Distribution of a Lysosomal Enzyme in the Adult Brain by Axonal Transport and by Cells of the Rostral Migratory Stream

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The Journal of Neuroscience, August 1, 2002, 22(15):6437-6446

Distribution of a Lysosomal Enzyme in the Adult Brain by Axonal Transport and by Cells of the Rostral Migratory Stream
Marco A. Passini, Edward B. Lee, Gregory G. Heuer, and John H. Wolfe
Department of Pathobiology and Center for Comparative Medical Genetics, School of Veterinary Medicine, University of Pennsylvania, and Division of Neurology, Children's Hospital of Philadelphia, Philadelphia, Pennsylvania 19104

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

A portion of the lysosomal enzymes produced by cells is secreted, diffuses through extracellular spaces, and can be takenup by distal cells via mannose-6-phosphate receptor-mediated endocytosis.This provides the basis for treating lysosomal storage diseases,many of which affect the CNS. Normal enzyme secreted from a clusterof genetically corrected cells has been shown to reverse storagelesions in a zone of surrounding brain tissue in mouse diseasemodels. However, low levels of enzyme activity and reduction ofstorage lesions also have been observed at sites in the brainthat may not be explained by a contiguous gradient of secretedenzyme diffusing away from the genetically corrected cells. Nodirect evidence for alternative mechanisms of enzyme transporthas been shown, and little is understood about the intracellularmovement of lysosomal enzymes in neurons. We investigated whetheraxonal transport could occur, by expressing an eukaryotic lysosomalenzyme that can be visualized in tissue sections ( $beta$ -glucuronidase)in brain structures that have defined axonal connections to otherstructures. This resulted in the transfer of enzyme to, and areversal of storage lesions in, neurons that project to the geneexpression site, but not in nearby structures that would havebeen corrected if the effect had been mediated by diffusion. Inaddition, transduction of cells in the subventricular zone resultedin the uptake of $beta$ -glucuronidase by cells entering the rostralmigratory stream. Gene transfer to specific neuronal circuitsor cells in migratory pathways may facilitate delivery to theglobal brain lesions found in thesedisorders.

Key words: adeno-associated virus; $beta$ -glucuronidase; septohippocampal system; axonal transport; rostral migratory stream; lysosomal storage disease; gene therapy

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The lysosomal storage diseases are a family of ~50 inherited disorders, most of which are caused by mutations in lysosomalacid hydrolase genes (Neufeld, 1991). The loss of these catabolicenzymes results in the accumulation of substrate in cells of theCNS and other organ systems, which eventually leads to lysosomedistention and loss of cellular function (Walkley, 1998). In thecase of mucopolysaccharidosis type VII (MPS VII), a homozygousnull mutation of the $beta$ -glucuronidase (GUSB) gene in mice resultsin the accumulation of glycosaminoglycans in neurons and glialcells throughout the brain (Birkenmeier et al., 1989; Vogler etal., 1990).

A feature of most lysosomal enzymes is that they are secreted into the extracellular space and taken up by other cells ina receptor-mediated endocytosis process called cross-correction(Neufeld and Fratantoni, 1970; Sando and Neufeld, 1977; Taylorand Wolfe, 1994). This mechanism has been shown in the MPS VIImouse brain to reverse storage lesions in neural cells surroundinga graft of genetically corrected fibroblasts (Taylor and Wolfe,1997). Direct intraparenchymal brain injections with several typesof viral vectors also have been effective (Ghodsi et al., 1998;Skorupa et al., 1999; Stein et al., 1999; Bosch et al., 2000a,b;Sferra et al., 2000; Zhu et al., 2000; Consiglio et al., 2001;Frisella et al., 2001). The sphere of enzyme-positive cells foundsurrounding the injection site is attributable to diffusion, butsome types of viruses also can move to distal sites by retrogradeaxonal transport where they express the transferred gene (Ghodsiet al., 1998; Stein et al., 1999; Zhu et al., 2000). However,the presence of low levels of enzyme activity and some correctionof storage in distal sites, including the contralateral hemisphere,have been observed with vectors that transduce cells only at thesite of injection (Skorupa et al., 1999; Bosch et al., 2000a,b;Consiglio et al., 2001). This suggests that the enzyme proteinitself may be transported. If lysosomal enzymes can be transportedwithin the CNS, transducing selected structures may help to distributethe therapeutic protein to the global lesions typical for thesedisorders.

In this study we tested whether other modes of enzyme transport occurred besides diffusion, by targeting specific anatomicalareas of the mouse brain that contain known axonal connectionsand migratory pathways. $beta$ -Glucuronidase was used as a model forlysosomal enzymes because single enzyme-positive cells can bedetected in tissue sections, allowing for localization of thetransported protein (Wolfe and Sands, 1996). We delivered GUSBto the brain with adeno-associated virus serotype 2 (AAV2) becausethis vector remains confined to the injection site and predominatelytransduces neurons (Kaplitt et al., 1994; Bartlett et al., 1998;Chamberlin et al., 1998). When the AAV2 vector was injected unilaterallyinto the hippocampus of GUSB-deficient mice, gene expression wasdetected only at the site of injection, but cells were stronglypositive for GUSB activity in both hemispheres of the hippocampusand in the septum. Only regions with axonal connections to thesite of transduction were enzyme positive. Moreover, the storagelesions in the distal structures were reversed. This indicatedthat, after the enzyme was transported along the axon, it enteredthe lysosomal compartment where it was enzymatically active andreversed the pathologic lesion. Furthermore, injection of thevector into the subventricular zone (SVZ) resulted in deliveryof GUSB to the olfactory bulb by cells migrating in the rostralmigratory stream. Both modes of transport occurred for at least18 months, which was attributable to the ability of the mammalianhousekeeping promoter in the viral vector to sustain expressionovertime.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animals. Normal C3H/HeOuJ mice were purchased from Jackson Laboratory (Bar Harbor, ME) and maintained in our breeding colony.MPS VII mice were produced by heterozygote matings of C57BL/6-ByBir-H-2^bm1gus^mps (Birkenmeier et al., 1989). Identification of affected mice,which contain a single base pair deletion in exon 10 of the GUSBgene, was verified by PCR (Sands and Birkenmeier, 1993; Wolfeand Sands, 1996). All treatments of mice were approved by andperformed according to the guidelines of the Institutional AnimalCare and UseCommittee.

AAV2 vectors. The detailed construction of the AAV2 vectors that were used in this study has been reported previously (Skorupaet al., 1999; Passini and Wolfe, 2001). AAV2 constructs containingeither the 378 bp human GUSB promoter (Shipley et al., 1991; Wolfeet al., 1995) or the human cytomegalovirus immediate-early (CMV)promoter were cloned upstream of the human GUSB cDNA (Oshima etal., 1987; Miller et al., 1990) and packaged by the Institutefor Human Gene Therapy Vector Core (see Fisher et al., 1997) intoAAV2-H $beta$ H and AAV2-CV $beta$ , respectively. Brains were injected at equaltiters of 4.5 × 10¹² genome equivalents/ml.

Stereotaxic injections into adult mice. Adult normal and mutant mice (10-12 weeks old) were injected in the intraperitonealcavity with an anesthesia dose of 100 mg/kg ketamine and 5 mg/kgxylazine. After we placed the mice in a stereotaxic frame, theirskulls were drilled, followed by the lowering of a 30-gauge Hamiltonsyringe into the appropriate brain structure. One microliter ofeither AAV2-H $beta$ H or AAV2-CV $beta$ was injected unilaterally into theappropriate structure over a 5 min period. The stereotaxic coordinatesfor each brain structure (Franklin and Paxinos, 1997) are writtenas follows: first coordinate, distance from the bregma line; secondcoordinate, distance left of the midline; third coordinate, distanceventral to the pial surface. These include the external capsuleand surrounding gray matter (0.00, 2.50, 1.75 mm), motor cortex(1.50 rostral of bregma, 1.50, 1.00 mm), somatosensory cortex(0.50 caudal of bregma, 2.50, 1.00 mm), striatum (0.00, 2.00,3.00 mm), subventricular zone (1.00 rostral of bregma, 1.25, 2.00mm), and ventral hippocampus (2.00 caudal of bregma, 1.50, 2.00mm).

Brain preparation. Mice to be killed were anesthetized deeply and perfused transcardially with 1× PBS, followed by ice-coldfixative (4% paraformaldehyde/0.1 M phosphate buffer, pH 7.4).Brains were dissected out of the skulls, drop-fixed overnightat 4°C, cryoprotected overnight in 30% sucrose/0.1 M phosphatebuffer at 4°C, transferred to plastic molds containing 100% optimalcutting temperature (OCT) solution, frozen over dry ice, and storedat $-$ 80°C. On the day before cryosectioning the frozen blocks ofbrain were placed at $-$ 20°C to equilibrate to the cutting temperature.Coronal serial sections were cut at 20 µm thickness at $-$ 20°C.Brain sections designated for enzyme histochemistry were storedat $-$ 20°C, and those designated for in situ hybridization werestored at $-$ 80°C.

In situ hybridization. The riboprobes and conditions that were used to detect the virally encoded human GUSB mRNA were describedin a recent report (Passini and Wolfe, 2001), which was basedon an in situ hybridization protocol published by Barthel andRaymond (2000).

Enzyme histochemistry. Frozen tissue sections were assayed for enzymatic activity with a naphthol-AS-BI- $beta$ -D-glucuronide substrateas reported previously (Wolfe and Sands, 1996). Endogenous GUSBprotein was heat inactivated as described to ensure that the positivecells reported in this study were from the viral vectors, becausehuman GUSB is not inactivated at 65°C (Frankel et al., 1977; Casaland Wolfe, 2001; Serguera et al., 2001).

Histology. Uninjected and injected MPS VII brains were analyzed for lysosomal storage vacuoles as reported previously (Skorupaet al., 1999). In brief, affected mice were perfused with 4% paraformaldehyde,and brains were removed and sliced into 500 µm coronal slabs witha tissue slicer (Snyder et al., 1995). Tissue slabs were embeddedin JB4 resin, sectioned at 1 µm, and stained with 5% toluidineblue (Wolfe and Sands, 1996).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Correlation of vector gene expression and enzymatic activity

For distribution studies the C3H/HeOuJ mouse strain was used because it has very low levels of GUSB activity in the brain,and the mouse GUSB protein can be heat inactivated relative tothe human protein (Johnson et al., 1986; Gallagher et al., 1987;Moullier et al., 1993; Casal and Wolfe, 2001). To show that theresults described herein were from exogenous GUSB, we injectednormal adult mice with the AAV2-H $beta$ H vector into the external capsuleand surrounding gray matter and compared them with uninjectedage-matched mice. In injected mice (Fig. 1A-C) the vector-encodedenzyme was detected in the somatosensory cortex, caudate putamen,and external capsule. A large number of transduced cells werefound in the somatosensory cortex and caudate putamen, whereasonly a low number of transduced cells were detected in the externalcapsule. The selective transduction of gray matter structurescompared with white matter tracts is consistent with AAV2 to infectneurons preferably over glial cells (Bartlett et al., 1998). Thelarger number of enzyme-positive cells relative to the in situhybridization-positive cells was attributable to local cross-correction.In uninjected mice (Fig. 1D-F) the corresponding structures werenegative for both enzyme histochemistry and in situ hybridization.The lack of detection of endogenous GUSB under the conditionsthat were used was verified for all brain structures in the followingexperiments (data not shown), demonstrating that the positivesignals reported in this study were from the transferred cDNA.

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Figure 1. Comparison of AAV2-H $beta$ H-injected (A-C) and AAV2-H $beta$ H-uninjected (D-F) brains in the C3H/HeOuJ mouse strain. Enzyme histochemistry (A, D) and in situ hybridization with the antisense riboprobe (ISH-antisense; B, E) detected many positive cells at 1 month PI, but did not detect positive cells in age-matched uninjected brains. In situ hybridization with the sense riboprobe (negative control) produced little positive signal in the injected brain (C) and no positive signal in the uninjected brain (F). CP, Caudate putamen; CTX, somatosensory cortex; EC, external capsule. Scale bar, 200 µm.

Axonal transport of GUSB in the hippocampus

To test whether GUSB can undergo axonal transport, we used AAV2 to transfer human GUSB into the ventral hippocampus, definedin this study as the cornu ammonis area 3 (CA3) and the dentategyrus, because the axons projecting into and from this regionhave well defined, predictable connections. Having a promotercapable of supporting AAV2-mediated gene expression is criticalto this investigation. However, a feature of AAV2 vectors is thatthe duration of transferred gene expression varies in differentstructures of the adult brain (McCown et al., 1996; Skorupa etal., 1999; Klein et al., 2000; Xu et al., 2001). The human GUSBpromoter may circumvent this temporal restriction because of thehousekeeping properties of this regulatory element (Kyle et al.,1990; Shipley et al., 1991).

The AAV2 vectors encoding the human GUSB cDNA, one containing the human GUSB promoter (AAV2-H $beta$ H) and the other containingthe CMV promoter (AAV2-CV $beta$ ), were each injected into groups ofadult mice in one hemisphere of the ventral hippocampus and wereanalyzed 1 and 3 months later (n = 3 for each vector at each timepoint). The resultant data were reproducible in all mice at alltimepoints.

Transduction with both vectors occurred in the CA3 pyramidal cell layer and in the granule cell layer (GCL) and hilus of thedentate gyrus at 1 month postinjection (PI) (Fig. 2A,B). Enzyme-positivecells were detected in a pattern that approximated the transductionpattern (Fig. 2D,E). Neither AAV2 vector spread to the contralateralside (Fig. 2C). However, unlike viral vector gene expression,GUSB enzymatic activity was present in the contralateral side,as demonstrated by a band of red stain in the innermost molecularlayer of the dentate gyrus, which wrapped around the circumferenceof the GCL (Fig. 2F). This enzyme pattern suggested a mode oftransport alternative to diffusion, because a gradient of enzyme-positivecells that extended throughout the contralateral hemisphere wouldhave been expected to be present if this were the case.

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Figure 2. Comparison between AAV2-CV $beta$ and AAV2-H $beta$ H in the hippocampus at 1 month PI (A-F) and 3 months PI (G-M). Shown are ISH-antisense (A-C, G-I) and enzyme histochemistry (D-F, J-M). The number of mRNA- and enzyme-positive cells decreased between 1 month PI (A, D) and 3 months PI (G, J) with AAV2-CV $beta$ . In contrast, the number of cells expressing GUSB mRNA did not change between 1 month (B) and 3 months (H) with AAV2-H $beta$ H. In addition, a substantial increase in the number of enzyme-positive cells was detected at 3 months (K) compared with 1 month (E) with AAV2-H $beta$ H. Enzyme-positive cells were clearly present in regions of the ipsilateral hippocampus that were negative for gene expression (K). There was a conspicuous absence of enzyme staining in the CA1-CA3 lacunosum moleculare layers at 3 months (asterisk in K). The number of enzyme-positive cells in the contralateral hemisphere was also greater at 3 months (L) compared with 1 month (F) with AAV2-H $beta$ H. At 1 month the enzyme-positive cells were restricted to the inner molecular layer of the dentate gyrus (F, arrow). This was verified by the staining of an enzyme-positive section with 0.1% cresyl violet, which labeled the dentate granule cell layer, but not the dentate molecular layer (small box, F). At 3 months the pattern of enzyme-positive cells extended to include other regions in the contralateral hippocampus, particularly the oriens and radiatum layers of CA1-CA3 (L). A high-magnification image of a cresyl violet-stained section demonstrated that enzymatic activity was maintained in the inner molecular layer of the dentate gyrus (small box, L). Transduced cells were not detected in the uninjected hemisphere at either time point with AAV2-H $beta$ H-injected brains (C, I). An entire brain section at 3 months PI demonstrated how well enzymatic activity was confined to the hippocampus, although a small number of positive cells could be seen in the overlying cortex (M). CA1p, CA1 pyramidal cell layer; CA3p, CA3 pyramidal cell layer; G, upper and lower blades of the dentate granule cell layer; H, hilus; L, stratum lacunosum moleculare; Mi, inner molecular layer of the dentate gyrus; Mo, outer molecular layer of the dentate gyrus; O, stratum oriens; R, stratum radiatum. Scale bars: A-L, 500 µm; M, 1000 µm.

By 3 months PI a difference in the expression pattern was apparent. Only a low number of transduced cells were still detectablefrom the AAV2-CV $beta$ vector (Fig. 2G), and the number of enzyme-positivecells was less than that at 1 month (Fig. 2D,J). In contrast,with the AAV2-H $beta$ H vector similar numbers of in situ hybridization-positivecells were present at 1 and 3 months (Fig. 2B,H). Although transducedcells were restricted to the ventral hippocampus, abundant enzyme-positivecells were found in the oriens, pyramidal, and radiatum layersof all three CA fields (CA1-CA3) and in the GCL, hilus, and molecularlayers of the dentate gyrus at 3 months (Fig. 2K,M). AAV2-H $beta$ Hvector gene expression was not detected in the contralateral hippocampusat 3 months (Fig. 2I). Nevertheless, a substantial increase inthe number of enzyme-positive cells was seen throughout the contralateralhippocampus (Fig. 2L,M).

For axonal transport of GUSB to the contralateral hemisphere to occur, it is predicted that enzyme would be present in thehippocampal commissure, a structure that is composed of hippocampalaxons projecting from opposite hemispheres. This was shown tobe true at 3 months PI, in which the hippocampal commissure waspositive for GUSB enzyme but negative for GUSB mRNA (Fig. 3A-C).The majority of enzyme activity stain produced a linear patternthat was localized precisely to the bundle of axons that connectthe hippocampal formations from the two sides of the brain. Anothernearby white matter tract, the overlying corpus callosum, whichdoes not contribute to the intrahippocampal circuitry, did notshow this pattern of staining. There was additional staining detectedin a small number of cell bodies in the region, which may be glialcells. Although it is unknown how these cell bodies acquired enzyme,cell-to-cell contact has been shown to transport GUSB betweencells (Olsen et al., 1981). Thus contact between neuronal axonsand glial cells may be an explanation.

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Figure 3. Long-term enzymatic activity and expression in the hippocampal commissure and hippocampus. Shown are enzyme histochemistry (A, B, G-I) and ISH-antisense (C-F) in the hippocampal commissure (A-C, I), ipsilateral hippocampus (D-G), and contralateral hippocampus (H). Unilateral injections of AAV2-H $beta$ H into the ventral hippocampus resulted in undetectable levels of enzyme staining at 1 month PI (A) but detectable levels at 3 months PI (B) in the hippocampal commissure. Although a small number of cell bodies were labeled, the majority of staining was present in a diffuse, linear pattern (B). Vector-encoded human GUSB mRNA was not present in a corresponding section at 3 months (C). Robust transduction was observed in the ventral hippocampus in all three mice at 18 months PI (D-F). In mouse 1 the GUSB-expressing cells were abundant in the CA3 pyramidal cell layer and in the ventral blade of the dentate GCL (D). In mouse 2 transduced cells were present in the pyramidal layer of CA2 and CA3 (E). In mouse 3 a large number of GUSB-expressing cells were detected in the CA3 pyramidal cell layer and in the GCL and hilus of the dentate gyrus (F). As represented by mouse 1, widespread enzyme-positive cells were detected in the injected (G) and uninjected (H) hemispheres of all three mice. The most robust enzyme staining in the uninjected hemisphere was detected in CA1-CA3 (H). Other regions, such as the inner molecular layer of the dentate gyrus, were also positive for enzymatic activity (H). A larger area of diffuse enzyme staining was observed in the hippocampal commissure at 18 months (I) compared with 1 month (A) and 3 months (B). Scale bars: A-D, G, H, 500 µm; E, F, I, 250 µm.

The ability of the human GUSB promoter to support long-term expression was demonstrated in the ventral hippocampus at 18 monthsPI (Fig. 3D-F). The maintenance of expression resulted in veryhigh levels of enzymatic activity, as illustrated by the blackenedstaining pattern at the injection site, which can occur in thepresence of supraphysiologic levels of GUSB activity (Fig. 3G).The spread of GUSB to the contralateral hemisphere increased at18 months, which was particularly evident in cells of the oriensand radiatum layers of CA1-CA3 (Fig. 3H). The increased areasof enzyme-positive staining in the contralateral hemisphere correlatedwith increased GUSB staining in the hippocampal commissure at18 months (Fig. 3I). Consistent with earlier time points, vector-encodedmRNA was not observed in the contralateral hemisphere or hippocampalcommissure at 18 months (data notshown).

Reversal of pathology by axonal transport

The extensive amount of lysosomal storage in the MPS VII hippocampus (Levy et al., 1996; Casal and Wolfe, 1998) is ideal fordetermining the therapeutic efficacy of axonal transport. Correctionof storage was tested with AAV2-H $beta$ H, because the human GUSB promoterwas clearly superior to CMV. Three months was chosen to take fulladvantage of the robust enzymatic activity that accumulated inthe both hemispheres. After unilateral injection of the MPS VIIventral hippocampus, storage was reversed in neurons and glialcells in both hemispheres of the CA3 field and the dentate gyrus(Fig. 4).

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Figure 4. Reversal of pathology in the MPS VII brains after unilateral injection of AAV2-H $beta$ H into the ventral hippocampus at 3 months PI. Shown are toluidine blue-stained plastic sections in uninjected (A, D) and injected (B, C, E, F) mice. Lysosomal storage vacuoles were visible in the uninjected GCL and hilus of the dentate gyrus (A) but were cleared in the ipsilateral (B) and contralateral (C) hemispheres of injected brains. Lysosomal storage vacuoles, which were present in the entire CA3 pyramidal cell layer in uninjected mice (D), were reversed in both the ipsilateral (E) and contralateral (F) hemispheres of injected brains. Arrows point to lysosomal storage vacuoles. Scale bar, 50 µm.

Axonal transport would be beneficial in treating the global lesions of storage if lysosomal enzymes could become distributedvia inter-regional systems. The potential for inter-regional axonaltransport was seen in the nigrostriatal system. Injection of AAV2-H $beta$ Hinto the striatum resulted in a high number of transduced cellsand a large area of enzyme-positive cells in this structure (Fig.5A,B). Enzyme-positive cells were detected in the substantia nigrafrom the striatal injections, but none of these cells was positivefor gene expression (Fig. 5C,D). This pattern is consistent withGUSB distribution by retrograde transport in neurons of the substantianigra, which send extensive inputs into the striatum (Kordoweret al., 2000; Peltekian et al., 2002).

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Figure 5. Axonal transport in the nigrostriatal (A-D) and septohippocampal (E-H) systems after AAV2-H $beta$ H vector injection. Shown are enzyme histochemistry (A, C, E-G) and ISH-antisense (B, D, H). Injections into the striatum resulted in many enzyme- and mRNA-positive cells in this structure at 18 months PI (A, B). Enzyme-positive cells were present in the substantia nigra after the striatal injections (C). However, the entire substantia nigra was negative for gene expression (D). After injection of the ventral hippocampus, enzyme-positive cells were undetectable in the septum at 1 month (E) but were detectable at 3 months (F) and 18 months (G). Enzyme-positive cells in the septum were observed in the medial nucleus and in both dorsolateral nuclei, but not in either ventrolateral nucleus (F, G). ISH-antisense did not produce positive cells in the septum at 18 months (H). Scale bars: A-D, 250 µm; E-H, 500 µm.

We took advantage of the well defined connections between the ventral hippocampus and the septum to investigate GUSB movementand reversal of pathology within the septohippocampal system.Unilateral injection of the ventral hippocampus with AAV2-H $beta$ Hresulted in numerous enzyme-positive cells in discrete regionsof the septum at 3 and 18 months PI (Fig. 5F,G). Positive cellswere restricted to the medial septal nucleus and to both dorsalseptal nuclei. The lack of detectable enzyme-positive cells at1 month in the septum (Fig. 5E), followed by detectable levelsat 3 and 18 months, is consistent with the temporal pattern ofGUSB in the contralateral hippocampus and hippocampal commissure.Transduced cells expressing mRNA were not detected in the septumat any time point (Fig. 5H).

Unilateral injections of AAV2-H $beta$ H into the MPS VII ventral hippocampus resulted in the reversal of pathology in the neuronaland glial cell populations of the medial and both lateral septalnuclei at 3 months (Fig. 6A-D). However, storage vacuoles werepresent in structures that were in relatively close proximityto the hippocampus and septum, such as the neocortex, piriformcortex, caudate putamen, and thalamus (Fig. 6E-H). This suggeststhat axonal transport was responsible for the clearance of storagein the contralateral hippocampus and septum, because nearby structuresalso would have been corrected if diffusion had occurred.

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Figure 6. Correction of storage in the septum after hippocampal injections. Shown are toluidine blue-stained plastic sections of the septum (A-D) and other brain structures (E-H). Storage vacuoles were present in many cells of the uninjected MPS VII medial (A) and lateral (C) septa. Reversal of pathology was observed in neurons and glial cells of the medial (B) and lateral (D) septum 3 months after AAV2-H $beta$ H vector injection of the MPS VII ventral hippocampus. These injections did not correct storage lesions in other brain structures, as illustrated by the neocortex (E), piriform cortex (F), caudate putamen (G), and thalamus (H). Arrows point to lysosomal storage vacuoles. Scale bar, 40 µm.

GUSB transport by migratory cells

We also determined that another mode of GUSB transport exists in the adult brain. Injection of the viral vector into the SVZresulted in GUSB delivery to the olfactory bulb by migrating cells.Stem cells occupying the anterior SVZ undergo tangential migrationto the olfactory bulb via the rostral migratory stream, a developmentalprocess that continues in the adult (Altman, 1969). On reachingthe subependymal zone of the olfactory bulb, these cells undergoradial migration to specific laminar layers occupied by granuleand periglomerular cells (Luskin, 1993; Lois and Alvarez-Buylla,1994; Uchida et al., 2000).

Unilateral injection of AAV2-H $beta$ H into the vicinity of the SVZ resulted in transduction at 1 month PI (Fig. 7A,D). A coronalsection through the rostral migratory stream, approximately midwaybetween the SVZ and olfactory bulb, showed a high-density chainof enzyme-positive cells that were negative for GUSB mRNA (Fig.7B,E). A very high number of enzyme-positive cells were observedin the subependymal zone and granule cell layer of the ipsilateralolfactory bulb (Fig. 7C). However, none of these cells was positiveby in situ hybridization (Fig. 7F). It is unlikely that the lackof expression in the olfactory bulb was attributable to promotershutdown, because the human GUSB promoter supports transcriptionin all layers of this structure (Passini and Wolfe, 2001).

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Figure 7. Transport of GUSB in the rostral migratory stream. Shown are enzyme histochemistry (A-C, G-I) and ISH-antisense (D-F, J-L) in coronal sections of the subventricular zone (A, D, G, J), the rostral migratory stream (B, E), and the main olfactory bulb (C, F, H, I, K, L) at 1 month PI (A-F) and 18 months PI (G-L). Scale bars: A, D, 500 µm; C, F, 400 µm; G, H, J, K, 250 µm; B, E, I, L, 60 µm.

Enzymatic activity and gene expression were still present in the SVZ at 18 months (Fig. 7G,J), which resulted in a populationof enzyme-positive cells in the granule cell layer of the olfactorybulb (Fig. 7H,I). As with axonal transport, this mode of transportis maintained over time, albeit with less accumulation of enzymaticactivity at the distal site. Virally encoded mRNA cells were notdetected in the olfactory bulb at 18 months (Fig. 7K,L).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

This study determined the different modes of GUSB transport in the brain with an AAV2 vector regulated by a mammalian housekeepingsequence. The ability of the human GUSB promoter to support geneexpression over time is beneficial to experiments that must relyon a continuing source of protein product. The maintenance ofGUSB expression in the brain resulted in saturation of enzymeat the injection site and accumulation in distal locations. Incontrast, the CMV promoter did not sustain expression over time,consistent with other AAV2 experiments that used viral promoters(Alexander et al., 1996; McCown et al., 1996; Davidson et al.,2000). Although mammalian regulatory sequences such as the neuronal-specificenolase and platelet-derived growth factor promoters support expressionin the CNS (Peel et al., 1997; Klein et al., 1998; Xu et al.,2001), the relatively large size of these promoters is a disadvantagewhen engineering AAV2 recombinant genomes because of size limitationsin the packaging reactions (Dong et al., 1996). The minimallysized 378 bp human GUSB promoter thus would provide a distinctadvantage in somatic gene transfer experiments involving largecDNAs.

A new finding was the transduction of the adult GCL with both AAV2-H $beta$ H and AAV2-CV $beta$ , which had not been seen in previous studiesthat used AAV2 vectors with either the neuronal-specific enolaseor CMV promoters (McCown et al., 1996; Bartlett et al., 1998;Klein et al., 1998; Xu et al., 2001). Interestingly, wild-typeAAV2 does not have a natural tropism for the GCL (Bartlett etal., 1998). Our data suggest that the transgene itself may influencethe transduction profile of a given AAV2 vector in the brain.This recently was shown to occur with an adenovirus vector, inwhich different transduction patterns were observed in the brainwhen different transgenes were used in an identical viral vectorbackbone (Zermansky et al., 2001). This implies that variegatedpatterns of transduction will arise in the CNS from unique combinationsof promoters andcDNAs.

Our data show that GUSB distribution and reversal of pathology in the contralateral hippocampus are attributable to axonaltransport. This is supported by several lines of evidence (Fig.8). First, the abundant enzyme-positive cells in the contralateraloriens and radiatum layers are explained by the extensive inputsfrom the commissural axons emanating from CA3 pyramidal neurons(Swanson et al., 1978; Amaral and Witter, 1989). Also, the widespreadenzyme pattern in the ipsilateral CA1 field may have occurredvia Schaffer collaterals. Second, the presence of enzyme stainingin the inner molecular layer of the dentate gyrus is consistentwith axonal transport by hilar neurons, because these cells sendaxons to opposite hemispheres and innervate a laminar positiondirectly adjacent to the GCL (Gottlieb and Cowan, 1973; Swansonand Cowan, 1977). Because the outer molecular layer does not receiveinput from the dentate gyrus, but rather from the perforant pathwaysof the entorhinal cortex (Blackstad, 1958; Raisman et al., 1965;Bayer, 1985), it would be predicted that the outer molecular layerwould not be positive for GUSB, which is what we have observed(Fig. 2F). In agreement, the lacunosum moleculare layers of CA1-CA3,which were negative for GUSB, also receive input primarily fromperforant axons (Hjorth-Simonsen, 1973; Steward, 1976). Finally,the detection of GUSB in the hippocampal commissure is consistentwith the presence of enzyme in the axons.

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Figure 8. Diagram showing the symmetrical circuitry of the intrahippocampal system. CA1 and CA3 pyramidal cells have dendrites that extend into the oriens, radiatum, and lacunosum layers (A). CA3 pyramidal cells send commissural collaterals to the contralateral CA1-CA3 radiatum and oriens layers and send Schaffer collaterals to the ipsilateral CA1 radiatum layer (A). Dentate granule cells have dendrites that extend into the inner and outer molecular layers (B). Hilar neurons of the dentate gyrus send ipsilateral and commissural collaterals to the inner one-third molecular layer and synapse with dentate granule cells (B). According to these connections the GUSB transport to the contralateral side probably occurred by secretion of GUSB into the ipsilateral synapse by the transduced cell (labeled as X), followed by uptake by the axonal termini (or terminus) of the contralateral cell and subsequent retrograde transport via the commissural axon to the soma. Although anterograde projections occur, it is not thought that lysosomes move to the synaptic terminus (Walkley, 1998). CC, Commissural collateral; IC, ipsilateral collateral; P, pyramidal cell layer; SC, Schaffer collateral; see Figure 2 for additional abbreviations.

The enzyme pattern in the septum after hippocampal injections further demonstrates that axonal transport occurred rather thandiffusion. GUSB was restricted to the dorsal nucleus of both lateralsepta, with no enzyme-positive cells being detected in the ventralnuclei. This pattern is predicted by the topographical organizationbetween the two structures. The rostral-ventral hippocampus (theinjected site) innervates the dorsal lateral septum and the caudal-ventralhippocampus innervates the ventral lateral septum (Swanson etal., 1981). If diffusion of GUSB to the septum had occurred, thenenzyme-positive cells would have been present in the entire lateralseptum, rather than just the dorsal region. Furthermore, structuresnear the septum and the hippocampus also would have been exposedto any secreted enzyme, but many of these nearby structures werenegative for enzyme staining and contained large numbers of cellswith storagelesions.

We could not determine unambiguously in which direction GUSB was moving through the circuits of the intrahippocampal and septohippocampalsystems. Although neurons in these systems connect in both theretrograde and anterograde directions (Figs. 8, 9), retrogradetransport is the most likely explanation for enzyme movement throughaxons, because endosome trafficking occurs from the synaptic terminito the perikarya in neurons (Nixon and Cataldo, 1995; Overly andHollenbeck, 1996; Walkley, 1998; Mathews et al., 2002). The correctionof storage lesions in neurons distal from the injection site indicatesthat endosomes carrying GUSB fused with lysosomes after retrogradetrafficking in vivo, because the enzyme must reach the acidifiedlysosome to be active catalytically.

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Figure 9. GUSB movement throughout the circuit of the septohippocampal system. Only one hemisphere of the ventral hippocampus is shown. Neurons from the medial septum project onto CA3 pyramidal and dentate hilar cells, whereas CA3 pyramidal cells project onto the lateral septal nuclei of both hemispheres (Swanson, 1977). Retrograde transport in axons of the medial septum is the likely mechanism for GUSB movement in this circuit. Because neurons of the lateral septum also project onto the medial septum, the enzyme pattern and reversal of pathology in the lateral septum probably occur by retrograde transport via a second axon (second-order neuron). CA3p, CA3 pyramidal cell layer; H, hilus; LS, lateral septum; MS, medial septum.

Glial cells surrounding the enzyme-positive distal neurons also were corrected. This indicates that, after the completionof axonal transport, some of the active enzyme was released intothe surrounding area and taken up by adjacent cells. This evidenceof enzyme in the extracellular space suggests that axon endingsin this area also were exposed to secreted enzyme, which wouldaccount for the presence of staining in some second-order neurons.This is illustrated by the retrograde transport of GUSB via twoconnecting neurons in the septohippocampal system (Fig. 9). Althoughthis ability to become transported along multiple neurons canincrease the distribution of GUSB in the brain, it was found onlyin someareas.

Unilateral injections of a lentivirus vector into the fimbria of another mouse model of lysosomal enzyme deficiency (metachromaticleukodystrophy) resulted in reversal of storage lesions in thecontralateral CA3 pyramidal cell layer and fimbria (Consiglioet al., 2001). However, because there is no available assay tostudy the arylsulfatase A enzyme pattern in situ, it could onlybe conjectured that axonal transport was responsible for enzymemovement throughout the hippocampus. Those data together withthe present study suggest that axonal transport may be a generalproperty of lysosomalenzymes.

GUSB also was transferred long distances by migrating cells. Injection of AAV2-H $beta$ H into the vicinity of the SVZ resulted inenzyme-positive cells in the olfactory bulb. However, there wasno gene expression detected by in situ hybridization in the rostralmigratory stream or olfactory bulb, indicating that the vectordid not transduce the stem cell population leaving the SVZ. Rather,transduced cells in the vicinity of the SVZ secreted GUSB, whichthen was taken up by cells entering the rostral migratory stream.The GUSB half-life of 3-6 d (Achord et al., 1977; Vogler et al.,1993) allows a significant amount of enzyme to survive the journeyto the olfactory bulb, because the time it takes for SVZ cellsto travel down the rostral migratory is also 3-6 d (Luskin, 1993).The lack of stem cell infection with AAV2 differs from SVZ injectionswith retrovirus and adenovirus, which resulted in stem cell transductionand subsequent delivery of the $beta$ -galactosidase reporter gene tothe granule and periglomerular cell layers (Luskin, 1993; Yoonet al., 1996).

In contrast to the SVZ, the maintenance of gene expression for at least 18 months in the GCL suggests that AAV2-H $beta$ H infectedstem cells of the dentate gyrus, which continuously supply newgranule cells to replace dying ones (Kaplan and Hinds, 1977; Bayer,1982; Gage, 2000). This differed from our recent finding withAAV2-H $beta$ H injections in the developing brain (Passini and Wolfe,2001), which resulted in a continual decrease in the number ofin situ hybridization-positive cells over time in the GCL, indicatingthat stem cells of the dentate gyrus were not infected at birth.The combined data from both studies suggest that AAV2 vectorsare permissive for the infection of some pools of stem cells,but not of others, and that transduction of a given stem cellpopulation can differ between a developing and maturebrain.

In conclusion, we determined that there are alternate ways in which lysosomal enzymes can become distributed throughout thebrain. The transport occurred for at least 18 months, demonstratingthat strategically placed enzyme-secreting foci can provide along-term supply of enzyme to locations far away from the injectionsite by diffusion, axonal transport, and migrating cross-correctedcells. The use of all three modes of transport in treatment strategiesshould be beneficial in reversing the global neuropathology oflysosomal storage diseases in future clinicaltrials.

  FOOTNOTES

Received Feb. 1, 2002; revised April 5, 2002; accepted May 2, 2002.

This study was supported by National Institutes of Health Grants NS38690 and DK42707 (J.H.W.) and by Institute for Human GeneTherapy Vector Core Center Grant DK47747. National Research ServiceAward training grants supported M.A.P. and G.G.H. (DK07748) andE.B.L. (AG00255); G.G.H. also was supported by a fellowship fromthe National Institute of Mental Health (MH12285). We thank A.Polesky, M. Parente, S. Gallagher, E. Cabacungan, C. Jones, A.Crystal, G. Gao, and G. Qu for theirassistance.

Correspondence should be addressed to Dr. John H. Wolfe, 502G Abramson Research Center, Children's Hospital of Philadelphia,3516 Civic Center Boulevard, Philadelphia, PA 19104. E-mail: jhwolfe{at}vet.upenn.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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