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Previous Article | Next Article
The Journal of Neuroscience, March 15, 2002, 22(6):2125-2134
Localization and Regulation of the Tissue Plasminogen Activator-Plasmin System in the Hippocampus
Fernando J. Sallés and Sidney Strickland Laboratory of Neurobiology and Genetics, The Rockefeller University, New York, New York 10021
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
The extracellular protease cascade of tissue plasminogen activator (tPA) and plasminogen has been implicated in neuronal plasticity and degeneration. We show here that unstimulated expression of tPA in the mouse hippocampus is concentrated in the mossy fiber pathway, with little or no expression within the perforant path, the Schaffer collaterals, or neuronal cell bodies. tPA protein is also expressed in vascular endothelial cells throughout the brain parenchyma. Four hours after excitotoxic injury, tPA protein is transiently induced within CA1 pyramidal neurons. The induced CA1 tPA is localized to neurons that survive the injury and is enzymatically active. Within the mossy fiber pathway, injury resulted in decreased tPA protein. In contrast, mossy fiber tPA activity displayed a biphasic character: transient increase at 8 hr, then a decrease by 24 hr after injury. Analysis of plasminogen activator inhibitor-1 (PAI-1) expression showed that PAI-1 antigen is upregulated by 24 hr and could account for the tPA activity downregulation seen at this time point. Plasminogen immunohistochemistry suggested an increase within the mossy fiber pathway after injury. Finally, hippocampal tPA expression among various mammalian species was strikingly different. These results indicate a complex control of tPA protein and enzymatic activity in the hippocampus that may help regulate neuronal plasticity.
Key words: tissue plasminogen activator (tPA); hippocampus; plasminogen activator inhibitor 1 (PAI-1); mossy fiber pathway; excitotoxic injury; protease; mouse; rat; human; hamster; gerbil; cat; synaptic plasticity
INTRODUCTION
Extracellular proteases are expressed by neurons in the CNS (Sappino et al., 1993
; Chen et al., 1995
Protease expression is balanced by proteolytic inhibitors (Festoff et al., 1996
Tissue plasminogen activator (tPA) is a serine protease that catalyzes the activation of plasminogen to plasmin. Previous experiments suggest the following model for tPA expression in adult neurons: tPA is synthesized under basal conditions and is stored in vesicles (Baranes et al., 1996
To better understand the localization and regulation of the PA-plasmin system within the CNS, we have identified several antibodies that have allowed us to localize the expression of tPA, PAI-1, and plasminogen in the hippocampus after excitotoxic injury. Our results suggest a more restricted expression of tPA within in the CNS than previously recognized and a complex regulatory pathway that includes control both of tPA expression and activity.
MATERIALS AND METHODS
Reagents and animals. Antibodies used were as follows: rabbit anti-human tPA antisera (Waller and Schleuning, 1985
/
Immunohistochemistry. Mouse, rat, and gerbil brain tissue was obtained from ice-cold PBS-perfused animals. All tissue was frozen in optimal cutting temperature compound under powdered dry ice, sectioned to 14 µm, and stored at
In situ zymography. Zymography to detect tPA was performed essentially as described by Sappino et al. (1993)
In situ hybridization. In situ hybridizations were performed using a modified version of the method of Hebert et al. (1991)
Stereotaxic injections. Intrahippocampal injections in mice were performed unilaterally as described previously (Tsirka et al., 1997
RESULTS
tPA is abundantly expressed in the mossy fiber pathway
Expression and localization of tPA protein were visualized using a rabbit polyclonal antibody (Waller and Schleuning, 1985
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Figure 1. tPA is abundantly expressed in the mossy fiber pathway. A, B, tPA immunohistochemistry on wild-type (wt) sections shows robust tPA staining (red) in the hippocampal mossy fiber pathway. Sections are counter-stained with hematoxylin to visualize the neuronal cell body layers of the hippocampus. DG, Dentate gyrus; MF, mossy fiber pathway; n = 20 animals. C, D, tPA immunostain without the hematoxylin counterstain showing lack of significant staining within the neuronal cell bodies (compare high-magnification B with D). Arrows in D highlight vascular endothelial cell staining that is seen throughout the brain. E, F, tPA immunohistochemistry on wild-type sections after preabsorbing the antibody (Figure legend continues.) (Figure legend continued.) with tPA as described in Materials and Methods. Notice the loss of mossy fiber and vascular staining but residual background parenchymal stain; n = 7 animals. G, tPA immunohistochemistry on tPA-deficient (tPA
Outside of the hippocampus, robust tPA staining could be observed in vascular tissue throughout the brain (Fig. 1D, arrows) and in the meninges as well as in the neuropil of the central nucleus, the bed nucleus, and the hypothalamus (data not shown). We did not find robust staining within microglia. The reasons for the discrepancy between this lack of staining and previous results that found microglial expression of tPA (Tsirka et al., 1997
tPA is upregulated in CA1 neurons after excitotoxic injury
Because we could not find significant tPA staining in the CA1 region in basal conditions, we examined tPA expression after excitotoxic injury. After unilateral kainic acid (KA) injection, tPA antigen was upregulated in CA1 neuronal cell bodies, consistent with its characterization as an immediate early gene (Qian et al., 1993
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Figure 2. tPA is upregulated in CA1 neurons after excitotoxic injury. A, After a weak excitotoxic injury (between 0.3 and 0.6 nmol of KA in a 300 nl volume, depending on lot potency), at 8 hr after injury tPA protein is upregulated in neuronal cell bodies within the CA1 layer (arrow); n = 18 animals, with 14 showing some level of staining. These neurons occupy the border of surviving and degenerating neurons as seen in the adjacent section (B) stained with Nissl (arrow). Degenerating neurons are visualized as having pyknotic nuclei versus the surviving neurons that appear normal. C, After a robust injury (between 0.9 and 1.2 nmol of KA in a 300 nl volume, depending on lot potency), at 8 hr after injury tPA protein is strongly upregulated within some neuronal cell bodies of the contralateral uninjected hippocampus (arrows); n = 16 animals, with 8 showing significant staining. Inset, Magnification of several pyramidal neurons within the CA1 showing cytoplasmic tPA accumulation. Note that not all CA1 neurons upregulate tPA. D, This upregulated protein is active, as measured by the zymographic analysis. Contralateral CA1 tPA expression was seen when treated with sufficient KA to destroy ~80% of ipsilateral hippocampus. In two animals, we could detect both ipsilateral and contralateral CA1 staining.
A time course revealed that the tPA induction was transient. On average, tPA protein staining could be detected by 2.5 hr, peaking between 5 and 8 hr and returning to baseline by 24-48 hr after injection (Fig. 3). Despite the variability in tPA induction noted above, in all cases, tPA staining was barely detectable by 24-48 hr (Fig. 3E). Subcutaneous administration of KA also produced tPA upregulation in the CA1 (data not shown).
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Figure 3. Time course of tPA induction in CA1 neurons after injury. Results show transiently upregulated neuronal cell body tPA in CA1 pyramidal neurons after injury in the contralateral uninjected hippocampus after a robust excitotoxic lesion. Sections were counterstained with hematoxylin to visualize the neuronal cell layer. Notice the lack of pyknotic nuclei and neuronal degeneration. A, No significant tPA staining is seen in the CA1 layer of control animals; n = 20 animals. B, CA1 neuronal cell layer 2.5 hr after lesion; n = 4 animals. C, tPA staining is induced 5 hr after injury (red staining within neuronal cell layer); n = 4 animals. D, tPA staining seen at 8 hr after injury; n = 8 animals. E, Forty-eight hours after injury, tPA is no longer detectable within the cell layer, yet the neurons still appear healthy; n = 4 animals. Additional time points assayed were 1 and 24 hr (data not shown).
To determine whether tPA protein upregulation was attributable to increased tPA mRNA, in situ hybridization was performed. These analyses revealed no detectable tPA mRNA staining under basal conditions in any region of the brain (Fig. 4A) even after long development periods for the in situ detection (>3 weeks). Our actin and laminin controls for mRNA detection robustly developed overnight (data not shown), indicating appropriate hybridization sensitivity. Eight hours after KA injection, however, when a strong upregulation of CA1 tPA antigen was detected, we could easily detect a strong induction of tPA mRNA in all pyramidal layers within a 3 d development period (Fig. 4B). Two lines of evidence indicate that the analysis is specific for tPA mRNA: (1) results were consistent using three different tPA mRNA probes (see Materials and Methods); and (2) tPA hybridization on brain sections from tPA-deficient animals was negative (Fig. 4C).
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Figure 4. tPA mRNA is strongly upregulated after excitotoxic injury in the contralateral uninjected CA1 pyramidal neurons by in situ hybridization. tPA mRNA was not detectable in control animals (n = 10; A) or tPA
Modulation of mossy fiber tPA activity by protease inhibitors
In wild-type samples (data not shown) and control PBS-injected samples, tPA protein staining (Fig. 5A) and activity levels (Fig. 5B) were equivalent in the ipsilateral (open arrows) and contralateral (closed arrows) hippocampus. By 8 hr after unilateral KA injection into CA1 neurons, we observed a consistent decrease in tPA protein staining in the ipsilateral mossy fiber pathway compared with the contralateral side (Fig, 5C, compare open, closed arrows). Surprisingly, tPA activity was transiently elevated in the injected side at this time point (Fig. 5D, open vs closed arrows). This increased activity coincides with the decrease in antigen staining, suggesting the downregulation of protease inhibitor activity between 0 and 8 hr after injection. At 24 hr after injury, tPA immunostaining (Fig. 5E) was the same as that observed at 8 hr, yet the level of tPA activity decreased to barely detectable levels for both sides of the hippocampus (Fig. 5, compare F, open, closed arrows, with B, open, closed arrows). This decrease in activity at 24 hr occurs despite the normal level of tPA protein staining in the contralateral control hippocampus (Fig. 5E, closed arrow) and the decreased but detectable level of tPA antigen in the ipsilateral hippocampus. This observation suggests that between 8 and 24 hr after injury, a protease inhibitor is upregulated within the hippocampus. PBS control injections showed no alteration in tPA protein staining or activity at either 8 or 24 hr after injection (8 hr, data not shown; 24 hr, Fig. 5A,B). Together, our evidence indicates a biphasic inhibitor profile: transient downregulation of protease inhibitor(s) by 8 hr with upregulation by 24 hr.
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Figure 5. Modulation of protease inhibitor activity in the hippocampus after excitotoxic injury. The dashed arrow represents the site of excitotoxin injection. A, C, E, G, tPA protein staining; B, D, F, H, tPA activity zymographies performed on sections adjacent to those displayed for protein stains. A, B, Control PBS-injected wild type brain harvested 24 hr after injection; n = 6 animals. C, D, KA-injected brain harvested 8 hr after injection; n = 6 animals. E, F, KA-injected brain harvested 24 hr after injection; n = 6 animals. High-level upregulation of CA1 tPA protein was not seen in this experiment (see Fig. 2 legend). G, H, KA-injected brain from a PAI-1
We analyzed whether PAI-1, a specific tPA inhibitor, could account for the biphasic nature of the inhibitory activity by assessing tPA regulation after excitotoxic injury in the hippocampus of PAI-1-deficient animals. There were no obvious differences in KA-induced neuronal death between the wild-type and PAI-1
To further analyze the expression of PAI-1, we screened for the presence of PAI-1 antigen using a polyclonal antibody raised in sheep (Fig. 6) in wild-type animals. Neither under basal conditions nor at 8 hr after injury could we detect significant specific PAI-1 protein staining in the brain (Fig. 6A,B) compared with control PAI-1
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Figure 6. PAI-1 upregulation in the hippocampus after excitotoxic injury. Ipsilateral injected hippocampus was immunostained for PAI-1. The dashed arrow represents the site of excitotoxin injection. A, Control PBS-injected wild-type brain harvested 24 hr after injection; n = 6 animals. B, KA-injected brain harvested 8 hr after injection; n = 6 animals. C, KA-injected brain harvested 24 hr after injection (SO, stratum oriens); n = 6 animals. D, KA-injected brain from a PAI-1
In an attempt to identify the presumptive proteolytic inhibitor whose activity is downregulated in the ipsilateral hippocampus at 8 hr after injury, we immunostained for neuroserpin, a serine protease inhibitor known to be expressed in hippocampal neurons. Under basal conditions, neuroserpin could be detected mostly in neuronal cell bodies, with no detectable staining within the mossy fiber pathway. At 8 hr after injury, there was a slight increase in staining within CA1 neurons of the injected hippocampus, and at later time points, staining was lost in the degenerating cell bodies. These data suggest that neuroserpin is not modulating the observed tPA activity upregulation seen (data not shown).
It is important to note that protease activities visualized in brain sections reflect the balance between proteases and inhibitory activity. Local proteolysis could be uncontrolled in pathological situations because of discrete compartmentalization. Sectioning and zymographic analyses could allow two localizations separated in vivo to intermingle through physical disruption. Additionally, it was possible that the increase in tPA activity seen at 8 hr after injection was attributable to release of vesicularly localized tPA. To test this hypothesis, we performed the in situ zymographies in the presence of 0.1 and 0.5% Triton X100 or saponin to promote vesicular tPA liberation. These treatments yielded a slightly more diffuse appearance to the zones of lysis but did not alter the lytic zone localizations or the overall level of activity (data not shown), indicating that the increase in tPA activity seen was not attributable to vesicular release.
Plasminogen expression after excitotoxic injury
Plasminogen is present at high concentrations in the blood and in the extracellular space of most tissues. However, little is known about the concentration of plasminogen in the basal neuropil and how that might change after injury. We used a sheep polyclonal antibody against rat plasminogen to determine the expression profile of plasminogen after injury. We could detect little to no plasminogen in wild-type brain tissue (PBS-perfused) when compared with immunostains of Plgn
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Figure 7. Expression of plasminogen in the hippocampus after excitotoxic injury. The dashed arrow represents the site of excitotoxin injection. A, Plasminogen immunostain on KA-injected wild-type brain section 8 hr after injection. Open arrows highlight areas of intense staining; n = 6 animals. B, Plasminogen immunostain on plg
Because this observed plasminogen staining could originate from a vascular source due to blood-brain barrier breakdown or from local protein synthesis, we analyzed vascular leakage by staining for IgG in the neuropil, the traditional marker for blood-brain barrier breakdown (data not shown). Using this assay, we could not exclude the possibility that the detected plasminogen was derived from vascular leakage, because the plasminogen staining pattern was always a subset of the visualized IgG staining (data not shown).
Basal high-level tPA mossy fiber expression varies among species
To determine whether our observed staining pattern of tPA expression in the hippocampus was consistent among different species, we first stained adult (300 gm) Sprague Dawley rat coronal brain sections using the tPA antibody to determine the expression of tPA in rat hippocampus. Surprisingly, the rat mossy fiber pathway does not express significant levels of tPA under basal conditions (Fig. 8A). The antibody used cross-reacts with rat antigen, as evidenced by the robust staining in the vascular endothelium (Fig. 8A, open arrows). The staining was also determined to be specific by immunodepletion using tPA-Sepharose (data not shown). This absence of basal mossy fiber tPA staining was corroborated by the lack of mossy fiber tPA activity, as measured by in situ zymography (Fig. 8B). A previous report had shown that tPA activity was upregulated in the rat hippocampus by KA injection into the ventricle in a pattern reminiscent of mossy fiber expression (Nagai et al., 1999
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Figure 8. Rat mossy fiber pathway is devoid of significant tPA staining but is upregulated after excitotoxic injury. A, tPA protein is seen primarily in vascular endothelial cells. The dotted line shows the position of hippocampal neuronal cell layers. Filled arrows point to the mossy fiber pathway, where no significant tPA staining is detected. Open arrows point to tPA-stained vascular endothelium; n = 6 animals. B, In situ zymography assay showing tPA activity and lack of any detectable activity in the mossy fiber pathway. C, tPA protein staining is upregulated (open arrow) in a portion of the mossy fiber pathway 8 hr after stereotaxic KA injection into the CA1 region (dotted arrow); n = 8 animals, with 5 showing some level of tPA upregulation.
We then examined a variety of other species to analyze the expression of tPA. Gerbil and hamster brains both expressed high basal levels of tPA in the mossy fiber pathway, whereas cat and human brains did not (data not shown). These differences in species staining led us to test a variety of mouse strains to see whether there were differences in hippocampal tPA staining among lines of mice. All strains tested basally expressed tPA specifically in the mossy fiber pathway.
DISCUSSION
Our results demonstrate that tPA protein and activity are concentrated in the mossy fiber pathway within the mouse hippocampus. This localization is essentially identical to the activity localization reported previously (Sappino et al., 1993
We therefore reasoned that the tPA mRNA in the CA1 may be under translational control, in which the mRNA would be continually present but only translated after significant activity or injury, providing rapid protease production. In oogenesis, tPA mRNA is under translational control (Huarte et al., 1987
Previous work has shown CA1 hippocampal neurons to be extremely sensitive to tPA-mediated excitotoxin-induced degeneration (Tsirka et al., 1995
So why are CA1 pyramidal neurons most sensitive to tPA-mediated excitotoxin-induced degeneration? There are several possible explanations. First, tPA might be expressed below the level of detection, and it is this low-level tPA that is crucial for CA1 neuronal degeneration. Second, cell death is likely to be attributable to a confluence of many factors, because we know that tPA overexpression alone is not sufficient to kill neurons (Tsirka et al., 1996
Chen et al. (1997)
Why is tPA so highly expressed under basal conditions in the mossy fiber pathway? Several studies suggest that a major role of tPA in neurons is synaptic plasticity (Frey et al., 1996
If protease expression is required for structural modifications during synaptic plasticity, a releasable "resident" protease may be required at all synaptic terminals to allow appropriate extracellular matrix modifications. There may be a variety of proteases with different inhibition characteristics, target protein specificities, and downstream signaling capabilities that participate in different synapse types, e.g., tPA and plasminogen in mossy fibers leading to CA3 neurons and neuropsin in Schaffer collaterals leading to CA1 neurons. It is quite possible that variations in neuronal protease expression alter circuitry as well as learning and memory characteristics. Interestingly the lack of significant tPA expression in the rat mossy fiber pathway may confer different electrophysiological, structural, or behavioral characteristics on mossy fibers between rats and mice. Additionally, under basal conditions, rat mossy fiber terminals might express high levels of a protease other than tPA.
Neuronal extracellular proteolytic activity when improperly released within a pathological setting may lead to excessive matrix modification and subsequent neuronal death. This is exemplified by experiments showing that loss of tPA or plasminogen conferred neuronal protection after excitotoxic injury (Tsirka et al., 1995
FOOTNOTES Received Sept. 18, 2001; revised Nov. 29, 2001; accepted Dec. 12, 2001.
This work was supported by National Institutes of Health Grants NS35704 and NS38472. We thank Katerina Akassoglou, Sarah Baker, Stephanie Bury, Zu-Lin Chen, Duane Day, Dennis Dickson, Andy Lee, Rime Mahdavi, Charles Ouimet, Ed Reich, Irene Solomon, Andre Stutz, Stella Tsirka, and the Strickland laboratory for helpful discussions and reagents. We are grateful to Robert Pawlak for very helpful comments on this manuscript.
Correspondence should be addressed to Dr. Fernando Sallés, Cogent Neuroscience, Inc., 4321 Medical Park Drive, Durham, NC 27704. E-mail: fsalles{at}cogentneuroscience.com.
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