystem (CNS)¹ from secondary injury (Ridet et al., 1997). Theastrocytic scar is very compact, which has led to the suggestionthat it may act as a physical barrier to axonal growth. Therole of scar formation in axonal regeneration has, however,been difficult to establish and remains controversial (reviewedin Frisén, 1997 and Ridet et al., 1997).

Various types of insults to the CNS, such as mechanical injury,lead to high level expression of the intermediate filament (IF)proteins glial fibrillary acidic protein (GFAP) and vimentinin astrocytes (Eddleston and Mucke, 1993). In response to injury,astrocytes also express a third IF protein, nestin (Lendahl et al., 1990;Clarke et al., 1994; Frisén et al., 1995; Lin et al., 1995).These changes in IF protein expression result in increaseddensity of IFs within the cells.

IFs of immature astrocyte precursors and astrocytes have beenshown to be composed of nestin and vimentin (Schnitzer et al., 1981;Bignami et al., 1982; Lendahl et al., 1990). As astrocytesmature, GFAP becomes expressed and vimentin expression decreases,in some astrocytes to undetectable levels (Bovolenta et al., 1984;Pixley and de Vellis, 1984). Many glial cells, such as astrocytesin the corpus callosum and hippocampus, tanycytes and Bergmann glia coexpress GFAP and vimentin in the adult animal (de Vitry et al., 1981;Lazarides, 1982).

IFs have been implicated in many cellular processes in differenttissues. Mutations in keratin genes result in skin blisteringdiseases and desmin deficiency leads to reduced tensile strengthin muscle cells (Li et al., 1997; Fuchs and Cleveland, 1998).These examples demonstrate a role for IFs in providing mechanicalstrength to certain types of cells. The role of IFs in astrocyteshas been difficult to establish. Manipulation of GFAP expressionlevels in vitro by overexpression or by the application ofantisense oligonucleotides has implicated GFAP in astrocyteprocess formation and in growth regulation (Weinstein et al., 1991; Rutka and Smith, 1993; Toda et al., 1994). However, mutantmice in which the GFAP (Gomi et al., 1995; Pekny et al., 1995;McCall et al., 1996) or vimentin (Colucci-Guyon et al., 1994)genes have been inactivated appear grossly normal. Detailedanalyses of GFAP–/– mice have revealed signs ofaltered neuronal function (Shibuki et al., 1996; McCall et al., 1996)and some GFAP–/– mice show late-onset CNS dysmyelinationand locally impaired blood-brain barrier function (Liedtke et al., 1996).We have studied the ability of cultured astrocytes to instruct vascular endothelial cells to develop blood-brain barrier propertiesin vitro and found that astrocytes from GFAP–/–mice failed to do so (Pekny et al., 1998a). Using primary culturesfrom GFAP–/– mice, we found that the ability ofastrocytes to extend processes in response to contact withneurons was preserved, but proliferation was increased in suchcultures (Pekny et al., 1998b).

Vimentin null mice have a reduced capacity to regulate vasculartone when challenged by ablation of renal tissue (Terzi et al., 1997).Furthermore, in the absence of vimentin, astrocyte IFs are composedsolely of GFAP and form abnormally compact bundles (Eliasson,C., C.-H. Berthold, and M. Pekny, unpublished data). Scar formationafter CNS injury appears normal in both GFAP–/–or vimentin–/– mice (Pekny et al., 1995; Galou et al., 1996). Similarly, GFAP–/– mice exhibit normal responseto scrapie infection (Gomi et al., 1995; Tatzelt et al., 1996). However, it is likely that GFAP and vimentin in part have overlapping functions and that one protein may be able to compensatefor the lack of the other protein in mutant mice.

We have generated mice carrying null mutations in both theGFAP and vimentin genes (GFAP–/–vim–/–)and observed that GFAP–/–vim–/– astrocyteslacked IFs completely in quiescent and reactive states in vivoas well as in vitro (Eliasson, C., C.-H. Berthold, and M. Pekny, unpublished data). GFAP–/–vim–/– micecan therefore be used to evaluate potential roles of IFs inastrocytic responses to injury. Here, we compared the reaction to mechanical brain or spinal cord injury in wild-type, GFAP–/–,vimentin–/–, or GFAP–/–vim–/–mice. We demonstrate that GFAP–/–vim–/–mice exhibit abnormal glial scar formation in response to injuryin the CNS.

Materials and Methods

Top
Abstract
Materials and Methods
Results
Discussion
References

Animals
Mice with null mutations in the GFAP (Pekny et al., 1995) orvimentin (Colucci-Guyon et al., 1994) genes were crossed togenerate double mutants. These mice reached adulthood and didnot display any overt anatomical or behavioral defects. Genotypeswere determined as described (Colucci-Guyon et al., 1994; Pekny et al., 1995).All the mice used in these studies were on C57BL/129 mixedgenetic background and were maintained in a conventional animalfacility.

Spinal Cord and Brain Injuries
Mice subjected to spinal cord or brain injury were killed shortlyafter the injury (2 or 3 d) or were allowed to survive for2 or 3 wk. In one group of animals the spinal cord dorsal funiculuswas transected at the upper thoracic level, and the injury wasextended 5 mm rostrally by a longitudinal incision (Frisén et al., 1992).In other animals, a 27-G needle was inserted through the skulland into the frontal cerebral cortex. After both types of injury,wild-type, GFAP–/–, or vimentin–/– animalsdid not display any recognizable symptoms after any of thelesions. The following number of animals were used for thespinal cord injury studies (shown as number of animals allowedto survive 2 d, 2 wk): wild-type (n = 10, 5), GFAP–/– (n = 8, 4), vimentin–/– (n = 2, 2), and GFAP–/–vim–/–(n = 3, 3). For the brain injury, these animals were used (shownas number of animals allowed to survive 3 d, 3 wk): wild-type(n = 3, 3), GFAP–/– (n = 4, 3), vimentin–/–(n = 2, 2), and GFAP–/–vim–/– (n = 5,3).

Nestin Immunohistochexmistry
Tissues were fixed by transcardial perfusion of anesthetizedmice with Tyrode's solution followed by 4% formaldehyde and0.4% picric acid in PBS or immersion fixation in Bouin's fixative(75 ml of saturated picric acid, 5 ml of glacial acetic acid,25 ml of 40% formaldehyde). Specimens were cryo-sectioned orembedded in paraffin and sectioned using a microtome. Sectionsfrom all animals were stained with hematoxylin and erythrosin/eosin (HE) using standard protocols. Immunohistochemistry with rabbitantiserum to nestin (no. 130, diluted 1:2,000; Dahlstrand et al., 1992;Tohyama et al., 1992) was performed as described (Frisén et al., 1995;Pekny et al., 1998b). Binding of primary antibodies was visualizedwith Cy2-conjugated donkey anti–rabbit antibodies (JacksonImmunoResearch) or HRP-conjugated goat antiserum against rabbitimmunoglobulins (Dako A/S). Peroxidase was detected with DAB(Dako A/S). Photomicrographs were scanned and mounted usingAdobe Photoshop.

In Situ Hybridization
Nestin mRNA expression in the injured spinal cord was detectedby in situ hybridization using digoxigenin labeled cRNA probesas described by Schaeren-Wiemers and Gerfin-Moser (1993). Theanimals were allowed to survive 4 d after the incision in thedorsal funiculus. The antisense probe was prepared with T3RNA polymerase from a NotI linearized plasmid containing amouse nestin cDNA corresponding to nucleotides 1630–2972(according to GenBank accession number M34384) and the senseprobe was generated with T7 polymerase from the same plasmidlinearized with XhoI. No specific hybridization was seen withthe sense probe.

Detection of Bromodeoxyuridine and S-100
Two mice of each genotype were used for the bromodeoxyuridine(BrdU) incorporation experiments. 1 h after the brain injury,which was performed as described above, the mice were injectedi.p. with BrdU (100 µg/g body weight). The injectionswere repeated 17 times for 50 h; injections were applied everysecond hour with a 10-h injection-free window each night. Themice were anesthetized and transcardially perfused with 0.1M phosphate buffer followed by 4% paraformaldehyde. Vibratomeor frozen sections were used for either simultaneous or sequentialdetection of BrdU and S-100. For BrdU detection sections weretreated with 2 M HCl for 30 min followed by 0.25% pepsin in0.1 M HCl for 2 min at 37°C before incubation with theprimary antibody. Mouse monoclonal antibody (M0744) and goatanti–mouse FITC-conjugated antibody (F0479; both DakoA/S) were used. For S-100 immunodetection, rabbit anti–cowS-100 antibody (Z311) was used followed by swine anti-rabbitTRITC-conjugated antibody (R0156; both Dako A/S).

Electron Microscopy
The following genotypes and number of mice were used for ultrastructural analysis: wild-type (n = 4), GFAP–/– (n = 3), vimentin–/–(n = 2), and GFAP–/–vim–/– (n = 3).3 d after a cortical stab wound, the mice were anesthetizedand transcardially perfused with Tyrode's solution followed by 500 ml of a solution containing 2% paraformaldehyde and2% glutaraldehyde dissolved in PBS. After postfixation overnight,the tissues were cut on an Oxford Vibratome and osmicated for4 h, dehydrated in acetone, and embedded in Vestopal W. Ultra-thinsections (80–100 nm thick) were cut from injured braincortex of all animals using an LKB Ultrotome. These sectionsmeasured 1.5 x 0.4 mm and included at one side the wound, coveredthe reaction zone, and displayed compact neuropile at the oppositeside. The sections were picked up on Formvar-coated one-slot copper grids, contrasted with lead citrate (Reynolds, 1963)and uranyl acetate, and examined in a Philips EM 400 electronmicroscope.

Morphological Measurements
Blood vessel diameters were measured in cross sections of thoracicspinal cord segments in a microscope fitted with a scale inthe eyepiece. The smallest distance across an individual bloodvessels was assigned as the diameter of the blood vessel. Thedistance from the dorsal spinal cord surface to the bottom ofthe indentation in the dorsal funiculus was considered as thedepth of the indentation below the superficial dorsal vessel (dorsal spinal vein). The genotypes of the animals were unknownto the person performing the measurements. Blood vessel diametersand dorsal funiculus indentations were measured in at leastsix animals of each genotype and at least 4 sections were analyzedfrom each animal. The average number of blood vessels widerthan 15 µm per section and the average depth of the indentationin the dorsal spinal cord was calculated for each animal, andwere used to calculate the mean and standard error of the meanfor animals of each genotype. Statistical significance was testedby Student's two-tailed t test. The differences were consideredsignificant if the P values were lower than 0.01.

Results

Top
Abstract
Materials and Methods
Results
Discussion
References

Dilated Blood Vessels and Altered Nestin Expression in Endothelial and Ependymal Cells
We first analyzed the uninjured nervous system of the mutantmice. Many blood vessels appeared dilated in the brain andspinal cord of GFAP–/–vim–/– mice (Fig.1). The lumina of these structures were lined with von Willebrandfactor–immunoreactive endothelial cells indicating thatthey were true blood vessels rather than, for example, cavitiesformed by degeneration (data not shown). Measurements of bloodvessel diameters in these mice revealed an almost threefoldincrease in the number of blood vessels with a diameter >15µm compared to wild-type mice (P < 0.0005; Fig. 2 A).We frequently noticed that there was an unusually deep indentationin the tissue of the dorsal spinal cord in many of the mutantmice. In wild-type mice, there is often an invagination belowthe dorsal spinal vein, but measurements of the depth of the invagination revealed a statistically significant increasein the depth compared to wild-type mice in GFAP–/–(P < 0.005), vimentin–/– (P < 0.0001), andGFAP–/–vim–/– mice (P < 0.0001;Figs. 2 B and 6, A–D).

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Figure 1 Blood vessel dilation. Hematoxylin and eosin stained coronal brain sections from wild-type (A) and GFAP–/–vim–/– (B) mice show an increased number of large diameter blood vessels in GFAP–/–vim–/– mice (some are indicated by arrowheads in B). The lumen of the lateral ventricle is indicated with an asterisk and the corpus callosum is labeled cc. Bar, 500 µm.

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Figure 2 Quantification of blood vessel dilation and the indentation below the dorsal spinal vein. (A) Average number of blood vessels with a diameter greater than 15 µm in spinal cord sections of mice of different genotypes. (B) Depth of the indentation in the spinal cord dorsal funiculus. Bars indicate SEM.

Endothelial and ependymal cells in the adult CNS express bothnestin (Dahlstrand et al., 1992; Frisén et al., 1995;Fig. 3 A) and vimentin (Franke et al., 1979), but not GFAPin wild-type mice. Nestin-immunoreactivity (IR) in these cellsappeared normal in GFAP–/– mice (data not shown).However, in vimentin–/– mice, nestin-IR was reducedto very low levels in both endothelial and ependymal cells (Fig.3 B). Moreover, nestin-IR did not display a filamentous patternbut was spread diffusely throughout the cytoplasm in thesecells (Fig. 3 B). The same nestin-IR pattern was seen in GFAP–/–vim–/–mice (data not shown).

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Figure 3 Altered nestin-IR in the absence of vimentin. Immunofluorescence localization of nestin in the uninjured spinal cord. (A) In a wild-type mouse, strong nestin-IR is seen in ependymal cells and endothelial cells. (B) Nestin-IR is weak and diffuse in vimentin–/– mouse. The arrows indicate the localization of the central canal. Bar, 100 µm.

Defective Glial Scar Formation after Spinal Cord Injury in GFAP–/–vim–/– Mice
We next analyzed scar formation in wild-type and mutant micein response to an incision in the spinal cord dorsal funiculus.The mice were allowed to survive 2 d or 2 wk after the injury,and tissue sections from the site of the injury and from aspinal cord segment 10 mm rostral to the lesion were analyzed.There were no consistent differences in the histology of thescar tissue between wild-type, GFAP–/–, or vimentin–/–mice revealed by HE staining (Fig. 4). However, the scar tissuewas much less dense in the GFAP–/–vim–/–mice, and the scar tissue was interrupted by numerous fissuresmost often running in a dorso-ventral orientation (Fig. 4,H and L). These fissures were filled with blood, tissue fluidor debris (Fig. 4 L). Moreover, in the GFAP–/–vim–/–animals there was a large number of red blood cells withinthe scar tissue, both 2 d and 2 wk after the injury, indicatingmore pronounced bleeding and/or defective clearance of bloodfrom the injury site (Fig. 4, H and L).

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Figure 4 Structure of the uninjured and injured spinal cord in wild-type and mutant mice. The micrographs show hematoxylin and eosin stained transverse sections of upper thoracic spinal cord from uninjured animals and from animals in which the dorsal funiculus was transected 2 wk before analysis. The arrows in C and D indicate invaginations in the dorsal funiculus. In I–L, details indicated by hatched boxes in E–H are shown at higher magnification. The injured area is demarcated by arrowheads in I. Note the abundance of erythrocytes at the injury in H and L. Bars: (H) 300 µm; (L) 100 µm.

Nestin Expression in the Injured Spinal Cord
Nestin expression is rapidly induced in astrocytes after CNSinjury and serves as a sensitive marker for reactive astrocytes(Clarke et al., 1994; Frisén et al., 1995; Lin et al., 1995).Nestin-IR was induced in response to spinal cord injury in miceof all genotypes (Fig. 5). However, nestin-IR was more restrictedin vimentin–/– or GFAP–/–vim–/– mice compared to wild-type or GFAP–/– mice (Fig.5). Whereas 2 d after the injury nestin-IR cells were seenat the site of the lesion and in the surrounding gray matterin wild-type (Frisén et al., 1995) or GFAP–/–mice, nestin-IR was less pronounced in the gray matter in vimentin–/– or GFAP–/–vim–/– mice (Fig. 5). Furthermore,2 wk after the lesion the levels of nestin-IR in the scar were lower in vimentin–/– or GFAP–/–vim–/–mice compared to wild-type or GFAP–/– mice (Fig.5). Whereas the scar tissue appeared dense after 2 wk in wild-type, GFAP–/– or vimentin–/– mice, the labeledcells were more sparse in GFAP–/–vim–/–mice and nestin-IR was diffusely spread throughout the cytoplasmof the cells (Fig. 5). Nestin-IR was induced within 2 d afterthe injury in segments rostral to the lesion, in the degeneratingaxonal tract, to a similar extent in mice of all genotypes (Fig. 6). However, 2 wk after the injury the level of nestin-IR in the degenerating tract had decreased substantially in the vimentin–/– or GFAP–/–vim–/–mice, whereas it remained strong in wild-type or GFAP–/–mice (Fig. 6).

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Figure 5 Nestin-IR at a spinal cord lesion in wild-type and mutant mice. Nestin-IR in the uninjured spinal cord and 2 d or 2 wk after a dorsal funiculus incision. Nestin-IR is induced at the injury in mice of all genotypes, but is weaker and more diffuse in vimentin–/– and GFAP–/–vim–/– mice compared with wild-type and GFAP–/– mice in E–P. The location of the central canal is indicated by arrows in A, E, and I. The arrow in D points at an indentation in the dorsal funiculus. The arrowheads in E indicate the approximate area affected by the injury. The arrows in L mark a fissure in the dorsal funiculus. The areas indicated by hatched boxes in I–L are shown at higher magnification in M–P. Bars: (L) 100 µm; (P) 30 µm.

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Figure 6 Nestin-IR in degenerating axonal tracts in wild-type and mutant mice. Nestin-IR in sections taken 10 mm rostral to a dorsal funiculus incision 2 d or 2 wk after the injury. Nestin-IR is induced in astrocytes in the dorsal and central part of the dorsal funiculus (indicated by arrowheads in A and E) due to Wallerian degeneration. The induction of nestin-IR is more transient in vimentin–/– or GFAP–/–vim–/– mice compared with wild-type or GFAP–/– mice. The arrows in A and E indicate the location of the central canal and the arrows in B–D, G, and H point at invaginations in the dorsal funiculus. The dorsal spinal vein located in the invagination is often destroyed during tissue processing but can be seen in D and G. A few wide blood vessels are indicated by arrowheads in G. Bar, 100 µm.

To determine whether the reduced nestin-IR in the injured spinalcord was caused by reduced transcription of the nestin genein vimentin–/– and GFAP–/–vim–/– mice, we performed in situ hybridization with nestin antisenseriboprobes in spinal cord sections from animals that underwenta dorsal funiculus incision 4 d before. Nestin mRNA was detectedin mice of all genotypes, and no reduction in nestin mRNA levelscould be found in vimentin–/– and GFAP–/–vim–/–mice (Fig. 7). Scattered cells in the dorsal funiculus expressednestin mRNA and their distribution was highly reminiscent ofthe nestin-IR pattern. No specific hybridization was seen withthe sense probe (Fig. 7, E and F).

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Figure 7 Nestin mRNA expression in the injured spinal cord. A digoxigenin labeled riboprobe was used to localize nestin mRNA in the spinal cord 4 d after an incision in the dorsal funiculus. Nestin mRNA is expressed in scattered cells at the injury site in wild-type (A), GFAP–/– (B), vimentin–/– (C), and GFAP–/– vim–/– mice (D). The micrographs show details from the dorsal funiculus. No specific hybridization was seen with sense probes in adjacent sections from wild-type (E) or GFAP–/–vim–/– (F) mice. Bar, 50 µm.

Responses to Brain Injury
Glial scar formation was also analyzed in the brain. A corticalstab wound was done with a fine needle, resulting in a muchmore restricted injury than the spinal cord lesion. Interestingly,3 out of 11 GFAP–/–vim–/– mice died shortly after the injury and the necropsy showed extensive intracranial bleeding that was interpreted as the cause of death (data not shown). In the group of GFAP–/–vim–/– mice that were killed 3 d after the injury, 3 out of 5 mice showed extensive bleeding at the site of injury (Fig. 8 D). Bleeding of comparable magnitude was not seen in mice of othergenotypes. In all wild-type, GFAP–/– and vimentin–/–mice, as well as in the GFAP–/–vim–/– mice that survived the operation, the discrete injury causedby the needle did not cause any apparent clinical symptomsand was sealed within 3 wk (Fig. 8). Nestin-IR was detectedaround the cortical lesion 3 d after the injury in mice ofall genotypes (Fig. 8). However, whereas nestin-IR was comparablystrong and revealed distinct reactive astrocytes in both wild-typeand GFAP–/– mice, it was weaker and diffuse invimentin–/– and GFAP–/–vim–/– mice (Fig. 8, G and H). Nestin-IR was reduced to undetectablelevels after 3 wk in mice of all genotypes (data not shown).

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Figure 8 Response to cortical injury in wild-type and mutant mice. Hematoxylin and erythrosin staining and nestin-IR in adjacent sections of frontal cortex from mice 3 d or 3 wk after a fine needle cortical injury. In most of GFAP–/–vim–/– mice 3 d after the injury, bleeding was detected within the lesion zone (D). Nestin-immunoreactive cells can be seen in the lesion area in all animals 3 d after the injury, but the labeling appears weaker and more diffuse in the cells of vimentin–/– and GFAP–/–vim–/– mice (G and H). The injury was sealed in animals of all genotypes 3 wk after this type of injury (I–L). Bar, 100 µm.

Ultrastructural Analysis of Scar Formation
To further characterize scar formation in the mutant mice, we analyzed the zone immediately adjacent to the central necroticarea of cortical injury by electron microscopy. This area wassimilar in wild-type, GFAP–/–, or vimentin–/–mice, but differed in GFAP–/–vim–/–mice. The difference was most apparent in the border zone between the severely disarranged tissue close to the wound and the more distant, compact and normal looking brain tissue. Here,the GFAP–/–vim–/– mice exhibited fragmented tissue with a high accumulation of extracellular debris. Thisdebris was diffuse, finely granular or filamentous of moderateelectron density (Fig. 9 d). This was in contrast to mice ofthe other genotypes (Fig. 9, a–c) in which the braintissue in the corresponding area showed easily identifiablecomponents (e.g., myelinated and unmyelinated axons, synaptosome-likeprofiles), narrow extracellular spaces and virtually no extracellulardebris.

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Figure 9 Ultrastructural analysis of a cortical stab wound. Electron micrographs of the frontal cerebral cortex 3 d after the injury. The pictures show the border zone between the spongy tissue of the wounded area and the surrounding compact cortical tissue. In wild-type (A), GFAP–/– (B), or vimentin–/– (C) mice, the extracellular space (small asterisk) is restricted and free of debris. In GFAP–/– vim–/– mice the extracellular space is filled with masses of filamentous and diffuse debris (large asterisk). A, astrocytic profile; M, myelinated axon; S, synaptosome-like profile. Bar, 1 µm.

Cell Proliferation after the Cortical Injury
To evaluate cell proliferation in the area affected by the cortical injury we have compared BrdU incorporation withina 50-h time window after the injury in wild-type, GFAP–/–,vimentin–/–, and GFAP–/–vim–/–mice. Using confocal microscopy we have counted BrdU-labeled cells within the volume of 5 x 10⁶ µm³ that includedthe injury area in the middle and was reconstructed from superimposedconfocal images. The number of BrdU-labeled cells within thisvolume ranged from 64 to 87 and no statistically significantdifferences were found between wild-type and mutant mice. Todetermine the proportion of astrocytes among the BrdU-labeledcells, S-100 positive cells were counted within the same volume.The number of S-100 positive cells ranged from 65 to 83 andno statistically significant differences were found betweenwild-type and mutant mice. Fig. 10 provides a comparison between individual (Fig. 10, a–d) and combined (Fig. 10, e andf) BrdU and S-100 immunostaining of the cortical injury area in wild-type and GFAP–/–vim–/– mice.Both contain comparable numbers of BrdU positive, S-100 positiveand double positive cells (some of these are indicated by arrows).Thus, the cortical injury in wild-type and mice deficient forGFAP and/or vimentin triggers a comparable induction of celldivision.

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Figure 10 Cell proliferation in the injury area in wild-type and mutant mice. Confocal images of BrdU labeling (A and B) and S-100 IR (C and D) in the area of brain cortical injury. No difference is apparent between wild-type and GFAP–/–vim–/– mice. Combined labeling reveals a proportion of double positive cells (E and F; some of them indicated by an arrow). Confocal pictures are maximal projections of superimposed images covering the thickness of 12 µm. Bar, 50 µm.

	Discussion

Top Abstract Materials and Methods Results Discussion References

The role of astrocytic IF proteins has been the subject of numerous studies, but has been difficult to establish. In thisstudy we have utilized mice carrying null mutations in theGFAP and/or vimentin genes. We found that GFAP and vimentinhave partly overlapping functions in the astrocytic responseto injury, and contribute to scar formation. Furthermore, bloodvessel dilation was seen in the brain and spinal cord of micelacking both vimentin and GFAP.

Altered Nestin Expression in Endothelial and Ependymal Cells and Dilation of Blood Vessels
In the nervous system of adult wild-type mice, nestin expressionis largely restricted to endothelial and ependymal cells (Dahlstrand et al., 1992;Frisén et al., 1995). Both of these cell types alsoexpress vimentin (Franke et al., 1979; Schnitzer et al., 1981).The nestin expression pattern was distinctly altered in vimentin–/–or GFAP–/–vim–/– mice. In wild-typeor GFAP–/– mice, nestin-IR in endothelial or ependymalcells exhibited a distinct pattern in contrast to the weakand diffuse nestin-IR seen in vimentin–/– or GFAP–/–vim–/–mice (Fig. 3 and data not shown). Analysis of reactive astrocytesin vivo and astrocytes in culture from GFAP–/–vim–/–mice revealed the lack of IFs in these cells in spite of nestinexpression, demonstrating that nestin fails to form IFs onits own in astrocytes (Eliasson et al., unpublished observations).The in situ hybridization data did not reveal any reductionin nestin mRNA expression in the spinal cord of vimentin–/–or GFAP–/–vim–/– mice compared to wild-type.This implies that the differences detected at the level of nestin-IR are posttranslational, probably caused by the changed equilibriumbetween unpolymerized and polymerized nestin in a situationwhen nestin polymerization cannot occur. This is further supportedby the results from the Northern blot analysis of the RNA fromastrocytes in vitro that showed rather an increase in nestintranscription in vimentin–/– and GFAP–/–vim–/–astrocytes (Eliasson et al., unpublished observations). Two-hybridanalysis has further indicated that nestin cannot bind to itselfand nestin also fails to form IFs in SW13 cells devoid of otherIF proteins, but incorporates into IFs once vimentin or desminis transfected into these cells (Sjöberg, G., and T. Sejersen,personal communication; Marvin et al., 1998). These data suggestthat the altered nestin-IR pattern observed in endothelialand ependymal cells in vimentin–/– or GFAP–/–vim–/–mice reflects the failure of nestin to form IFs in the absenceof other IF proteins also in these cells.

Many blood vessels were dilated in the brain and spinal cordin GFAP–/–vim–/– mice. Vimentin, butnot GFAP, is normally expressed both in endothelial cells andin perivascular cells such as pericytes and smooth muscle cells (Franke et al., 1979; Gabbiani et al., 1981). A reductionor lack of IFs in endothelial and perivascular cells may decreasethe mechanical strength of blood vessels and consequently theircapacity to withstand dilation. The observed increase in bloodvessel diameter in the CNS of GFAP–/–vim–/–mice may be caused by altered properties of endothelial or perivascularcells (as a consequence of vimentin absence in these cells)and a reduced capacity of the surrounding tissue to withstandblood vessel dilation (the consequence of absence of GFAP andvimentin in astroglial cells). Such a concept is supported by the finding of a progressively deeper indentation beneath the dorsal spinal vein in GFAP–/–, vimentin–/–,and in GFAP–/–vim–/– mice, respectively.

Defective CNS Scar Formation in GFAP–/–vim–/– Mice
Scar formation after a spinal cord or brain injury appeared comparable in wild-type, GFAP–/–, or vimentin–/– mice, but was defective in mice lacking both GFAP and vimentin,indicating that these proteins may have partly overlappingfunctions in this process. In such mice, the glial scar wasless compact, contained more debris compared to the mice ofthe other genotypes, and the scar tissue was disrupted by fissures.Using BrdU incorporation, we did not detect any differencesin cell proliferation in the injury area. Also, the amountof astrocytes, detected as S-100 positive cells, in the injuryarea was comparable between the mice of different genotypes.These results imply that even in GFAP–/–vim–/–mice, the injury results in a normal response at the levelof cell proliferation.

Major similarities exist between the epithelial response toinjury and reactive gliosis in the CNS. In both cases, productionof IF proteins accompanies cell activation and the processresults in the closure of the wound. In case of stratifiedepithelia, such as the epidermis of the skin, the wound closurehappens in an orchestrated action of keratinocyte migrationfrom the surrounding healthy tissue and a contraction of theconnective wound bed mediated by migrating fibroblasts (forreview see McGowan and Coulombe, 1998). Keratinocyte activationand migration parallel induction of the wound repair-associatedIF proteins in these cells, namely keratins 6, 16, and 17, which happens within 6–12 h after injury (Paladini et al., 1996). In the injured CNS, proliferation of stem cells is induced by injury, and the progeny of the stem cells migrate towardsthe injury where they differentiate to astrocytes (Johansson et al., 1999).Thus, cell migration and wound contraction may be phenomenaplaying a major role in wound closure in general. Our preliminaryexperiments suggest that in the scrape wounding assay in vitro,cultures of GFAP–/–vim–/– astrocytesrequire longer time to close the defect (unpublished data).Therefore, it is possible that reactive astrocytes withoutIFs exhibit a cell migration deficit. To address the contractileproperties of astrocytes from wild-type and GFAP and/or vimentindeficient mice, we investigated whether primary cultured astrocytesfrom these mice can contract collagen gels. All type of astrocyteswere able to contract the gels and no quantitative differencesbetween wild-type, GFAP–/–, vimentin–/–, and GFAP–/–vim–/– astrocytes were detected(data not shown).

The defective scar formation in GFAP–/–vim–/– mice may not only be a result of astrocytic dysfunction but may also relate to the abnormal blood vessels seen in these mice. It is unlikely that the blood vessel abnormality is the major reason for defective scar formation in these mice, sincescar formation appeared normal in vimentin–/– miceand only vimentin, and not GFAP, is expressed in cells of theblood vessel. The bleeding seen in GFAP–/– vim–/–mice therefore probably results from the combination of abnormalblood vessels and defective closure of the wound.

The amount of debris was clearly elevated in glial scar tissueof GFAP–/–vim–/– mice compared to miceof the other genotypes. This can either be a result of defectiveclearance of tissue debris or its increased production. Astrocytesare capable of phagocytosis and the abundance of debris inGFAP–/–vim–/– mice may result from impairmentof this function. Alternatively, the bleeding observed in GFAP–/–vim–/–mice may result in the formation of more debris in the formingglial scar and its immediate vicinity.

Multiple fissures traversed through the scar in the injuredspinal cord of GFAP–/–vim–/– mice. Thismay be a consequence of reduced astrocytic process formation with deficient bridging and sealing of the wound. Absence of IFs in astrocytes is likely to reduce the tensile strength of individual astrocytes, and as a consequence, of the tissue.A low resistance to mechanical forces is likely to inhibit scarformation, especially in the spinal cord that has to adaptto movements of the vertebral column, a situation distinctfrom that in the skull-enclosed brain. Irrespective of itscause, defective scar formation may lead to repeated tearingof the tissue and recurring bleeding, potentially explainingthe abundance of red blood cells in the scar tissue of GFAP–/–vim–/–mice. The defective glial scar formation in GFAP–/–vim–/–mice described here reveals the importance of GFAP and vimentinfor this process as well as a certain degree of functionaloverlap between these two proteins.

Acknowledgments

We wish to thank Dr. Kristofer Rubin for performing the collagengel contraction assays, Dr. Charles Babinet for providing thevimentin null mice, Dr. Martha Marvin for the gift of nestincDNA, Dr. Charles Babinet and Dr. Alain Privat for valuablediscussions, Ms. Ulrika Wilhemsson for genotyping some of theanimals, and Ms. Marianne Eriksson and Ms. Rita Grandérfor technical help with processing the tissue for electron microscopy.

This study was supported by grants from the Swedish MedicalResearch Council (project nos. 11548, 09041, 12183, and 03157),the Swedish Cancer Foundation (project no. 3622), the KingGustav V Foundation, the Swedish Society for Medicine, theSwedish Society for Medical Research, A⁺ Science Invest, StiftelsenSigurd och Elsa Goljes minne, Stiftelsen Lars Hiertas Minne,Björklunds fond, Jeanssons stiftelse, Ostermans stiftelse, Magnus Bergvalls stiftelse, Marcus Borgströms stiftelse,Tore Nilssons stiftelse, the Wenner-Gren foundations, ÅkeWibergs stiftelse, Kapten Arthur Erikssons fond, Inga-Brittand Arne Lundberg foundation, and Gustafsson foundation. M.Pekny was supported by a fellowship from the Swedish Societyfor Medical Research.

Submitted: 17 April 1998

Revised: 17 March 1999

The first three authors contributed equally to this study.

References

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Abstract
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References

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