Role of Tissue Plasminogen Activator Receptor LRP in Hippocampal Long-Term Potentiation

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The Journal of Neuroscience, January 15, 2000, 20(2):542-549

Role of Tissue Plasminogen Activator Receptor LRP in Hippocampal Long-Term Potentiation
Min Zhuo¹, David M. Holtzman²^,³, Yonghe Li⁴, Hiroshi Osaka⁴, Joe DeMaro², Mark Jacquin², and Guojun Bu⁴^,⁵
Departments of ¹ Anesthesiology, ² Neurology, ³ Molecular Biology and Pharmacology, ⁴ Pediatrics, and ⁵ Cell Biology and Physiology, Washington University School of Medicine, St. Louis, Missouri 63110

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The low-density lipoprotein (LDL) receptor-related protein (LRP) is a multifunctional endocytic receptor that is expressedabundantly in neurons of the CNS. Both LRP and several of itsligands, including tissue plasminogen activator (tPA), apolipoproteinE/lipoproteins, $alpha$ ₂-macroglobulin, and the $beta$ -amyloid precursorprotein, have been implicated in various neuronal functions andin the pathogenesis of Alzheimer's disease. It has been reportedthat induction of tPA expression may contribute to activity-dependentsynaptic plasticity in the hippocampus and cerebellum. In addition,long-term potentiation (LTP) is significantly decreased in micelacking tPA. Here we demonstrate that tPA receptor LRP is abundantlyexpressed in hippocampal neurons and participates in hippocampalLTP. Perfusion of hippocampal slices with receptor-associatedprotein (RAP), an antagonist for ligand interactions with LRP,significantly reduced late-phase LTP (L-LTP). In addition, RAPalso blocked the enhancing effect of synaptic potentiation byexogenous tPA in hippocampal slices prepared from tPA knock-outmice. Metabolic labeling and ligand binding analyses showed thatboth tPA and LRP are synthesized by hippocampal neurons and thatLRP is the major cell surface receptor that binds tPA. Finally,we found that tPA binding to LRP in hippocampal neurons enhancesthe activity of cyclic AMP-dependent protein kinase, a key moleculethat is known to be involved in L-LTP. Taken together, our resultsdemonstrate that interactions between tPA and cell surface LRPare important for hippocampal L-LTP.

Key words: LRP; tPA; LTP; PKA; Alzheimer's disease; hippocampus

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The low-density lipoprotein (LDL) receptor-related protein (LRP) is a large multifunctional endocytic receptor that belongsto the LDL receptor gene family (Herz et al., 1988; Krieger andHerz, 1994; Bu, 1998). It is highly expressed in neurons of theCNS and binds and endocytoses more than 10 structurally and functionallydistinct ligands, including apolipoprotein E (apoE)/lipoprotein, $beta$ -amyloid precursor protein (APP), and $alpha$ ₂-macroglobulin ( $alpha$ ₂M)(Krieger and Herz, 1994). Recently, several lines of evidencehave implicated LRP and LRP ligands in the pathogenesis of Alzheimer'sdisease (AD). A 39 kDa receptor-associated protein (RAP) functionsas a molecular chaperone during the folding process of LRP andas a receptor antagonist to prevent premature ligand interactionwith LRP during its trafficking within the secretory pathway (Buand Schwartz, 1998). Recombinant RAP has been used extensivelyas an antagonist in the study of LRP biology (Bu, 1998).

One of the most significant clinical symptoms of AD is memory loss. Thus, understanding the physiological mechanism of age-and AD-related memory loss may potentially provide clues as tohow this process can be intervened during aging and AD. Evi- dencefrom different studies demonstrates that the hippocampus and itsrelated temporal lobe structures are important for explicit formsof memory (Squire and Zola-Morgan, 1991). Long-term potentiation(LTP) is one of the best models for investigating cellular andmolecular mechanisms for memory formation and storage (Nicolland Malenka, 1995). In the CA1 region of the hippocampus, LTPhas two distinct phases: early-phase LTP (E-LTP) and late-phaseLTP (L-LTP). One unique feature making L-LTP different from E-LTPis that it requires new protein synthesis, activity of cAMP-dependentprotein kinase (PKA), and transcription (Frey et al., 1988, 1993,1995; Huang and Kandel, 1994; Nguyen et al., 1994; Nguyen andKandel, 1996; Qi et al., 1996) (for review, see Schuman, 1997).

Tissue plasminogen activator (tPA) has been identified as one of the immediate early genes induced by neuronal activity includingLTP (Qian et al., 1993). Under normal physiological conditions,tPA is widely expressed in the CNS (Qian et al., 1993; Bu et al.,1994; Seeds et al., 1995; Ware et al., 1995; Hayden and Seeds,1996). However, the level of tPA is finely regulated by its inhibitorand cell surface receptor LRP (Bu et al., 1992a,b; Orth et al.,1992), and its synthesis is increased by activators of the cAMP-PKApathway (Baranes et al., 1998). In the hippocampus, Qian et al.(1993) found that neuronal activity could induce the expressionof mRNA of tPA in pyramidal neurons. More interestingly, L-LTPbut not E-LTP is significantly decreased in mice lacking the geneencoding tPA (Carmeliet et al., 1994; Frey et al., 1996; Huanget al., 1996). These findings indicate that tPA plays an importantrole in L-LTP in the hippocampus. However, whether interactionbetween tPA and its cellular receptor LRP participates in L-LTPis unknown. Here, we present several lines of evidence indicatingthat interaction between tPA and LRP is important for hippocampalL-LTP.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Materials. Human recombinant tPA was kindly provided by Genentech (South San Francisco, CA). tPA was initially dissolved inarginine phosphate buffer and dialyzed against PBS before use(Bu et al., 1992a). Recombinant rat RAP was produced as fusionprotein with glutathione S-transferase (GST). The GST portionwas cleaved off, and RAP was repurified via heparin-Sepharosecolumn (Warshawsky et al., 1993). Polyclonal anti-human LRP [cross-reactswith mouse LRP; see Holtzman et al. (1995)], anti-rat RAP, andanti-human tPA [cross-reacts with mouse tPA; see Bu et al. (1992a)]antibodies have been described previously (Bu et al., 1992a,b,1993, 1994, 1995; Holtzman et al., 1995).

Hippocampal slice preparation. For LTP recordings, transverse slices of hippocampus (400 µm thick) were prepared from wild-type(C57BL/6J, 8- to 12-weeks-old; The Jackson Laboratory, Bar Harbor,ME) or tPA knock-out mice (C57BL/6J, 8-12 weeks old; The JacksonLaboratory). The slices were maintained between 28°C and 30°Cin a chamber where they were subfused with artificial CSF (ACSF)consisting of (in mM): 124 NaCl, 4.0 KCl, 2.0 CaCl₂, 1.0 MgSO₄,1.0 Na₂HPO₄, 24.1 NaHCO₃, 10 glucose, bubbled with 95% O₂, 5%CO₂. Slices were allowed to recover for at least 2 hr beforeexperiments.

Electrophysiology. A bipolar tungsten stimulating electrode was placed to evoke postsynaptic responses. Extracellular fieldpotentials were recorded with a glass microelectrode (3-12 M $Omega$ ,filled with ACSF). In some experiments, a second stimulating electrodewas placed to serve as an independent control response in thesame slice. The postsynaptic EPSPs were evoked at 0.02 Hz witha bipolar tungsten electrode placed at the CA3 region. The intensityof stimulation was decreased to evoke ~1 mV EPSP. Paired-pulsefacilitation was tested with different time intervals. The initialmagnitude of the first EPSP was adjusted to 1.0 mV by changingthe intensity of electrical stimulation. E-LTP was induced byone train tetanus consisting of one 100 Hz train for 1 sec attesting intensity (the intensity used for evoke baseline EPSPresponses). Four-train tetanic stimulation, consisting of four100 Hz trains for 1 sec at testing intensity with a 5 min intervalbetween trains, was used to induce L-LTP. Field recordings ofNMDA receptor-mediated EPSPs were performed in the presence of10 µM CNQX and 100 µM Mg²⁺. Data are presented as a mean value ± SEM or percentage changesfrom control. Statistical comparisons are made with the use ofeither two-way or one-way ANOVAs (Newman-Keuls test for post hoccomparison). Student's test was applied for comparisons betweenpaired groups. In all cases, p < 0.05 is consideredsignificant.

Ligand binding assay. Freshly prepared mouse hippocampal slices (see above) were used for binding analysis of ¹²⁵I-tPA (5 nM) in the absence or presence of unlabeled tPA (500nM) or RAP (500 nM) (Bu et al., 1992a, 1994). After 2 hr incubationat 4°C, slices were washed three times with cold buffer, and radioactivityassociated with each slice was determined. The slices were thenlysed with PBS containing 1% Triton X-100 for 1 hr at 4°C, andthe protein concentration was determined. Each experiment wasperformed in triplicate with SEM given as errorbars.

Primary hippocampal neuron cultures. Primary neurons from embryonic day 17-19 (E17-19) Swiss-Webster mouse embryos were preparedusing the method described previously (Narita et al., 1997). Inbrief, hippocampal neurons were mechanically dissociated aftertreatment with trypsin (0.5 mg/ml, 15 min, 37°C). Cells were thenplated onto poly-D-lysine (100 mg/ml)-coated six-well plates ata density of ~200 neurons per millimeters squared and maintainedin DMEM medium containing 5% horse serum, 5% fetal bovine serum,2 mM glutamine, at 37°C in a humidified 5% CO₂ incubator and used24 hr afterplating.

Ligand endocytosis assay. Hippocampal neurons were prepared and plated in 24-well plates. Binding of ¹²⁵I-tPA (5 nM) in the absence or presence of unlabeled RAP (500nM) was performed at 4°C for 2 hr as described previously (Buet al., 1992a, 1994). After washing at 4°C, some plates were warmedup to 37°C for the indicated time before returning to 4°C. RAP(500 nM) was included in the warm-up media to prevent rebindingof dissociated ligand. Cell monolayers were then treated with0.25% (w/v) Pronase (Calbiochem, La Jolla, CA) in PBS for 30 minat 4°C to remove the remaining cell surface-bound ligands (Buet al., 1992a). The solution that contained detached cells wasthen centrifuged at 4°C to pellet cells. Radioactivity associatedwith cell pellets represents internalized ligand, whereas radioactivityin the supernatant fraction represents surface-boundligand.

Metabolic labeling and immunoprecipitation. Neurons were metabolically labeled with 200 mCi/ml [³⁵S]methionine for 4 hr (Bu et al., 1992a). Both overlying mediaand cell lysates were then immunoprecipitated with either anti-tPAor anti-LRP antibody and analyzed via SDS-PAGE (7.5% acrylamide).Coimmunoprecipitation experiments of RAP and tPA were performedin the absence of detergent as described previously (Bu et al.,1995).

PKA assay. PKA activity was determined by using the PKA assay system from Life Technologies/BRL (Gaithersburg, MD). Hippocampalneurons were incubated with serum-free media without or with tPA(50 nM), or with tPA (50 nM) and RAP (500 nM) for 20 min at 37°C.After washing two times with ice-cold PBS, cell monolayers werescraped and homogenized in extraction buffer containing 1 mM 3-isobutyl-1-methylxanthineand protease inhibitor cocktail (Complete, Boehringer Mannheim,Indianapolis, IN) (Goretzki and Mueller, 1998). After removalof cell debris via centrifugation, PKA activity was determinedaccording to the manufacturer'sinstructions.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

It has been reported that induction of tPA expression may contribute to activity-dependent synaptic plasticity in the hippocampusand cerebellum (Qian et al., 1993; Seeds et al., 1995). In addition,L-LTP is significantly decreased in mice lacking tPA (Huang etal., 1996). Although the mechanism of tPA's involvement in L-LTPis unknown, the importance of its interaction with cell surfacereceptors has been suspected. To test whether the interactionof tPA with its endocytic receptor LRP participates in L-LTP,we examined the potential effects of the LRP antagonist RAP onL-LTP. Hippocampal slices from mice were perfused with eitherbuffer alone or buffer containing RAP, followed by induction ofL-LTP. We found that application of RAP resulted in an inhibitionof synaptic potentiation induced by a four-train tetanic stimulation(n = 7) (Fig. 1A). The effect of RAP is dose-related, becauseperfusion with a lower concentration of RAP produced a smallerinhibition (n = 5) (Fig. 1B). RAP itself did not significantlyaffect baseline EPSPs (n = 5) or potentiate EPSPs applied at 10min after the delivery of four-train stimulation (n = 3). In someexperiments, a second electrode was placed at the other side ofthe first electrode, and synaptic responses were tested beforeand 1 hr after the four-train stimulation. Synaptic responsesat this second independent pathway were not significantly affected(n = 3).

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Figure 1. LRP is important for hippocampal L-LTP. A, L-LTP is abolished by RAP pretreatment (0.5 µM, closed squares). L-LTP recorded with buffer alone is shown with open squares. Four-train stimulation is marked with arrowheads. Inset, Traces of EPSPs indicating that 40 min after the induction of L-LTP, hippocampal potentials with RAP treatment have returned to those of baseline. B, RAP at a lower concentration (50 nM) produces a smaller inhibition. C, RAP (0.5 µM, closed squares) does not affect E-LTP induced by one-train stimulation. E-LTP recorded with buffer alone is shown with open squares. D, Synaptic responses to a paired-pulse stimulation at different intervals (25, 50, 75, and 100 msec) are not affected by RAP (0.5 µM, closed squares). Open squares are recordings with buffer alone. E, RAP does not affect NMDA receptor-mediated EPSPs. F, The input-output curves of NMDA receptor-mediated EPSPs in control medium (open squares) and medium containing RAP (0.5 µM, closed squares).

In contrast to L-LTP, potentiation induced by one-train stimulation was not significantly affected by RAP perfusion (n = 5)(Fig. 1C), indicating that LRP is not required for E-LTP. In addition,neither presynaptic fiber volley (Fig. 1E) nor the paired-pulsefacilitation was affected by RAP treatment (Fig. 1D). Finally,NMDA receptor-mediated responses were not significantly affectedby RAP (Fig. 1E,F), indicating that RAP did not produce its effectthrough inhibition of NMDA receptors. The small changes of thefiber volley of responses in the recordings shown are mostly likelyattributable to population responses recorded, because in theseexperiments the NMDA receptor-mediated currents were not affected,and the stimulation intensities were not changed over the entirerecordingperiod.

The inhibition of L-LTP by RAP mimics the abnormalities found in hippocampal slices of tPA knock-out mice (Huang et al., 1996),except that a complete disappearance of L-LTP in tPA knock-outmice requires 2 hr, whereas inhibition by RAP is seen within 40min from the start of induction. Thus, although other ligandsof LRP may also participate in L-LTP, we suspected that tPA waslikely the major ligand whose interaction with LRP contributedto L-LTP. To directly assess whether interaction between tPA andLRP is important for L-LTP, we tested whether exogenous tPA canenhance synaptic potentiation in hippocampal slices of tPA knock-outmice and whether RAP could block this effect. Consistent witha previous report (Huang et al., 1996), synaptic potentiationinduced by multiple tetanic stimulation was significantly decreasedin tPA knock-out mice (n = 3). Application of tPA induced concentration-dependentpotentiation. At a concentration of 10 nM, tPA produced a slightincrease in potentiation, whereas at 50 nM, exogenous tPA inducedsignificant potentiation (n = 6) (Fig. 2). To examine whetherthe enhancement by tPA is mediated via its receptor LRP, we testedthe effect of RAP. As seen in Figure 2, tPA-induced potentiationwas completely blocked by pretreatment of slices with RAP (0.5µM) for 30 min (n = 6). These results strongly suggest that tPAparticipates in L-LTP through its interaction with cell surfaceLRP. We also examined the potential effect of tPA on NMDA receptors.Application of tPA for an identical time period did not significantlyaffect NMDA receptor-mediated EPSCs (n = 3) (data not shown).

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Figure 2. tPA-induced synaptic potentiation is blocked by RAP in tPA knock-out mice. A, Traces of EPSPs before and 60 min after 50 nM tPA application in the absence (left) or presence of 0.5 µM RAP (right). B, RAP pretreatment (0.5 µM, open squares) blocked synaptic potentiation induced by tPA. EPSPs in the absence of RAP pretreatment are indicated by filled squares. Application of 50 nM tPA is indicated by a bar.

To exclude the possibility that RAP interacts directly with tPA and interferes with tPA function, we examined whether thetwo proteins interact with one another. First, we incubated RAPand tPA under conditions similar to those used in the electrophysiologicalexperiments and immunoprecipitated the mixture with normal rabbitIgG, anti-tPA IgG, or anti-RAP IgG. The immunoprecipitated materialswere then Western-blotted with either anti-tPA IgG or anti-RAPIgG (Fig. 3A). As seen in the figure, anti-tPA antibody did notcoimmunoprecipitate RAP in a mixture of tPA and RAP. Similarlyanti-RAP antibody did not coimmunoprecipitate tPA. In the secondexperiment, we examined the ability of RAP-Sepharose to bind ¹²⁵I-tPA. We have used this RAP-Sepharose previously to precipitateLRP and purify specific anti-RAP IgG (Bu et al., 1995). The resultshows that RAP-Sepharose does not bind ¹²⁵I-tPA (Fig. 3B). These results clearly show that RAP does notinteract with tPA. Thus, the results we obtained with RAP perfusionin our electrophysiological experiments are consistent with RAPantagonizing tPA's interaction with LRP.

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Figure 3. RAP does not interact directly with tPA. A, RAP (1 µg) and tPA (1 µg) were incubated in ACSF for 1 hr at 30°C. The incubation mixture was then divided and incubated with normal rabbit IgG (NR), anti-tPA IgG, or anti-RAP IgG, followed with immunoprecipitation (IP) without detergent. The immunoprecipitated materials were then immunoblotted (IB) with either anti-tPA IgG or anti-RAP IgG. B, RAP-Sepharose was incubated with ¹²⁵I-tPA (5 nM) in ACSF for 1 hr at 30°C. After washing, both supernatant (S) and pellet (P) were analyzed via SDS-PAGE.

Both LRP and a mannose receptor have been shown to bind tPA (Otter et al., 1991; Bu et al., 1992b). In addition, several studieshave described various tPA binding receptors on the cell surfaceof both endothelial and neuronal cells (Pittman et al., 1989;Verrall and Seeds, 1989; Hajjar et al., 1994; Fukao and Matsuo,1998). However, only binding to LRP is inhibited by RAP (Bu etal., 1998). To determine which of these receptors plays a rolein tPA binding to hippocampal neurons, we performed binding analysisof ¹²⁵I-tPA to hippocampal slices. The binding experiments were performedin the absence or presence of excess unlabeled tPA or RAP. Asseen in Figure 4A, RAP inhibited ¹²⁵I-tPA binding to hippocampal slices to the same extent as unlabeledtPA, suggesting that specific binding of tPA to hippocampal slicesis mediated primarily via LRP.

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Figure 4. LRP is the major endocytic receptor for tPA expressed in hippocampal neurons. A, Fresh hippocampal slices are prepared and used for binding analysis of ¹²⁵I-tPA (5 nM) in the absence or presence of unlabeled tPA (500 nM) or RAP (500 nM). The experiment was performed in triplicate, with error bars representing SEM. RAP inhibits ¹²⁵I-tPA binding to hippocampal slices to the same extent as unlabeled tPA, suggesting that binding of tPA to hippocampal slices is mediated entirely via LRP. B, Hippocampal neurons were prepared and plated in 24-well plates. Binding of ¹²⁵I-tPA (5 nM) in the absence or presence of unlabeled RAP (500 nM) was performed at 4°C for 2 hr. Some plates were then warmed up to 37°C for either 5 or 10 min before returning to 4°C. Cell monolayers were then treated with 0.25% (w/v) Pronase for 30 min at 4°C to remove remaining cell surface-bound ligands. Radioactivity associated with cell pellets represents internalized ligand, whereas radioactivity in the supernatant fraction represents surface-bound ligand. Data represent LRP-mediated endocytosis after subtraction of those in the presence of excess RAP. The experiment was performed in triplicate, error bars representing SEM.

To examine whether LRP serves as an tPA endocytic receptor in neuronal cells similar to its role in hepatoma cells, we analyzedthe kinetics of LRP-mediated tPA binding and uptake with primarycultured hippocampal neurons. First, we performed a saturationbinding analysis of ¹²⁵I-tPA on primary cultured neurons and found that there were ~52,000tPA-binding sites/neuron (data not shown) (Bu et al., 1992a, 1993).We then examined the kinetics of ¹²⁵I-tPA uptake by hippocampal neurons. ¹²⁵I-tPA (5 nM) was first allowed to bind to neurons at 4°C in theabsence or presence of excess RAP. Some plates were then warmedup to 37°C for either 5 or 10 min, followed by analysis of cellsurface and intracellular ligand distribution (Bu et al., 1992a,1993). As shown in Figure 4B, nearly 80% of cell surface-boundtPA had been endocytosed after 5 min of 37°C incubation. Thesekinetics of tPA internalization by LRP in neurons are similarto what we observed with hepatoma cells (Bu et al., 1992a, 1993)and suggest that LRP functions as an endocytic receptor for tPAinneurons.

To further examine the potential function of tPA and LRP, we analyzed the expression of tPA and LRP in hippocampal neurons.Primary cultured hippocampal neurons from E17 mouse embryos weremetabolically labeled with [³⁵S]cysteine for 4 hr. Both cell lysates and overlying media werethen immunoprecipitated with either anti-tPA antibody or anti-LRPantibody, followed by analysis via SDS-PAGE. As seen in Figure5A, both tPA and LRP are detected in cell lysates, demonstratingthat mouse hippocampal neurons synthesize both tPA and its receptorLRP. The immunoprecipitation condition (including 1% SDS) doesnot preserve any potential interaction between endogenous tPAand LRP, and thus potential interaction between these two proteinsis not detected in this experiment. tPA is also detected in theoverlying media, suggesting that tPA is actively secreted by theseneurons and could potentially function extracellularly. We alsodetected complexes of tPA with its physiological inhibitor plasminogenactivator inhibitor type-1 (PAI-1), which can either be producedby hippocampal neurons or be present as residual protein fromserum used to culture neuronal cells. The abundant expressionof LRP seen in these experiments is consistent with our previousstudies on the distribution of LRP in the hippocampus, which showedstrong immunoreactivity of LRP in hippocampal neurons and theirprocesses (Holtzman and Fagan, 1998).

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Figure 5. tPA and LRP expression in hippocampal neurons and activation of PKA. A, Primary cultured hippocampal neurons from E17 mouse embryos were metabolically labeled with [³⁵S]cysteine for 4 hr. Both cell lysates (C) and overlying media (M) were immunoprecipitated with either anti-tPA antibody or anti-LRP antibody, followed by analysis via SDS-PAGE (7.5% acrylamide) and autoradiography. LRP is abundantly expressed in these neurons, whereas tPA is synthesized and secreted by these neurons. A band corresponding to the migration of tPA/PAI-1 complexes is also detected. The molecular size markers are given in kilodaltons. B, Binding of tPA to LRP enhances PKA activity. Primary hippocampal neurons were incubated without or with tPA (50 nM) or tPA (50 nM) and RAP (500 nM) at 37°C for 20 min. Cell lysates were then assayed for PKA activity. Results are averages of triplicate determinations, error bars representing SEM. *p < 0.05 compared with no treatment control.

Several studies have shown that cAMP and PKA play important roles in L-LTP (Qi et al., 1996; Abel et al., 1997). A recentstudy by Goretzki and Mueller (1998) has shown that binding ofLRP with its ligand lactoferrin or uPA/PAI-1 complex in a humanmelanoma cell line caused a significant elevation of cAMP andPKA activity. In addition, tPA was found to induce endothelialcell proliferation by activating PKA (Welling et al., 1996). Thus,we examined whether tPA binding to LRP in hippocampal neuronsalso activates the cAMP/PKA pathway. As shown in Figure 5B, PKAactivity was significantly increased when hippocampal neuronswere incubated with exogenous tPA (50 nM). In addition, the activationof PKA activity by tPA was attenuated in the presence of excessRAP. These results suggest that the cAMP/PKA pathway is at leastone of the intracellular events activated by tPA-LRPinteractions.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In the current study, we present evidence showing that interaction of tPA with its cell surface receptor LRP appears to playan important role in hippocampal L-LTP. Perfusion of hippocampalslices with LRP antagonist RAP significantly and rapidly abolishedhippocampal L-LTP. In addition, RAP also abolished the enhancingeffects of exogenous tPA on synaptic transmission in hippocampalslices of tPA knock-out mice. We also present evidence that LRPis abundantly expressed in hippocampal neurons and is the majortPA receptor present on the cell surface. Finally, we demonstratedthat tPA binding to LRP in hippocampal neurons increases PKA activity,an intracellular signaling pathway that is known to be involvedin L-LTP.

tPA is a serine protease that catalyzes the conversion of plasminogen to plasmin and degrades certain components of extracellularmatrix (Lijnen and Collen, 1991). tPA activity is regulated viaboth inactivation by its inhibitor PAI-1 and cellular clearanceby cell surface LRP. A recent study has suggested that tPA inhibitorscan block the function of tPA in L-LTP (Baranes et al., 1998).However, our current studies demonstrated that binding of tPAto its cell surface receptor LRP plays an important role in L-LTP.Thus, it is possible that L-LTP is maintained by both intracellularsignaling events (e.g., Ca²⁺ influx, PKA activation, etc.) and extracellular structural changes(e.g., synaptic growth, synaptic connections). The former events(intracellular signaling) may be triggered by tPA binding to LRP,whereas tPA's protease activity may contribute to structural changesthat associate with L-LTP and learning and memory (Baranes etal., 1998). Because binding of tPA to LRP does not require itsprotease activity (Bu et al., 1992a,b; Orth et al., 1994), itis possible that the receptor binding function and the proteaseactivity of tPA have distinct roles in neuronal plasticity andother neuronal activity. In support of this hypothesis, a recentstudy has demonstrated a nonproteolytic function by tPA in neuroprotection(Kim et al., 1999). Alternatively, inhibitors of tPA proteaseactivity such as PAI-1 may alter the way tPA interacts with LRP,which in turn blocks the signaling events induced by interactionof LRP with native tPA. Toward this possibility, it is interestingto note that studies by Willnow et al. (1994) and Orth et al.(1994) have shown that tPA and tPA/PAI-1 complexes bind to overlappingbut not identical sites within the second domain ofLRP.

Several previous studies have suggested the presence of tPA binding protein on the cell surface that might serve as a dockingreceptor for tPA (Pittman et al., 1989; Verrall and Seeds, 1989;Hajjar et al., 1994; Fukao and Matsuo, 1998). However, our currentstudy suggests that tPA is rapidly endocytosed by LRP after itsbinding to the receptor, suggesting that LRP likely functionsas an endocytosis/signaling receptor as opposed to a docking receptor.This function of LRP is similar to those of neurotrophin receptors,which on binding of neurotrophin trigger both endocytosis andsignal transduction. In the case of NGF binding to its receptortrkA, it is interesting to note that studies by Grimes et al.(1996) have shown that trkA continues to signal after endocytosisvia "signaling endosomes," as a means of retrograde signalingfrom distal axons to the neuronal cell body. Thus, the major eventsoccurring after tPA interaction with LRP on neurons may includeboth endocytosis and signal transduction. The later event maylink to intracellular signaling pathways involved in L-LTP. Takentogether, we propose the following model regarding how the tPA/LRPpathway might participate in L-LTP in the CA1 region of the hippocampus(Fig. 6).

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Figure 6. Schematic model of tPA/LTP pathway in L-LTP. See Discussion.

During the induction of LTP, postsynaptic depolarization induced by tetanic stimulation removes Mg²⁺ blockade of NMDA receptors at postsynaptic cells. Ca²⁺ influx through the NMDA receptor channels activates a seriesof postsynaptic signaling pathways, including action on adenylylcyclase and production of a second messenger cAMP. cAMP then activatesPKA, which in turn activates various intracellular pathways andimmediate early genes, including that of tPA. As a result, thesynthesis of tPA in the ER is increased. After trafficking throughthe secretory pathway, tPA is secreted into extracellular spacewhere it either functions in extracellular matrix as a proteasein synaptic plasticity (Baranes et al., 1998) or binds to itscell surface receptor LRP (which can be antagonized by RAP) andactivates cellular processes that enhance synaptic potentiation,as demonstrated in the current study. The later process may bea result of intracellular signaling events (e.g., further activationof PKA) on tPA-LRP interaction and/or regulation of the AMPA receptor.Potential signaling functions of LRP have been suggested fromvarious observations. First, several studies have shown that apoE3,a ligand of LRP, increases neurite extension via LRP (Bellostaet al., 1995; Holtzman et al., 1995; Narita et al., 1997). Second,our previous studies have shown that negative feedback regulationof tPA gene expression in colon fibroblasts is mediated via tPAinteraction with cell surface LRP (Hardy et al., 1997). Third,recent studies have shown that the LRP tail interacts with a heterotrimericGTP-binding protein (Goretzki and Mueller, 1998) and two cytoplasmicadaptor proteins, FE65 and mammalian Disabled (Trommsdorff etal., 1998).

Gene-disruption studies by Herz et al. (1992) have concluded that LRP is essential for early mouse embryonic development.Embryos homozygous for LRP deficiency do not survive long enoughto allow examination of LRP's role during neuronal development,although some developmental neuronal delay was observed in homozygousLRP knock-out embryos (Herz et al., 1993). Recent studies haveshown that functional cell surface LRP is required for normalhippocampal neuronal process development and growth in vitro (Naritaet al., 1997). In addition, a recent study using a genetic approachdemonstrated that two members of the LDL receptor family, thevery low density lipoprotein receptor and apoE receptor 2, playimportant roles in neuronal migration and hippocampal development(Trommsdorff et al., 1999). Thus, it is possible that tPA-LRPinteraction is essential during neuronal development, similarto its role in L-LTP as described in the currentstudy.

Additionally, genetic and other evidence suggest that at least three LRP ligands $---$ apoE/lipoprotein, APP, and $alpha$ ₂M $---$ are likelyto play important roles in the pathogenesis of AD. First, LRPis the major neuronal receptor for apoE/lipoproteins (Bellostaet al., 1995; Holtzman et al., 1995; Fagan et al., 1996), andthe $epsilon$ 4 allele of apoE is a strong genetic risk factor for AD (Corderet al., 1993; Strittmatter et al., 1993). Second, immunoreactivityfor several LRP ligands (e.g., apoE, $alpha$ ₂M, and tissue factor pathwayinhibitor), as well as LRP itself, has been found in senile plaques(Abraham et al., 1988; Rebeck et al., 1995; Hollister et al.,1996). Third, LRP has been shown to mediate the endocytosis ofboth secreted and transmembrane forms of APP (Kounnas et al.,1995; Knauer et al., 1996), suggesting that LRP may play a rolein the metabolism of APP and in some way modify the generationof amyloid peptides. Fourth, several recent studies (Kang et al.,1997; Lendon et al., 1997; Hollenbach et al., 1998) have reporteda possible association between polymorphisms within the LRP geneand AD. Finally, studies by Blacker et al. (1998) and Liao etal. (1998) identified a genetic association between polymorphismswithin $alpha$ ₂M and risk of AD. In sum, it is possible that regulationof LRP expression in CNS neurons can directly impact the catabolismand functions of its ligands, such that decreased uptake and signalingor increased extracellular accumulation of these ligands, or both,lead to the neuropathological changes associated with AD. Theseresults indicate that LRP and its interactions with some of itsligands may play an important role in neuronal function and inthe pathogenesis of neurological diseases. Disruption of theseinteractions may lead to neuronal impairment, including some ofthose seen in AD. Our current results provide the first evidencethat an interaction between tPA and LRP plays an important rolein L-LTP, a form of synaptic plasticity that is believed to contributeto learning and memory (Hawkins et al., 1993; Moser et al., 1998).Our biochemical and cellular analyses as well as previous work(Qian et al., 1993; Seeds et al., 1995; Huang et al., 1996) confirmthe presence of these molecular components within hippocampalneurons, indicating that these molecules are likely to participatein synaptic potentiation in vivo.

Although our analyses with apoE-knock-out mice did not show any abnormality in L-LTP (data not shown), it is interesting tonote that mice expressing the C terminus of APP (Nalbantoglu etal., 1997) or APP₆₉₅SWE (Chapman et al., 1999) had impaired learningand decreased LTP. In addition, a recent study has found impairedsynaptic transmission in the hippocampus of mice overexpressinga mutant form of APP (717_V-F), which preceded amyloid depositionby several months (Hsia et al., 1999). These results togetherwith our present study suggest that cellular components (e.g.,LRP, tPA, APP) that are important for synaptic transmission couldbe disrupted independent of amyloid plaque formation during agingandAD.

  FOOTNOTES

Received Sept. 9, 1999; revised Oct. 22, 1999; accepted Oct. 22, 1999.

This work was supported by National Institutes of Health (NIH) Grant NS37525 and a Faculty Scholar Award from Alzheimer'sAssociation to G.B., NIH Grant AG13956 to D.H., and a grant fromthe Alzheimer's Disease Research Center at Washington UniversitySchool of Medicine to M.Z. We thank Masaaki Narita for preparationof primary hippocampal neurons and Alan Schwartz for criticalreading and comments on thismanuscript.
Correspondence should be addressed to Dr. Guojun Bu, Department of Pediatrics, Washington University School of Medicine, CB8116, One Children's Place, St. Louis, MO 63110. E-mail: bu{at}kids.wustl.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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