Abstract
Tuberous sclerosis (TSC) is a hamartoma syndrome caused by mutations in TSC1 or TSC2 in which cerebral cortical tubers and seizures are major clinical issues. We have engineered mice in which most cortical neurons lose Tsc1 expression during embryonic development. These Tsc1 mutant mice display several neurological abnormalities beginning at postnatal day 5 with subsequent failure to thrive and median survival of 35 d. The mice also display clinical and electrographic seizures both spontaneously and with physical stimulation, and some seizures end in a fatal tonic phase. Many cortical and hippocampal neurons are enlarged and/or dysplastic in the Tsc1 mutant mice, strongly express phospho-S6, and are ectopic in multiple sites in the cortex and hippocampus. There is a striking delay in myelination in the mutant mice, which appears to be caused by an inductive neuronal defect. This new TSC brain model replicates several features of human TSC brain lesions and implicates an important function of Tsc1/Tsc2 in neuronal development.
Introduction
Tuberous sclerosis (TSC) is an autosomal dominant hamartoma syndrome in which involvement of the brain causes prominent neurologic symptoms (Gomez et al., 1999; Curatolo, 2003; Crino, 2004; DiMario, 2004). Cortical tubers, the hallmark TSC lesion in the brain, occur in nearly all TSC patients and are associated with a variety of forms of epilepsy, including infantile spasms (Thiele, 2004). Developmental delay and abnormal behavioral phenotypes, including autism, are also commonly seen in TSC (de Vries et al., 2005; Wiznitzer, 2004). Pathologically, cortical tubers are characterized by a regional loss of normal cortical architecture, with prominent giant cells that have enlarged nuclei and soma and are often multinucleated (Scheithauer and Reagan, 1999; Crino, 2004). Large numbers of disordered and dysplastic neurons are also seen within cortical tubers, as well as increased numbers of astrocytes (Crino, 2004; Miyata et al., 2004). A second TSC brain lesion is the subependymal nodule, which is found lining the ventricular wall, typically in the lateral ventricles, and can progress to a subependymal giant cell tumor.
TSC is caused by inactivating mutations in either of TSC1 or TSC2 (Kwiatkowski and Manning, 2005). Mutations can be identified in one or the other of these two genes in ∼85% of TSC patients; the remainder are likely attributable to mosaicism or undetected mutations, as there is no evidence for a third gene (Kwiatkowski, 2003). The protein products of these genes, hamartin and tuberin, respectively, have been shown to play an important role in a conserved signaling pathway that regulates both cell size and cell growth (Astrinidis and Henske, 2005; Inoki et al., 2005; Kwiatkowski and Manning, 2005; Sarbassov et al., 2005; Tee and Blenis, 2005). Hamartin and tuberin form a complex, and a GTPase-activating protein (GAP) domain within tuberin functions to accelerate conversion of Rheb-GTP to Rheb-GDP. Rheb-GTP activates the mTORC1 kinase complex, which leads to both cell size enlargement and protein translation by phosphorylating several downstream effectors, including p70S6 kinase and 4E-BP1 (Holz et al., 2005). Biallelic inactivation of either TSC1 or TSC2 is seen in most hamartomas from TSC patients, corresponding to the germline mutation (Cheadle et al., 2000; Tucker and Friedman, 2002; Chan et al., 2004). Thus, in TSC lesions, there is loss of the hamartin–tuberin GAP activity with consequent constitutive activation of mTORC1 and its downstream effectors. One mTORC1 effector, p70S6 kinase, phosphorylates the ribosomal protein S6, and phospho-S6 (pS6) is present at high levels in TSC hamartomas (Goncharova et al., 2002; El-Hashemite et al., 2003). In contrast to hamartomas, the evidence for biallelic inactivation of TSC1 or TSC2 in cortical tubers has been very limited (Niida et al., 2001; Tucker and Friedman, 2002), and there is a suggestion of an alternative pathogenesis (Han et al., 2004). However, tuber giant cells express pS6 and other markers of mTORC1 activation at high levels, similar to subependymal giant cell astrocytomas (Baybis et al., 2004; Chan et al., 2004; Miyata et al., 2004).
We and others have generated and evaluated several rodent models of TSC. The Eker rat arose as a spontaneous inactivating mutation in Tsc2 and has been shown to develop approximately one brain hamartoma per rat (Yeung et al., 1997; Wenzel et al., 2004). These lesions have some resemblance to the brain lesions occurring in TSC, but there is no associated clinical phenotype. Tsc1w− and Tsc2w− mice have been generated but develop no significant brain pathology (Onda et al., 2002). More recently, we have generated a conditional, floxed allele of Tsc1 (Tsc1c ) (Kwiatkowski et al., 2002; Meikle et al., 2005). Using this allele, mice lacking Tsc1 expression in astrocytes have been generated, and although these mice develop seizures and significant brain pathology, this model does not produce pathology similar to that seen in TSC cortical tubers (Uhlmann et al., 2002).
Here, we report the generation and characterization of a new brain model of TSC, using the Tsc1c allele. Tsc1 expression is ablated in most neurons beginning at approximately embryonic day 13 (E13) through use of a synapsin promoter to drive cre recombinase expression (Zhu et al., 2001). These mice display delayed development beginning at postnatal day 5 (P5), spontaneous seizures, shortened lifespan, and neuropathological abnormalities including ectopic, enlarged, and aberrant neurons in multiple locations. These abnormal neurons have features similar to the dysplastic neurons seen in TSC cortical tubers. Persistent hypomyelination is also seen in these mice, although axon and oligodendrocyte distribution appear normal.
Materials and Methods
Mouse procedures.
Mouse experiments were performed in a mixed-strain background (129S4/SvJae, C57BL/6, and CBA) to accommodate the combination of alleles studied here. Mice bearing the SynI-cre allele were a generous gift from Jamey Marth (University of California, San Diego, La Jolla, CA) (Zhu et al., 2001). Mice were generated through breedings between Tsc1cc females and either Tsc1w−SynI-cre + or Tsc1w−SynI-cre ++ males or between Tsc1cc males and Tsc1cwSynI-cre + females. (We use c, w, and − to denote the conditional (floxed), wild-type, and null alleles of Tsc1, respectively; the formal name of the c allele is Tsc1tm1Djk .) All Tsc1cc mice used were also homozygous for a floxed β-galactosidase (β-gal) reporter allele from which β-gal expression occurs only after cre recombination (Mao et al., 1999). Generation of the Tsc1c and Tsc1− alleles was described previously (Kwiatkowski et al., 2002; Meikle et al., 2005). In the Tsc1c allele, there are loxP sequences flanking exons 17 and 18. When recombination occurs, deletion of these two exons leads to no Tsc1 protein expression, a null allele (Kwiatkowski et al., 2002). All procedures were performed in accordance with the Guide for the Humane Use and Care of Laboratory Animals, and the study was approved by the Harvard Medical Area Standing Committee on Animals and the Animal Care and Use Committee of Children's Hospital, Boston. Mice were killed when weight loss of 20%, greatly reduced movement, or other signs of morbidity were seen.
DNA analyses.
DNA was prepared from mouse toes/tails by standard procedures for genotyping. Genotyping at the Tsc1 gene was performed using a three-primer system that allows simultaneous analysis of both conditional and wild-type alleles, followed by agarose gel electrophoresis (Meikle et al., 2005). Primers that amplify a 300 bp portion of the cre recombinase were used to assess the presence of the SynI-cre allele (Meikle et al., 2005). Southern blot analysis was performed on brain DNA following standard methods (Kwiatkowski et al., 2002).
Antibodies.
Antibodies used were as follows: S6K, Tsc2 (C20), Akt, and ERK2 (extracellular signal-regulated kinase 2) (Santa Cruz Biotechnology, Santa Cruz, CA); pS6 (S240/244), pS6 (S235/236), and Tsc1 (Cell Signaling Technology, Bedford, MA); NeuN (MAB377), glutamate decarboxylase 67 (GAD67; MAB351), galactocerebroside (GalC; MAB342), neurofilament (NF; MAB4245), myelin basic protein (MBP; AB980), growth-associated protein 43 (GAP-43; MAB347), nestin (MAB353), and neuron-specific enolase (NSE; AB951) (Millipore, Billerica, MA); GFAP (SMI 22), nonphosphorylated neurofilament (SMI 311), phosphorylated neurofilament (SMI 312), and MBP (SMI 99) (Sternberger Monoclonals, Lutherville, MD); O4 (gift from S. Pfeiffer, Farmington, CT); and Tsc1 (gift from V. Ramesh, Boston, MA).
Immunoblotting.
Mice were killed at P21, and the whole brains were rapidly removed. Half-brains were isolated, snap frozen in liquid nitrogen, and stored at −80°C. Each frozen half-brain was homogenized in 5× volume TBSV lysis buffer [(in mm) 20 Tris-Cl, pH 7.5, 140 NaCl, 10 NaF, 1 Na3VO4, and 1 EDTA] with 0.1% Triton X-100, and one “Complete Mini” protease inhibitor mixture tablet (Roche, Indianapolis, IN) per 50 ml. Samples were then diluted in Laemmli's SDS-sample buffer. Proteins were separated by electrophoresis on 4–12% Bis-Tris gels (Novex; Invitrogen, Carlsbad, CA) and transferred onto trans-blot nitrocellulose membranes. Coomassie staining was performed to confirm that the samples were loaded equally. The membranes were blocked in 5% nonfat dry milk in PBS, pH 7.4, with 0.1% Tween 20 (PBS-Tween) for 1 h at room temperature. Primary antibodies were diluted in the blocking solution, and the membranes were incubated overnight at 4°C. The primary antibody was removed, and the blots were washed in PBS-Tween and then incubated for 1 h at room temperature in horseradish peroxidase-conjugated secondary antibodies (Santa Cruz Biotechnology). Reactive proteins were visualized using SuperSignal West Pico chemiluminescence reagent (Pierce Biotechnology, Rockford, IL) and exposure to x-ray film (BioMax MR; Kodak, Rochester, NY). All immunoblots shown in one row of a figure are from the same gel-blot exposure.
Histological preparation and immunohistological staining of brain sections.
Mice at ages P14 and P21 were anesthetized, and transcardiac perfusion was performed using PBS, followed by 4% paraformaldehyde (PFA) in PBS. Whole brains were then removed and postfixed overnight at 4°C in 4% PFA solution. P7 mice were anesthetized and decapitated, and whole brains were removed and fixed overnight at 4°C in the same 4% PFA solution. Paraffin sections were prepared for standard histological examination. For immunostaining, fixed brains were cryoprotected in 30% sucrose in PBS for 1–14 d at 4°C, and coronal sections were cut at 50 μm using a Microm K400 Fast Freezing Unit and HM 450 Sliding Electronic Microtome and were then stored in PBS at 4°C until use (Talos et al., 2006). Free-floating sections were incubated in blocking solution (PBS with 0.1% Triton X-100 and 5% normal goat serum; except for GalC and O4, for which Triton X-100 was omitted) for 1 h at room temperature, followed by incubation with primary antibody overnight at 4°C. After three 20 min PBS washes, sections were incubated in secondary antibody solution containing Alexa Fluor 568 goat anti-rabbit/anti-mouse IgG/IgM or Oregon green 488 goat anti-rabbit/anti-mouse IgG (Invitrogen), for 1 h at room temperature. After three washes in PBS, sections were mounted onto positively charged slides and coverslipped with antifade medium (Fluoromount-G; Southern Biotechnology, Birmingham, AL). Control sections were done with omission of one or both primary antibodies, adding both secondary antibodies, to establish specificity. Fluoro Jade B (AB310; Millipore) staining was performed on 50 μm free-floating sections following standard histological procedures (Schmued et al., 2005). Slides were viewed on a Nikon (Tokyo, Japan) TE2000-E inverted microscope equipped with 20×, 10×, and 4× objectives. Illumination wavelength, intensity, and exposure times were selected using a dual filterwheel apparatus containing an electronically controlled shutter and filters for the different fluorophore wavelengths (Lambda 10-2; Sutter Instruments, Novato, CA). Digital images were captured using an Orca-II ER cooled CCD camera (Hamamatsu Photonics, Hamamatsu, Japan) and MetaMorph. Digital images were then processed and analyzed using Adobe (San Jose, CA) Photoshop, including pseudocolorization.
5-Bromo-4-chloro-3-indolyl-β-d-galactopyranoside (X-gal) staining of brain sections to assess β-gal expression was performed using a kit (Millipore) following the manufacturer's instructions. Immunoperoxidase staining on these same sections was performed after X-gal staining, using a three-step avidin–biotin–peroxidase system. After exposure to primary antibodies, sections were incubated in biotinylated secondary antibodies, followed by ABC reagent (Vectastain; Vector Laboratories, Orton Southgate, Peterborough, UK). Diaminobenzidine was used as substrate to detect bound peroxidase, and the reaction was stopped when a brown color appeared; incubation of all sections was terminated simultaneously. Slides were viewed on a Nikon Eclipse E400 microscope, and images were captured using Spot software v4.0.5.
For all histological and immunostaining observations, a minimum of three (range, 3–12) pairs of mutant and control mice were examined from stereotactically matched brain sections.
Confocal images were captured using a Zeiss (Thornwood, NY) LSM 510 scanning laser microscope with 20× and 63× objectives. For cell size determination, a Z-stack of confocal images at 0.5 μm intervals was collected from the somatosensory cortex in layer V (−2 to −2.2 mm from bregma and 3.2–3.4 mm lateral to midline) for each of two matched mutant and control mice. Images were examined using ImageJ software 1.31v (W. Rasband, National Institutes of Health, Bethesda, MD) to calculate cell size in pixels after manual drawing of cell margins. All SMI 311+ cells in a 20× field were measured, independent of pS6 staining, for a minimum of eight cells per mouse. Measurements were compared using the Mann–Whitney U test in Prism (GraphPad, San Diego, CA).
Mouse electroencephalogram methods.
Mouse electroencephalogram (EEG) recordings were acquired with Teflon-coated silver/silver chloride (Ag/AgCl) subdermal wire electrodes (SWEs) (Ives, 2005). Three electrodes were positioned in the dorsal scalp: one wire at midline over the olfactory bulb and two wires over the left and right parietal regions. A fourth SWE was placed subcutaneously over the thorax to record the electrocardiogram (EKG). The electrodes were placed using 26 ga syringe needles as guides, but only the thin flexible electrode strands were left in the scalp and torso. Splayed wires at the terminus of the electrode kept wires in position during recording. The animals tolerated this procedure well and appeared in no acute distress at the time of electrode placement.
For the duration of the recording, the animals were gently restrained with broad straps and adhesive tape such that the torso and limbs were immobilized, but the head and tail had full freedom of movement to monitor for clinical seizures. The EEG signal was amplified and recorded using a Grass 15A94 amplifier with Grass Gamma 4.3 acquisition software (Grass-Telefactor, West Warwick, RI). Mice were monitored continuously by either video camera or direct observation, and movement artifact on tracings was minimal. For review, the tracings were filtered at 1–70 Hz and viewed as a bipolar montage of the three available cranial electrode pairs along with continuous EKG. The tracings were analyzed by a single electrophysiologist (A.R.) blinded to the animals' genotype.
Results
Neurodevelopment of mice with a deletion of Tsc1 in neurons
To explore the effects of loss of Tsc1 in neurons, we interbred a conditional allele of Tsc1 (Tsc1c ) with a synapsin I promoter-driven cre recombinase allele (SynICre) that has been shown to lead to recombination of nearby loxP sites in the majority of neurons beginning at E12.5 (Zhu et al., 2001). Onset of cre recombinase expression at E12.5 and localization to spinal cord and brain was confirmed through use of a lacZ reporter allele (data not shown). Tsc1c−SynICre + mice were derived from breeding schemes that also generated Tsc1cwSynICre + and Tsc1c−SynICre− mice, which were used as controls (w denotes wild-type allele; − denotes null allele). Control mice showed no phenotype, and >95% survived >6 months. We chose to study Tsc1c−SynICre + as opposed to Tsc1ccSynICre + mice, because the systemic loss of one allele of Tsc1 in the former matches the genotype of TSC patients with a mutation in TSC1.
Tsc1c−SynICre + mice were born in Mendelian ratios (19 of 79 pups were Tsc1c−SynICre + genotyped at P7 in one breeding scheme, compared with 25% expected) and were indistinguishable from control littermates until ∼P5. Thereafter, they failed to gain weight at the same rate as control littermates. By P10, hyperactivity and an enhanced startle response were apparent, as well as a progressive high-frequency (10–15 Hz) trunk and limb tremor at rest. Tsc1c−SynICre + mice had a median survival of 35 d, none survived past 65 d, and their average maximum weight was 10 g (Fig. 1 A,B).
Tsc1c−SynICre + survival, weight gain, phenotype, and EEG. A , Cumulative survival curve for Tsc1c−SynICre + (filled squares) and control (open squares) mice. B , Weight gain of Tsc1c−SynICre + (filled squares) and control (open squares) mice. C , Photograph of P21 Tsc1c−SynICre + mouse demonstrates hunched back, Straub tail, and out-turned paws. D , EEG segments (10 s) showing normal continuous control mouse background (I), a spike burst occurring in a somewhat irregular background in a mutant mouse (II), relative high-frequency desynchronization during a tonic seizure in a Tsc1c−SynICre + mouse (III), and frequent high-amplitude sharp waves in a mutant mouse (IV).
Neurologic assessment indicated that Tsc1c−SynICre + mice had dorsiflexion of the tail (Straub tail) (Fig. 1 C) and posterior limb-clasping behavior when lifted by their tails. Tsc1c−SynICre + mice showed a progressive decline in activity with limited mobility and development of a humped posture, typically in the third or fourth week. Most deaths occurred in the third to fifth postnatal week, and mice were typically found postmortem in an extensor posture of both the forelimbs and hindlimbs.
Seizure activity in mice with a deletion of Tsc1 in neurons
In addition to the neurological abnormalities described above, Tsc1c−SynICre + mice also developed clinical seizures. Spontaneous seizure activity was seen in ∼10% of mice, but seizures were more consistently provoked by physical stimulation, such as handling and sudden movements of the cage. Two seizure types were observed. Severe seizures, seen both spontaneously and with handling, were characterized by a brief (1–3 s) behavioral arrest, followed by several seconds of clonic activity, followed by tonic extensor posturing of trunk and limbs for 15–45 s. When suspended by the tail after age P21, gentle spinning consistently led to this sequence of events followed by bradycardia and death. A second milder seizure type seen only spontaneously was brief myoclonic jerking of head and torso.
To further characterize the seizures of Tsc1c−SynICre + mice, digital EEGs were recorded from seven mutant and 11 control littermates at ages P21–P48 for 1–3 h. Control mice showed the expected 4–6 Hz background activity at rest with appropriate reactivity to salient stimuli (Fig. 1 D, I). Three electrographic abnormalities were recorded in the mutant mice: (1) short spike bursts (seven of seven mice), (2) spontaneous periods of desynchronization with electrodecrement (one of seven), and (3) frequent high-amplitude sharp waves (one of seven). The interictal 1–2 s bursts of high-amplitude 7–8 Hz spikes (Fig. 1 D, II) seen in all mutants resembled pentylene tetrazole-triggered spikes in control mice (data not shown). Two short bursts of similar spikes were recorded in one of the 11 control mice (p = 0.0003; Fisher exact test, compared with mutants). However, the average frequency of these epileptiform discharges was much higher in the Tsc1c−SynICre + mice (2.8 vs 0.1 bursts/h in controls; p = .001; Mann–Whitney). In six of seven Tsc1c−SynICre + mice, the spontaneous spike bursts were without obvious clinical correlate.
However, in one of seven Tsc1c−SynICre + mice, the spike bursts were temporally associated with myoclonic jerks of head and torso. The same animal also had a single unprovoked seizure characterized clinically by unresponsiveness with tonic stiffening of torso and tail. This was a fatal tonic seizure that led to bradycardia within 2 s of electrographic seizure onset and death 19 s after clinical onset. Electrographically, the seizure started as 12–14 Hz low-amplitude activity (Fig. 1 D, III) and evolved to 2–3 Hz rhythmic high-amplitude spikes, followed by reduction in EEG amplitude and ultimate loss of EEG signal, likely reflecting brain death. Additionally, four of four Tsc1c−SynICre + mice displayed an identical electroclinical sequence after gentle tail spinning.
One Tsc1c−SynICre + mouse had frequent high-amplitude sharp waves throughout the recording period (Fig. 1 D, IV). These were without clinical correlate and were neither rhythmic nor sustained sufficiently to qualify as electrographic seizures.
In aggregate, the observed electrographic abnormalities and clinical seizures, including two seizure types captured on EEG, indicate that the Tsc1c−SynICre + mice have a marked tendency toward early-onset epilepsy. We considered the possibility that poor feeding and/or metabolic factors might contribute to these EEG abnormalities and seizures. However, serum Na+, glucose, blood urea nitrogen, and Ca2+ levels at age 30 d were similar among Tsc1c−SynICre + mice and controls.
Analysis of brain-specific recombination in Tsc1
We confirmed that recombination at the Tsc1c allele occurred in the brains of the Tsc1c−SynICre + mice by several methods. First, Southern blot analysis indicated that there was substantial conversion of the c to the − allele in cortex and diencephalon by age 3 weeks, whereas in contrast, relatively little recombination occurred in the cerebellum (Fig. 2 A). Second, PCR analysis showed that there was substantial conversion of the c allele to the − allele in brain DNA preparations from the mice (data not shown). Third, immunoblot analysis showed that there was a major reduction in the amount of Tsc1 and Tsc2 present in whole-brain homogenates prepared from the Tsc1c−SynICre + mice compared with controls (Fig. 2 B). Reduction in Tsc2 protein levels was expected, given its dependence on Tsc1 expression for stabilization (Benvenuto et al., 2000). Complete loss of Tsc1 expression would not be expected if recombination is restricted to neurons, as reported previously for this SynICre allele (Zhu et al., 2001). Also consistent with loss of Tsc1 was the marked increase in levels of pS6 in brain lysates (Fig. 2 B), a protein known to be phosphorylated at high levels in cells lacking Tsc1 or Tsc2 (Kwiatkowski et al., 2002; Onda et al., 2002; Tavazoie et al., 2005). Similar amounts of NeuN and NSE were seen in mutant and control brains, indicating that the overall amount of neuronal protein was similar in these brain homogenates.
Loss of Tsc1 and brain structural abnormalities in the Tsc1c−SynICre+ mice. A , Southern blot analysis demonstrating recombination in brain DNA samples from Tsc1c−SynICre + compared with Tsc1c−SynICre− mice. The 4.2 kb (c allele) and 2.4 kb (− allele) bands are of equal intensity in the Tsc1c−SynICre− samples, whereas there is a marked shift from the 4.2 kb to the 2.4 kb band in the Tsc1c−SynICre + samples from cortex (Cor) and diencephalon (Dien) but not cerebellum (Cere). B , Immunoblot analysis showing reduction in expression of both tuberin (Tsc2) and hamartin (Tsc1), and elevated pS6 (S240–244) in the brains of Tsc1c−SynICre + mice. AKT is a loading control. NeuN and NSE blots show no difference between Tsc1c−SynICre + and control mice. C, D , Coronal sections from P21 Tsc1cwSynICre + ( C ) and Tsc1c−SynICre + ( D ) mice stained with H&E demonstrate an additional layer of cells at the base of the mutant cortex (asterisk) and widespread cell enlargement ( Ca, Da ). Cb, Cc, Db, Dc , Higher magnification of cortex layer V ( Cb, Db ) and layer VI ( Cc, Dc ) shows enlarged cells in both of these regions of Tsc1c−SynICre + brain. E, F , Combined X-gal–pS6 immunoperoxidase staining of coronal sections reveals widespread recombination in the form of X-gal product, which is blue in both Tsc1cwSynICre + ( E ) and Tsc1c−SynICre + mice ( F ). Ea, Fa , In contrast to control ( Ea ), in the Tsc1c−SynICre + brain ( Fa ), enlarged pS6+ cells (brown) in layer V, base of cortex (asterisk), and the stratum oriens (arrowheads) of the hippocampal CA1, associate with the X-gal blue precipitate. Eb, Fb , High-power view of stratum oriens shows a correlation between blue stain indicating cre expression, pS6 positivity, and cell enlargement in Tsc1c−SynICre + mice. Scale bars: Ca, Da , 50 μm; Cb, Cc, Db, Dc , 25 μm; Ea, Fa , 20 μm; Eb, Fb , 25 μm.
Cortical and hippocampal structural abnormalities in Tsc1c−SynICre+ mice
Cortical tubers in TSC patients are characterized by a regional loss of normal cortical architecture and the presence of enlarged cells. Therefore, we asked whether cortical architecture was preserved in the Tsc1c−SynICre + mice. Hematoxylin and eosin (H&E) staining of P21 coronal sections demonstrated that laminar organization in the cerebral cortex was less distinct in Tsc1c−SynICre + mice than in the six cortical layers of controls (Fig. 2 Ca,Da). Furthermore, unusually large cells were seen in each of the six cortical layers in Tsc1c−SynICre + mice, particularly layer V (Fig. 2 Cb,Db). In addition, in contrast to control cortex (Fig. 2 Ca,Cc), a layer of enlarged cells was seen at the gray–white border throughout the mutant cortex at P21 (Fig. 2 Da, asterisk, Dc). These findings indicate cell enlargement in the neocortex of the Tsc1c−SynICre + mice, similar to that seen in cortical tubers in TSC patients.
Because the hippocampal formation is associated with epileptic discharges in many mouse models, we also analyzed the cytoarchitecture of the hippocampus. Although overall the structural organization of the hippocampus was normal, enlarged cells were seen throughout the pyramidal cell layer, especially in the cornu ammonis 3 (CA3) region (data not shown) (see below). Many enlarged cells were also seen within the hilus of the dentate gyrus in mutant animals. Enlarged ectopic cells were also seen outside the CA1–CA3 fields in the stratum oriens and stratum radiatum (data not shown). In addition to the neocortex and the hippocampus, enlarged cells were also seen in other brain regions, including subcortical gray matter structures such as thalamus, hypothalamus, and brainstem. Despite these changes in cell distribution and size, there was no evidence of increased cell loss or degeneration in any brain area by H&E staining, silver staining, or Fluoro Jade B staining (data not shown).
To confirm that recombination and loss of Tsc1, and subsequent mTORC1 activation, were occurring in the enlarged cells, we used a lacZ reporter allele. The X-gal blue precipitate was seen widely distributed in the cortex and hippocampus of both Tsc1c−SynICre + and Tsc1cwSynICre + mice and was strongest and most uniform in cortical layer V, the base of the cortex, and the CA3 region, and least consistent in the CA1 region (Fig. 2 E,F). In Tsc1c−SynICre + mice, accumulation of X-gal stain in layer V and at the cortical–white matter border was accompanied by the presence of enlarged, strongly pS6+ cells (Fig. 2 Fa). In contrast, cells located in the CA1 pyramidal layer demonstrated little or no X-gal staining, as well as low pS6 expression and relatively normal morphology. However, in the stratum oriens above CA1, numerous cells containing the X-gal blue precipitate were enlarged and pS6 positive (Fig. 2 Fb). In contrast, in controls X-gal blue precipitate was seen in cells of normal size without pS6 staining in the stratum oriens (Fig. 2 Ea,Eb). These observations indicate that recombination and loss of Tsc1 is not occurring in all neurons, but rather a major subset, consistent with previous observations using this SynICre allele (Zhu et al., 2001).
mTORC1 activation in enlarged neurons of the neocortex, hippocampus, and subcortical gray matter
To determine the cellular specificity of Tsc1 loss and subsequent mTORC1 activation, the nature and distribution of the enlarged cells were examined in greater detail. We used neuronal markers NeuN, SMI 311, GAD-67, and the astrocytic marker GFAP, in concert with pS6 and Tsc1, to indicate mTORC1 activation and directly confirm Tsc1 loss. Relatively weak pS6 staining was seen in normal-appearing pyramidal neurons throughout the cortex and subcortical gray matter of the control brain (Fig. 3 A–C,G–I). Intense pS6 reactivity was observed in the majority of enlarged and ectopic NeuN+ neurons throughout the Tsc1c−SynICre + brain. Both motor and sensory cortices were strongly pS6+, with highest expression seen in the pyramidal cell layers (II/III and V), and the extra layer of cells below layer VI (Fig. 3 D–F,J–L). Enlarged pyramidal neurons in the Tsc1c−SynICre + mice had also lost expression of Tsc1 (supplemental Fig. 1, compare D–F with A–C, available at www.jneurosci.org as supplemental material). Strongly pS6-positive cells of normal size were found in the piriform cortex and the supraoptic nucleus of control brains (data not shown), possibly related to a high level of translational activity in those cells.
Increased pS6 and widespread architectural abnormalities in P21 Tsc1c−SynICre + mice. A–F , In the RSG region of the motor cortex, there is increased pS6 expression in multiple cell layers, including a layer of pS6+ neurons at the base of the cortex in Tsc1c−SynICre + mice ( D–F ). G–L , In the somatosensory cortex, pS6+ neurons are prominent in cortical layer V and at the gray–white matter border at the base of the cortex in Tsc1c−SynICre + mice ( J–L ). Occasional large pS6+ neurons are seen in the CA1 pyramidal cell layer of the hippocampus but are also seen ectopically in the stratum oriens. M–R , In the hippocampal CA3 region, nearly all neurons are pS6+, including those outside the pyramidal cell layer in Tsc1c−SynICre + mice ( P–R ). S–X , In the dentate gyrus, there are occasional enlarged pS6+ cells in the granule cell layer in Tsc1c−SynICre + ( V–X ) mice. However, cells within the hilus are more severely affected, and ectopic pS6+ neurons are also apparent. Scale bars: A–F , 85 μm; G–X , 50 μm.
pS6 expression was highly variable within the CA1 region of the Tsc1c−SynICre + hippocampus. A fraction of CA1 pyramidal neurons were highly pS6+ and enlarged, and those cells were typically seen at the margin of the stratum pyramidale or were ectopically placed in the stratum oriens [Figs. 2 Fb, 3, compare J–L with G–I (control)]. In contrast, nearly all neurons in the CA3 region of the hippocampus were enlarged and pS6+, but similar to the CA1 region, many pS6+ neurons were seen in both the stratum oriens and stratum radiatum [Fig. 3, compare P–R with M–O (control)]. There were occasional large pS6+ neurons in the granule cell layer of the dentate gyrus, but the majority of cells showed weak pS6 staining [Fig. 3, compare V–X with S–U (control)]. However, many strongly pS6+ enlarged neurons were seen in the hilus of the dentate gyrus [Fig. 3, compare V–X with S–U (control)].
We also observed enlarged, strongly pS6+ neurons in many other regions of the Tsc1c−SynICre + brains, including thalamus, hypothalamus, and the red nucleus of the brainstem (supplemental Fig. 2, available at www.jneurosci.org as supplemental material). In contrast, other subcortical regions were largely unaffected, including caudate and putamen (data not shown). It has recently been noted that mTORC1 activity in the hypothalamus plays a critical role in the regulation of food intake (Cota et al., 2006). The poor weight gain seen in these mice was severe, and although this may have been caused by generalized effects of brain dysfunction, it is possible that overactive mTORC1 in the hypothalamus contributed to reduced food intake.
Interneurons were widely distributed in the Tsc1c−SynICre + mouse brain, as assessed by staining for GAD67, a biosynthetic enzyme required for generation of the inhibitory GABA neurotransmitter. These cells were generally pS6+ and enlarged [Fig. 4, compare D–F with A–C (control)]. Many of the ectopic neurons seen in the subcortical white matter (Fig. 4 F, asterisk), hippocampal stratum oriens, and dentate hilus (data not shown) were pS6+ GAD67+ interneurons. Tsc1 expression was lost in those GAD67+ cells that were enlarged (supplemental Fig. 1, compare J–L with G–I, available at www.jneurosci.org as supplemental material). These observations indicate that both excitatory and inhibitory neurons are affected in this model.
Tsc1c−SynICre + interneurons are pS6+ and enlarged. A–F , Confocal images demonstrate that GAD67+ interneurons in P21 Tsc1c−SynICre + mice ( D–F ) are enlarged and pS6+ compared with control brain interneurons ( A–C ). Insets, Size comparison for single cells (arrowheads). In addition, some ectopic neurons in the white matter of Tsc1c−SynICre + brains are pS6+ GAD67+ interneurons (*). Scale bars, 20 μm.
Double labeling for pS6 and GFAP (for mature astrocytes) demonstrated that astrocytes throughout the brain, including hippocampus and cortex, were not enlarged and were not pS6+ in Tsc1c−SynICre + mice (Fig. 5 D–I). In addition, Tsc1 expression was preserved in astrocytes (supplemental Fig. 1M–R, available at www.jneurosci.org as supplemental material). The distribution and degree of GFAP expression was comparable in Tsc1c−SynICre + and controls in all brain regions [Fig. 5, compare D–E with A–C (controls)], indicating that there was no reactive astrogliosis in these mice.
mTORC1 activation resulting from Tsc1 loss is restricted to neurons in Tsc1c−SynICre + mice. A–F , GFAP-positive astrocytes in the CA3 region of the hippocampus are distinct from pS6+ neurons in both P21 control ( A–C ) and Tsc1c−SynICre + ( D–F ) brains. D–I , The number and distribution of GFAP-positive cells in the Tsc1c−SynICre + hippocampus ( D–F ) and cortex ( G–I ) shows no evidence for astrogliosis in the mutant brain. Scale bars: A–F , 20 μm; G–I , 50 μm.
These observations indicate that the clinical phenotype of the Tsc1c−SynICre + mice was attributable to selective neuronal loss of Tsc1, with no contribution from astrocyte Tsc1 loss or secondary astrogliosis.
Patterns of neuronal dysplasia are seen in Tsc1c−SynICre+ mice
Dysplastic enlarged neurons are a characteristic feature of human TSC tubers, in addition to giant cells (Arseni et al., 1972; Huttenlocher and Heydemann, 1984; Hirose et al., 1995; Crino, 2004; Miyata et al., 2004). Abundant Nissl substance and cytoskeleton abnormalities, such as abnormal cytoplasmic accumulation of argyrophilic fibrils and increased expression of neurofilament proteins, are the most prominent characteristics of dysplastic neurons in cortical tubers (Huttenlocher and Heydemann, 1984; Hirose et al., 1995). To delineate such cells in the Tsc1c−SynICre + brains, we used expression of nonphosphorylated neurofilament (SMI 311). In control mice, SMI 311 labeled a defined subpopulation of weakly pS6+ pyramidal neurons belonging to cortical layers III, V, and (rarely) nonpyramidal layer VI neurons (Fig. 6 A–D) (Ulfig et al., 1998; da Silva et al., 2005). This staining was particularly strong in the retrosplenial granular (RSG) cortex (Fig. 6 A–C). In the Tsc1c−SynICre + brains, nonphosphorylated neurofilament staining was stronger, and nearly all SMI 311+ neurons were intensely pS6+ (Fig. 6 E–G,H). Many SMI 311+ cells in Tsc1c−SynICre + mice demonstrated a clear pyramidal morphology but were larger with thicker dendritic arbors than their counterparts in control mice (Fig. 6, compare H–I with D). SMI 311+, pS6+ neurons in the hippocampus demonstrated similar dysplastic features (Fig. 6 J). Nissl bodies and filamentous aggregates were also detected in enlarged neurons by thionine and silver staining, most prominently in the brainstem, although rarely in enlarged cortical cells (data not shown). Some of these neurons were aberrantly localized outside the primary pyramidal cell layers, including the molecular layer and subcortical white matter (Fig. 6 E–G). These ectopic neurons were isolated and not incorporated into clusters or columns, and some neurons showed abnormal polarity (inverted pyramids) (data not shown). None of these enlarged, pS6+ neurons expressed neuroprogenitor or glial markers, such as nestin or GFAP (data not shown).
Enlarged, dysplastic pyramidal neurons in Tsc1c−SynICre + brains. A–C, E–G , In the RSG region of the motor cortex, the majority of pyramidal neurons identified by SMI 311 staining in layers V and III are strongly pS6+ in P21 Tsc1c−SynICre + ( E–G ) mice, in contrast to controls ( A–C ). E–G , Disruption of normal cortical lamination in Tsc1c−SynICre + mice is also evident, with enlarged SMI 311+/pS6+ cells outside layers III and V. H , Confocal images of layer V pyramidal neurons show enlarged dysplastic neurons with thickened dendritic arbors in Tsc1c−SynICre + mice (compare with D ). I, J , Higher-power view of typical enlarged dysplastic SMI 311+/pS6+ neurons in cortical layer V ( I ) and in the granule cell layer of the dentate gyrus ( J ) in Tsc1c−SynICre + mice. K , Quantitative size analysis of SMI 311+ cells (y-axis, pixels) in layer V (−2 to −2.2 mm from bregma and 3.2–3.4 mm lateral to midline) shows increased soma size in Tsc1c−SynICre + mice when compared with controls (p = 0.0002). Scale bars: A–C, E–G , 100 μm; D, H , 25 μm; I, J , 10 μm.
To confirm a difference in neuronal cell size, we measured the total soma area of all SMI 311+ cells in layer V in matched 20× fields of somatosensory cortex using confocal images from Tsc1c−SynICre + and control mice. There was a significant, 60% increase in soma area in Tsc1c−SynICre + mice compared with age-matched controls (p = 0.0002) (Fig. 6 K). This difference in cell size caused by loss of Tsc1 clearly parallels the cell enlargement seen in both dysplastic neurons and giant cells of human TSC cortical tubers.
Reduced myelination is seen in Tsc1c−SynICre+ mice
Because hypomyelination is a feature of human TSC lesions (Ridler et al., 2001), we examined myelination in the Tsc1c−SynICre + mice. Reduced MBP expression was seen throughout the mutant brain, being most pronounced in the cortex [Fig. 7, compare D, A (control)] and hippocampus [supplemental Fig. 3, compare F, B (control), available at www.jneurosci.org as supplemental material], but also seen in the thalamus and hypothalamus (data not shown). There appeared to be a correlation between the increase in pS6 expression in cortical neurons and the regional reduction in myelination [Fig. 7, compare D–F with A–C (control)], suggesting that this effect was caused by neuronal loss of Tsc1. MBP expression was significantly reduced in the Tsc1c−SynICre + mice at P7, P14, and P21, demonstrating that there was myelination failure as opposed to a demyelinating process [Fig. 8, compare D–F with A–C (control)].
Hypomyelination in Tsc1c−SynICre + brains. A–F , Compared with controls ( A–C ), the RSG region of motor cortex of Tsc1c−SynICre + brains shows a marked reduction in MBP expression ( D–F ) in the corpus callosum, the pericallosal white matter, and radiating fibers extending into the cerebral cortex. Scale bars, 100 μm.
Developmental analysis of MBP expression, oligodendrocyte distribution and differential expression of neuronal proteins in Tsc1c−SynICre + mice. A–F , MBP expression (red) is reduced at P7, P14, and P21 in the external capsule of Tsc1c−SynICre + cortex ( D–F ) compared with controls ( A–C ). A persistent immature patchy pattern of MBP expression is seen throughout development in the mutant cortex. G–K , Premyelinating oligodendrocytes, as assessed by GalC (red; G, I ) and O4 (red; J, K ) staining, are present throughout the P7 Tsc1c−SynICre + brain but are pS6 negative (green; H, I, K ). L , Immunoblot analysis of brain lysates shows that MBP levels are reduced in Tsc1c−SynICre + brains, whereas levels of nonphosphorylated and phosphorylated medium chain neurofilament and GAP-43 are increased, compared with controls. Scale bars: A–F , 50 μm; G–K , 20 μm.
To determine whether there was a role for oligodendrocyte loss or dysfunction in the myelination deficit, we analyzed immature oligodendrocytes and oligodendrocyte precursors in the cortex and subcortical white matter by staining for galactocerebroside GalC and O4 (Boggs et al., 2004; Polito and Reynolds, 2005)(Fig. 8 G–K). In contrast to the MBP deficiency, GalC+ and O4+ oligodendrocytes were widely distributed throughout the brain and did not differ from control mice (data not shown). Double staining with pS6 and GalC (Fig. 8 G–I) or O4 (Fig. 8 J–K) showed that these cells were pS6 negative, suggesting that they were expressing normal levels of Tsc1.
Because oligodendrocyte distribution and number appeared similar in Tsc1c−SynICre + mice and controls, we examined whether this myelination failure was attributable to an axonal defect. Axons were identified by staining for the NF 160 kDa isoform. Despite the major reduction in myelination in the hippocampus and cortex, axonal pro-jections appeared normal in the Tsc1c−SynICre + mice in these regions [supplemental Fig. 3, compare H, M–P with A–D, I–L (controls)].
To examine potential differences in MBP and NF isoform expression in greater detail in the Tsc1c−SynICre + brains, immunoblot analysis of whole-brain homogenates was performed. MBP expression was significantly reduced, and levels of phosphorylated and nonphosphorylated medium chain NF were both increased in Tsc1c−SynICre + brains compared with controls (Fig. 8 L). Moreover, GAP-43 expression was significantly increased in whole-brain homogenates from the Tsc1c−SynICre + mice, compared with controls. Because GAP-43 expression is a marker for active growth cones, these results suggest that the Tsc1c−SynICre + neurons are still actively growing. Thus, these results in aggregate suggest that there is a primary axonal developmental defect caused by loss of Tsc1, which leads to a secondary myelination failure.
Comparison between Tsc1c−SynICre+ and Tsc1ccSynICre+ mice
We considered the possibility that the phenotype of the Tsc1c−SynICre + mice might be more severe than that seen in Tsc1ccSynICre + mice, because of effects of 50% expression of Tsc1 in all cells, including astrocytes, oligodendrocytes, and neurons in which recombination did not occur. However, clinical features, survival, and brain pathology, including neuronal enlargement, pS6 expression, and lack of myelination, were all indistinguishable in mice of these two genotypes (data not shown). The reduced myelination in the Tsc1ccSynICre + mice provides additional evidence that oligodendrocyte abnormalities do not contribute to this effect.
Discussion
Here, we have used a Tsc1 floxed allele combined with a Synapsin I promoter-driven Cre allele to eliminate Tsc1 in the majority of differentiating neurons beginning at E13. This novel model provides the opportunity for analysis of the in vivo functions of the Tsc proteins in neuronal development and matches multiple clinical and neuropathological features that are seen in TSC patients. The survival of the mutant mice is markedly compromised, because of poor development with a wasting syndrome, and the mice exhibit spontaneous seizures as well as enhanced seizure susceptibility and EEG abnormalities. Furthermore, the brain cytoarchitecture in these mice is highly abnormal. Enlarged, highly pS6+, Tsc1-negative, dysplastic neurons are seen throughout the cortex, hippocampus, and other subcortical gray matter regions, many of which have thickened dendritic arbors and are in ectopic positions. Aberrant cortical lamination is evident throughout the mutant brain, and an additional layer of enlarged pS6+ neurons is present at the base of the cortex. Myelination is also markedly reduced in a pattern indicative of a secondary myelination defect caused by axonal dysfunction resulting from loss of Tsc1 in neurons. It is notable that none of these findings were seen in Tsc1c− mice or in Tsc1cwSynICre + mice, which made up most of the controls used in this study. Overall, this model highlights the critical function of the Tsc genes and proteins in neuronal function and development.
Most types of TSC hamartoma, including subependymal giant cell astrocytomas, follow the classic two-hit paradigm for complete loss of tumor suppressor gene function, in which an inherited, germline, inactivated allele is complemented by somatic loss of the second (wild-type) allele in hamartomas (Cheadle et al., 2000; Tucker and Friedman, 2002; Chan et al., 2004). However, the molecular pathogenesis of TSC cortical tubers has been less clear. Despite concerted attempts, loss of heterozygosity for a TSC1 or TSC2 allele has been seen in very few lesions (Tucker and Friedman, 2002). Laser-capture microdissection to isolate tuber giant cells has also failed to provide evidence for two-hit pathogenesis, leading to the proposal that alternative genetic events might contribute to tuber development (Han et al., 2004). Nonetheless, much circumstantial evidence points to complete loss of gene function in a subset of cells comprising TSC tubers as key to tuber development. Tuber giant cells have markedly increased expression of pS6 and other markers of mTORC1 activation (Baybis et al., 2004; Miyata et al., 2004). Murine neuroepithelial precursor cells lacking Tsc2 are enlarged and have an aberrant mRNA expression pattern similar to tuber giant cells (Onda et al., 2002). Reduction of Tsc1 or Tsc2 in murine hippocampal slice cultures leads to cell-autonomous enlargement, with extensive abnormalities of the dendritic spines (Tavazoie et al., 2005). The dysplastic, enlarged, and ectopic neurons generated in the current model, in which complete loss of Tsc1 occurs during neuronal differentiation, provide additional strong support for the two-hit model for tuber pathogenesis.
Although the model we have generated directly tests the function of Tsc1 in neurons in vivo, it is remarkable that the degree of reduction in Tsc2 expression is essentially the same as that seen for Tsc1 (Fig. 2 B). This is consistent with observations on the role of Tsc1 as a critical binding partner of Tsc2 that prevents its degradation (Benvenuto et al., 2000; Chong-Kopera et al., 2006). Thus, it is likely that loss of Tsc1 and loss of Tsc2 have equivalent effects on mTORC1 and other signaling abnormalities leading to aberrant neuronal development.
The clinical and neuropathologic phenotype of the Tsc1c−SynICre + mice has several important similarities to that observed in human TSC patients. Cortex and hippocampus are significantly affected, with many enlarged pS6+ dysplastic neurons, as well as hypomyelination. Other areas with abnormal cytoarchitecture include the red nucleus, and these changes are likely to contribute to the abnormal tone (clasping) and tremor observed in these mice. The mice display a high incidence of stimulation-evoked and spontaneous seizures. Because the majority of neurons are affected by the mutation, there is widespread disruption of laminar organization in cortex and hippocampus, and both interictal and ictal EEG show lack of substantial synchrony. Although most neurons undergo recombination and loss of Tsc1, the mixture of Tsc1c− and pS6+ neurons is similar to the mixture of cell types present in TSC cortical tubers.
The Tsc1c−SynICre + mice demonstrated an early-onset seizure disorder, which appeared in many cases to cause the death of older animals. In contrast to previous suggestions that seizures in TSC might be related to astrocyte dysfunction consequent to loss of Tsc1/Tsc2 (Uhlmann et al., 2002; Wong et al., 2003), these observations establish that neuronal loss of Tsc1/Tsc2 leads to clinically important seizure predisposition. These in vivo findings are consistent with previous in vitro data demonstrating that loss of Tsc1 and Tsc2 in neurons leads to enhanced glutamatergic neurotransmission (Tavazoie et al., 2005).
Enlarged multinucleated giant cells, such as those seen in TSC cortical tubers, are not seen in these mice. We suspect that this is because of the timing of loss of Tsc1 in this model, with cre-mediated recombination occurring at the beginning of neuronal differentiation (E12.5) (Zhu et al., 2001) (data not shown) and loss of Tsc1 protein following thereafter. Indeed, loss of Tsc1 engineered through use of a nestin promoter-driven cre in neuroepithelial progenitor cells, as early as E8.5, leads to mice with markedly enlarged “giant” cells in the cortex and hippocampus (H. Onda and D. J. Kwiatkowski, unpublished observations), consistent with an important developmental effect of loss of Tsc1. Others have also proposed that second hit events occur in TSC patients at earlier time points in brain development to lead to generation of giant cells (Ess et al., 2005). A previously described Tsc mouse model, in which the Tsc1c allele was combined with a GFAP-cre allele, also had a pronounced seizure phenotype, shortened survival (although much longer than seen here), generalized astrogliosis, and hippocampal neuronal abnormalities (Uhlmann et al., 2002; Wong et al., 2003; Ess et al., 2004). However, cortical neuronal abnormalities were not seen in those mice, and it was not clear whether the seizure predisposition was attributable to astrocytic or hippocampal neuronal loss of Tsc1. Nonetheless, both neurons and astrocytes are abnormal in TSC tubers, and likely both contribute to epileptogenesis.
Cortical tubers occur as multiple, discrete supratentorial gray matter lesions in which normal cortical lamination is disrupted. In contrast, the Tsc1c−SynICre + mouse brain is more diffusely affected both cortically and subcortically. Changes in cortical lamination were delineated by analysis of NeuN and pS6 expression in the Tsc1c−SynICre + mice, demonstrating an additional layer of enlarged pS6+ neurons at the base of the cortex. It is possible that these cells are residual subplate cells that have failed to undergo apoptosis, as they are seen in control brains at P7. However, aberrantly positioned (“ectopic”) cells were widespread in the white matter and hippocampus, suggesting that neuronal migration was more generally perturbed in these mice because of loss of Tsc1. This phenomenon may be related to cytoskeletal abnormalities in Tsc1-deficient neurons, including abnormal neurofilament expression (Fig. 8 L) and elevated levels of phospho-cofilin (Tavazoie et al., 2005).
Myelination defects are commonly observed in the TSC brain, both focally within tubers and more diffusely (Ridler et al., 2001; Zikou et al., 2005). However, it has been unclear whether the defect in myelination is a cell-autonomous defect caused by loss of TSC function in oligodendrocytes or indirect as a result of neuronal dysfunction. Previous studies have indicated that in the adult CNS, myelin and growth-associated protein GAP-43 have an inverse regional distribution (Kapfhammer and Schwab, 1994). Furthermore, after suppression of myelination by X-irradiation of the spinal cord, GAP-43 is upregulated. These experiments have led to the hypothesis that myelin-associated inhibitors stabilize neuronal growth and limit plasticity in the adult CNS. Although the effect of oligodendrocyte-derived inhibitors on neurons is well established, less is known about the effect of neurons on oligodendrocyte development. Accumulating evidence suggests that neuron-derived factors can regulate oligodendrocyte development at multiple stages, such as proliferation, survival, differentiation, and formation of myelin (Barres and Raff, 1999; Simons and Trajkovic, 2006). Thus, there appears to be mutual regulation of neurons and oligodendrocytes that is required for proper myelination and effective neuronal function.
Striking myelination delay was seen in the Tsc1c−SynICre + mice from P7 through P21. GAP-43, which is normally expressed during axonal outgrowth before P7 (Erzurumlu et al., 1990), was highly expressed in P21 Tsc1c-SynICre + mice suggesting that axons are in a persistent growth-enabled state because of the loss of Tsc1 (Benowitz and Routtenberg, 1997). The normal distribution of premyelinating oligodendrocytes and their lack of pS6 expression suggest that oligodendrocytes have normal levels of Tsc1 and are not directly affected in this model. Rather, it appears that loss of Tsc1 in neurons causes a lack of induction of myelination, consistent with an important developmental role of interaction between neurons and oligodendrocytes (Boiko and Winckler, 2006). It is not clear whether loss of Tsc1 leads to abnormal expression of neuronal signaling molecules that can regulate oligodendrocyte development. Alternatively, loss of Tsc1 can interfere with intracellular signaling pathways such as those regulating rho GTPases. Many axon guidance molecules such as Semaphorin 3A and myelin-associated inhibitors, including Nogo, reduce axonal growth cone extension in a signaling pathway that involves rhoA, ROCK, and LIM kinase, and leads to phosphorylation of cofilin at S3 (Wu et al., 2005; Hsieh et al., 2006). The recent observation that pS3-cofilin levels are increased in single neurons lacking Tsc1 (Tavazoie et al., 2005) and evidence of an interaction between Tsc1/Tsc2 and rho (Lamb et al., 2000; Astrinidis et al., 2002; Goncharova et al., 2004) suggest that alterations in rho activation in neurons lacking Tsc1 may lead to growth cone developmental abnormalities causing this myelination defect. Experiments investigating the role of Tsc proteins in the neuron–oligodendrocyte interaction using cocultures systems are underway and may shed light into the mechanisms of myelination in the CNS.
Neuron-specific deletion of Tsc1 provides a novel model to study the in vivo functions of the Tsc proteins in neuronal development and indicates that Tsc1/2 complex is critical for cell size, migration, neuritic outgrowth, and myelination in the developing brain. Based on previous in vitro studies, activation of the translational machinery via mTORC1 is likely to underlie many of the functions of TSC complex in this model, suggesting that the developmental defects observed in these mice may be reversible by inhibition of mTORC1 using rapamycin and its analogs. Treatment of Tsc1c−SynICre mice with rapamycin during different periods of development can provide critical preclinical data for use of rapamycin in TSC patients and also provide insights as to how and when the TSC/mTORC1 pathway and the associated translational machinery is involved in neuronal developmental processes such as cell size regulation, migration, axonal and dendritic arborization, and myelination.
Note added in proof.
In simultaneous studies performed on mice of this same genotype (founders provided by us), Wang et al. (2007) have recently reported on multiple aspects of histopathology, brain anatomy, and electrical activity in Tsc1ccSynICre + mice. In general, their findings are consistent with those reported here. However, they did not perform double labeling of brain sections with antibodies against pS6 and a variety of cell-specific markers, and we suspect that this accounts for their failure to observe the abnormalities of cortical organization and ectopic neurons that we have noted. In addition, Wang et al. (2007) did not find differences in the size of SMI 311+ neurons in mutant mice compared with controls in a two-dimensional study of randomly sampled neurons. This difference from the present study may be attributable to the fact that we sampled a population of SMI 311+ neurons in layer V of neocortex, in which neuronal size is homogeneous in controls. In addition, our use of 50 μm sections and confocal fluorescence microscopy (in contrast to Wang et al., 2007) may have afforded better quantitation of these differences.
Footnotes
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This work was supported by the National Institutes of Health National Institute of Neurological Disorders and Stroke NS24279 (D.J.K.), NS31718 (F.E.J.), the Tuberous Sclerosis Alliance (L.M., D.M.T., M.S., F.E.J., D.J.K.), and the Rothberg Courage Fund (D.J.K.). We thank Thomas Diefenbach and the Developmental Disabilities Research Center imaging core for assistance with confocal microscopy, Rod Bronson for assistance with brain pathology, Victoria Walker for technical assistance, Larry Benowitz for useful discussions on GAP-43, and Vijaya Ramesh for providing the Tsc1 antibody.
- Correspondence should be addressed to either of the following: David J. Kwiatkowski, One Blackfan Circle, 6-216, Division of Translational Medicine, Department of Medicine, Brigham and Women's Hospital, Boston, MA 02115, dk{at}rics.bwh.harvard.edu; or Frances E. Jensen, Enders 348, Neurology, Children's Hospital, Boston, 300 Longwood Avenue, Boston, MA 02115, E-mail: frances.jensen{at}childrens.harvard.edu