Extended Plasticity of Visual Cortex in Dark-Reared Animals May Result from Prolonged Expression of cpg15-Like Genes

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The Journal of Neuroscience, March 1, 2002, 22(5):1807-1815

Extended Plasticity of Visual Cortex in Dark-Reared Animals May Result from Prolonged Expression of cpg15-Like Genes
Wei-Chung Allen Lee and Elly Nedivi
Center for Learning and Memory, Departments of Brain and Cognitive Sciences and Biology, Massachusetts Institute of Technology, Cambridge, Massachusetts 02139

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

cpg15 is an activity-regulated gene that encodes a membrane-bound ligand that coordinately regulates growth of apposing dendriticand axonal arbors and the maturation of their synapses. Theseproperties make it an attractive candidate for participating inplasticity of the mammalian visual system. Here we compare cpg15expression during normal development of the rat visual systemwith that seen in response to dark rearing, monocular blockadeof retinal action potentials, or monocular deprivation. Our resultsshow that the onset of cpg15 expression in the visual cortex iscoincident with eye opening, and it increases until the peak ofthe critical period at postnatal day 28 (P28). This early expressionis independent of both retinal activity and visual experience.After P28, a component of cpg15 expression in the visual cortex,lateral geniculate nucleus (LGN), and superior colliculus (SC)develops a progressively stronger dependence on retinally drivenaction potentials. Dark rearing does not affect cpg15 mRNA expressionin the LGN and SC at any age, but it does significantly affectits expression in the visual cortex from the peak of the criticalperiod and into adulthood. In dark-reared rats, the peak levelof cpg15 expression in the visual cortex at P28 is lower thanin controls. Rather than showing the normal decline with maturation,these levels are maintained in dark-reared animals. We suggestthat the prolonged plasticity in the visual cortex that is seenin dark-reared animals may result from failure to downregulategenes such as cpg15 that could promote structural remodeling andsynapticmaturation.

Key words: dark rearing; visual system; cpg15; critical period; cortex; plasticity; TTX; monocular deprivation

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The critical period for susceptibility to environmental influences is one of the central concepts to emerge from studies ofvisual system development. The capacity for change in responseto manipulation of patterned visual input is normally restrictedto a defined age window during postnatal development (Hubel andWiesel, 1970; Hubel et al., 1977). However, in kittens or ratsdark-reared (DR) past the end of the normal critical period, manipulationof visual input results in significant plasticity of corticalbinocular connectivity as measured by electrophysiological recordings(Cynader and Mitchell, 1980; Mower et al., 1981; Fagiolini etal., 1994; Guire et al., 1999). This prolonged plasticity is notaccompanied by a prolonged plasticity measured by anatomical methods.When visualized by autoradiography of geniculocortical afferents,the segregation of ocular dominance columns is incomplete in DRcats and is not altered by later visual manipulations (Mower etal., 1985). The complexity of interpreting dark-rearing experimentshighlights our poor understanding of the molecular mechanismsthat underlie plasticity during the criticalperiod.

Electrophysiological studies of the rodent visual system show that cortical neurons develop well-defined functional propertiesrelating to eye preference and orientation selectivity, althoughthey are not anatomically segregated according to these propertiesas is seen in the visual cortex (VC) of cats and monkeys (Parnavelaset al., 1981; Maffei et al., 1992; Fagiolini et al., 1994; Gordonand Stryker, 1996; Antonini et al., 1999). In a manner similarto that in cats and monkeys, cells in the primary visual cortexof rodents are capable of undergoing shifts in eye preferenceduring a critical period in development (Drager, 1978; Fagioliniet al., 1994; Gordon and Stryker, 1996; Guire et al., 1999). Anatomicalstudies show that in mice, monocular deprivation (MD) during thecritical period affects arbor growth of thalamocortical afferents(Antonini et al., 1999). These studies, in combination with newtechnologies for manipulating mouse genetics, argue that the rodentvisual projection can be a valuable experimental system for examiningthe cellular and molecular mechanisms of developmentalplasticity.

Candidate plasticity gene 15 (cpg15) was isolated in a screen for seizure-induced genes in the dentate gyrus of the rat hippocampus(Nedivi et al., 1993). cpg15 expression is regulated by lightin the visual cortex of adult rats (Nedivi et al., 1996); itslocalization and regulation in the developing visual system ofcats are consistent with a role in activity-dependent plasticity(Corriveau et al., 1999). cpg15 overexpression in the developingXenopus optic tectum induces exuberant growth of dendritic arborsin tectal cells (Nedivi et al., 1998); this is accompanied byenhanced growth of retinal axon arbors and retinotectal synapseformation (Cantallops et al., 2000). The effects of cpg15 on thesedifferent aspects of circuit formation are all non-cell autonomous,consistent with its glycosylphosphatidylinositol cell-surfaceattachment (Nedivi et al., 1998; Cantallops et al., 2000).

The potential role of cpg15 in dendritic and axonal arbor restructuring and synaptic maturation led us to study the effectof dark rearing on its expression and regulation. We monitoredcpg15 mRNA levels in the visual structures of the rat before,during, and after the cortical critical period for the developmentof eye-specific preference. We compared the effects of dark rearingwith those of retinal action potential blockade and MD. Our resultssuggest a mechanism whereby the visual cortex of DR animals maintainsa capacity for delayed plasticity through elevated levels of genessuch as cpg15 that can enhance local circuit remodeling and newsynaptic stabilization. These results may provide a clue to theintriguing discrepancy seen in DR animals between the capacityfor change as measured by anatomical methods and that measuredby electrophysiologicalmethods.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animal manipulations and tissue isolation. All animal work was approved by the Massachusetts Institute of Technology Committeeon Animal Care; it conforms to National Institutes of Health guidelinesfor the use and care of vertebrate animals. Wistar-Kyoto rats(Taconic, Germantown, NY) were housed either in a room with a12 hr light/dark cycle or in a room sealed from visible light.A 15 W safelight shielded by a number 2 Kodak dark-red filter(Eastman Kodak, Rochester, NY) was used for the daily care andmaintenance of animals housed in the darkroom (~30 min/d). Atvarious points during the experiment, Polaroid (Cambridge, MA)photographic paper placed in the darkroom was monitored for exposure.In cats, intermittent exposure to a safelight can be sufficientto prevent the apparent extension of the critical period by darkrearing. To test whether exposure to a safelight affected thedark rearing of rats, a group of animals handled with an infraredviewing system (950 nm) was raised in the dark to 3, 4, 5, and8 weeks of age (each group, n = 3). The levels of cpg15 expressionin the rats handled with intermittent exposure to a safelightwere not significantly different from those handled under infraredconditions; both were significantly different from their age-matchedcontrols at 4 and 8 weeks (data not shown). The difference insensitivity to exposure to a safelight may reflect the relativelypoor vision of albino rats compared withcats.

Rats were reared under normal conditions (12 hr light/dark cycle), dark-reared from birth, or dark-adapted at different developmentaltime points. DR and age-matched control animals were killed postnatallyat progressive times, starting at postnatal day 10 (P10) and at1 week intervals from P14 (the approximate day of eye opening)to 8 weeks (P10, each group, n = 2; P14, P21, 5 weeks, 6 weeks,each group, n = 4; 4 weeks, DR, n = 4; controls, n = 3; 8 weeksDR, n = 3; controls, n = 5). A group of DR 8-week-old rats wasexposed to light for 6, 12, or 24 hr or for 7 or 14 d (n = 2-3for each time point). Dark-adapted adult rats were placed in thedark for 2 weeks and killed in the dark, with a parallel set killedafter re-exposure to 24 hr of light (each group, n = 3). Ratsthat were raised as dark-adapted until adulthood were raised normallyto 2, 3, 4, or 5 weeks; placed in the dark until 8 weeks; andkilled in the dark or after re-exposure to light for 24 hr (n= 3 per group per time point). Two additional groups of rats wereallowed a 1 week window of visual experience [between weeks 3and 4 (Lt3-4) or between weeks 4 and 5 (Lt4-5)] during dark rearing.At 8 weeks, these animals were killed in the dark (each group,n = 3) or after 24 hr of exposure to light (Lt3-4, n = 3; Lt4-5,n =2).

Monocular blockades of retinal action potentials were done essentially as described previously (Prusky and Ramoa, 1999). Astrip of Elvax containing either tetrodotoxin (TTX) or citratebuffer was surgically implanted into the vitreous of the lefteye of each animal for 3 d of sustained release, starting at P11,P18, P25, P32, P39, and P53 (TTX, n = 3; citrate, n = 2). Briefly,200 mg of washed Elvax beads (DuPont NEN, Wilmington, DE) weredissolved in methylene chloride. The dissolved Elvax was mixedwith 20 µl of 1% Fast Green in dimethylsulfoxide and either 20µl of 0.3 M TTX in citrate buffer (Calbiochem, La Jolla, CA) or20 µl of 18.6 mM citrate buffer (Sigma, St. Louis, MO). The methylenechloride was slowly evaporated over the course of 1 d at $-$ 70°Cand for 5 d subsequently at $-$ 20°C. The Elvax was then sectionedinto 180-µm-thick disks by cryostat and stored at $-$ 80°C. Beforesurgeries, the Elvax was washed in 70% ethanol for 30 min andtwice in sterile PBS for 30 min. For younger animals, the Elvaxwas cut into ~2 × 0.75 mm strips. For older animals, the Elvaxstrips were ~4 × 1 mm. The strips were carefully inserted intothe vitreous after making a small incision at the edge of thesclera. One eye in each animal was treated with either TTX orcitrate Elvax; the other eye remained intact. Anesthesia was maintainedby halothane/O₂ via mask. After Elvax implantation, the rats recoveredfrom anesthesia under observation. The effectiveness of activityblockade was monitored daily by assaying for consensual pupilresponse to bright white illumination under light halothane/O₂anesthesia.

MD by eyelid suture was initiated at P18, P25, P32, P39, and P53 (for each time point, n = 3). Under ketamine/xylazine (80/10mg/kg) anesthesia, the area surrounding the left eye was cleanedwith povidone-iodine and isopropyl alcohol. The lid margins weretrimmed and the eye was flushed with sterile PBS. Two to threehorizontal mattress sutures using 6.0 Ethilon (Johnson & Johnson,Somerville, NJ) closed the length of the apposed lids. Ophthalmicointment (Fougera, Melville, NY) was applied and the animals weremonitored for recovery. For the P14 time point (n = 3), ratherthan suture the unopened eye, tissue adhesive (Vetbond; 3M, St.Paul, MN) was applied at P11 to prevent possible eye opening.After 3 d of TTX blockade or MD, animals were decapitated by guillotine;the brains were removed immediately and trimmed and positionedfor coronal sectioning before being frozen on powdered dry iceand stored at $-$ 80°C.

In situ hybridization. Coronal sections (10 µm) through the anterior visual cortex were sectioned by cryostat, thaw-mountedon Superfrost/plus microscope slides (VWR Scientific, West Chester,PA), dried, fixed in 4% paraformaldehyde, washed in PBS, dehydratedin ethanol, air-dried, and stored desiccated at $-$ 80°C. Beforehybridization, slides were pretreated (at room temperature, unlessotherwise stated) with 0.2 M HCl (20 min), double distilled water(DDW) (5 min), 2× SSC (30 min at 70°C), and DDW (5 min). The nextprehybridization treatments, from pronase (type XIV) (Sigma) toair-drying slides for 1 hr, were conducted as described previously(Hogan et al., 1994). RNA probes were synthesized with an RNAtranscription kit (Stratagene, La Jolla, CA) and ³⁵S-UTP (800 Ci/mmol; Amersham Biosciences, Piscataway, NJ), usinglinearized cpg15 cDNA as a template. Hybridizations were doneas described previously (Nedivi et al., 1996). Posthybridizationwash conditions were as follows: 3 hr at 50°C in 50% formamideand 1× salt solution (Hogan et al., 1994) with 10 mM DTT; 15 minat 37°C in TNE (10 mM Tris, pH 7.5, 0.5 M NaCl, 1 mM EDTA); 30min at 37°C in TNE containing RNase A (20 µg/ml; Sigma); 30 minat 37°C in TNE; and finally overnight at 50°C in 50% formamideand 1× salt solution. Slides were dehydrated with 0.3 M NH₄Acin ethanol, air-dried, and processed for autoradiography as describedpreviously (Hogan et al., 1994), using autoradiographic emulsiontype NTB-2 (Eastman Kodak) diluted 1:1 with 2% glycerol, and exposedfor 3-5 d at 4°C.

Quantitative data analysis. Dark-field images of two to four sections from each brain were imported into Adobe Photoshop 5.0(Adobe Systems, San Jose, CA) with a Diagnostic Instruments (SterlingHeights, MI) Spot2 digital camera mounted on a Nikon (Tokyo, Japan)Eclipse E600 using a 1×/0.04 Plan ultrawide objective. Imageswere saved as gray-scale TIFFs and imported into NIH Image (version1.62). In addition to the VC and the superior colliculus (SC),each section contained the medial geniculate body (MGB) of thethalamus, an auditory sensory area (Fig. 1). Areas were definedby Nissl staining of alternate sections. Mean pixel density measurementswere taken from four areas on each section: the VC, the SC, thebackground, and the MGB. Pixel density was measured on a 0-255scale, on which 255 is white. The background served as a zero-labelingnegative control, whereas the MGB served as a positive controlwith a high level of labeling that is unaffected by visual manipulations.VC and SC measurements were normalized on a scale of 0-1 interpolatingbetween the background (0) and MGB (1) values. The backgroundmean pixel density was first subtracted from the mean pixel densitiesin the VC, the SC, and the MGB, yielding the net mean pixel densitiesfor each area. The net mean pixel density in the VC or SC wasthen divided by the net mean pixel density from the MGB in thesame section. Statistical significance was determined by unpairedStudent's t test. To confirm that measurements were unbiased,image files from four groups (4 week and 8 week controls, and4 week and 8 week DR) were coded, mixed, and remeasured by technicianswho were unaware of the experimental treatment. All data setswere not significantly different between blind and nonblind measurements.

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Figure 1. In situ hybridization on a coronal section through rat visual cortex using a cpg15 probe. The regions relevant for quantification are outlined. Mean pixel densities were measured in four areas on each section: the VC, the SC, the MGB, and an area of the section with zero labeling for background (BG). The background is used as the zero point, whereas the MGB served as a positive control with a high level of labeling that is unaffected by visual manipulations (see Materials and Methods).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Developmental profile of cpg15 expression

To investigate a role for cpg15 in the activity-dependent phase of the development of the rat visual system, in situ hybridizationswith a cpg15 probe were conducted on sections through visual structuresstarting at P10. The lateral geniculate nucleus (LGN), SC, andVC were monitored before and after eye opening, throughout thecritical period for development of eye-specific preference inthe binocular zone of primary VC, and in the adult. At birth andup to P10, expression of cpg15 is undetectable in the neocortex(Nedivi et al., 1996). At P10, 4 d before eye opening, low levelsof cpg15 mRNA were visible at the apex of the cortical hemispheres(Fig. 2). General onset of cpg15 expression in the VC occurredcoincident with eye opening at 2 weeks after birth, with the highestexpression in layers 2/3, 4, and 6. Subsequently, cpg15 mRNA expressionlevels gradually increased, peaking at P28, the height of thephysiologically characterized critical period for the developmentof eye-specific preference in the VC. cpg15 mRNA levels then declinedto a lower basal adult level. These results show that cpg15 levelsin the rat VC correspond well with the electrophysiologicallymapped critical period.

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Figure 2. Developmental time course of cpg15 expression in the VC of normal and DR rats. Representative dark-field photomicrographs of in situ hybridizations for cpg15 mRNA are shown. Coronal sections through the VC of normal animals (left) and dark-reared animals (right) are shown at the designated postnatal ages. The onset of cpg15 expression in the neocortex for both normal and DR animals is coincident with eye opening at 2 weeks of age. Normally, cpg15 expression peaks at 4 weeks and then declines to a lower basal adult level. In DR animals, cpg15 levels remain elevated past 5 weeks. Arrowheads point to the earliest cpg15 expression at the medial apex of the neocortex. Some individual panels (untreated, 6 weeks; DR, 6 weeks; untreated, 4 weeks; DR, 4 weeks; DR, 3 weeks; and DR, 2 weeks) were normalized with respect to the MGB for assembly of the montage. Scale bar, 1 mm.

Effect of dark rearing on cpg15 expression

To test whether regulation of cpg15 expression was sensitive to visual input, rats were deprived of visual experience by darkrearing to various developmental ages. cpg15 mRNA levels werecompared in DR animals and age-matched controls. Dark rearingdid not alter the time of onset or the early increase in levelsof cpg15 expression in the VC (Fig. 2). At P28, cpg15 mRNA levelsin DR animals plateaued, but at a significantly lower level ofexpression than in age-matched controls (Figs. 2 and 3a). Thislevel of expression persisted in older DR animals, so that after8 weeks of dark rearing, cpg15 expression levels were significantlyhigher than in their age-matched controls, in which cpg15 expressionnormally declined after P28 (Figs. 2 and 3a). Differences in cpg15mRNA levels between normal and DR animals were not seen in theLGN or SC (data not shown). The enhanced expression levels ofcpg15 in the VC, seen with dark rearing, may be a molecular indicatorof the prolonged plasticity specific to this region.

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Figure 3. Quantification of cpg15 expression in the VC of control (normal) rats, DR rats, rats after blockade of retinal activity, or rats after MD. In all cases, after background subtraction, the net average pixel value in the VC was normalized by the net average pixel value of the MGB (see Materials and Methods for details). a, Effect of dark rearing on cpg15 expression in the VC. Data from four in situ experiments are shown, of which Figure 2 is representative. Solid circles, DR animals; open circles, untreated control animals. Error bars indicate the SEM. Points marked with asterisks are significantly different between normal and DR animals (at 4 weeks, p = 0.001; at 8 weeks, p = 0.016; unpaired Student's t test). b, Effect on cpg15 expression in the VC of monocular TTX blockade for 3 d initiated at different developmental times. Data from three in situ experiments are shown, of which Figure 5 is representative. Solid circles, VC contralateral to TTX blockade; open circles, VC of control animals implanted with a citrate control in the contralateral eye. Error bars indicate the SEM. Points marked with asterisks are significantly different between the VC of control and TTX-treated rats (at 5 weeks, p = 0.0012; at 6 weeks, p = 0.032; at 8 weeks, p = 0.0008; unpaired Student's t test). c, Effect on cpg15 expression in the VC of MD for 3 d by eyelid suture initiated at different developmental time points. Solid circles, VC contralateral to the sutured eye; open circles, VC of untreated control animals. Error bars indicate the SEM. Points marked with asterisks are significantly different between the VC of control and MD rats (at 4 weeks, p = 0.003; at 5 weeks, p = 0.006; at 6 weeks, p = 0.007; unpaired Student's t test).

Reportedly, a short exposure to light can trigger the end of the delayed plasticity seen in DR animals (Mower et al., 1983;Philpot et al., 2001). To test whether a late onset of visualexperience affects cpg15 expression, animals were dark-rearedto 8 weeks and then exposed to light for 6, 12, or 24 hr or for7 or 14 d. In situ hybridizations show that with exposure to lightof up to 12 hr, cpg15 expression remains significantly higherthan normal (Fig. 4). After 24 hr of exposure to light, DR animalsshowed cpg15 mRNA expression levels that were comparable withthose found in normally raised adults (Fig. 4). These experimentsindicate that brief visual experience in DR adults can reset cpg15expression to normal levels. This downregulation of expressionmay be a molecular representation of the light-induced end ofthe delayed plasticity in DR animals.

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Figure 4. Light triggers downregulation of cpg15 expression in DR rats. Quantification of cpg15 expression in the VC of animals DR to 8 weeks and subsequently exposed to light (LT) for designated times. Data from two in situ experiments are shown. In each section, the net average pixel value in the VC is normalized by the net average pixel value of the MGB. Abnormally high levels of cpg15 expression in animals dark-reared to 8 weeks decline to normal adult levels within 24 hr of exposure to light. Error bars indicate the SEM. Asterisks mark significant differences compared with normal animals at 8 weeks (DR, 8 weeks, p = 0.016; DR, 8 weeks plus 6 hr of light, p = 0.009; DR, 8 weeks plus 12 hr of light, p = 0.0086; unpaired Student's t test).

Effect of blockade of retinal action potentials on cpg15 expression

To investigate whether cpg15 mRNA expression in the VC is dependent on retinally driven action potential activity, the Na⁺ channel blocker TTX was applied to the left retina of normallyraised rats for 3 d periods, starting at different developmentaltimes. Age-matched control animals were treated with citrate bufferapplied to the left retina. cpg15 mRNA levels in the VC contralateralto the TTX-treated eye were compared with those in the VC contralateralto the citrate-treated eye in control animals. There was no changein the onset of cpg15 expression in response to monocular retinalactivity blockade, and there was no significant influence on corticallevels of cpg15 mRNA during early postnatal development (Fig.5). Mean levels of cpg15 expression at 2, 3, and 4 weeks afterbirth were not significantly different between the VC contralateralto the blocked eye and the VC contralateral to the citrate-treatedcontrols (Fig. 3b). In contrast, after the peak of the criticalperiod and into adulthood, monocular retinal action potentialblockade decreased cpg15 expression in the VC contralateral tothe blocked eye (Figs. 3b and 5).

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Figure 5. cpg15 expression in the VC after 3 d of monocular TTX blockade initiated at different developmental times. Dark-field photomicrographs of in situ hybridizations for cpg15 mRNA in coronal sections through the VC contralateral to the treated eye of either control animals (left) implanted with the citrate vehicle or TTX-treated animals (right), at the designated ages. Starting at 5 weeks after birth, retinal TTX blockade decreases levels of cpg15 expression in the VC (see cortical area between arrowheads). Starting at 4 weeks after birth, retinal TTX blockade causes a downregulation of cpg15 expression in the SC (SC indicated by two arrows). Some individual panels (citrate, 4 weeks; TTX, 4 weeks; TTX, 3 weeks) in this figure were normalized with respect to the MGB for assembly of the montage. Scale bar, 1 mm.

Monocular TTX blockade also decreased cpg15 expression in the contralateral LGN and SC starting 3 weeks after birth. For boththe LGN and superficial layers of the SC contralateral to thetreated eye, the effect of TTX blockade became more pronouncedwith age (LGN not shown; for SC, see Figs. 5 and 6). These experimentsindicate that in all of the visual structures tested, the developmentalregulation of cpg15 expression is divided into two phases. Earlycpg15 expression is independent of retinally driven action potentials.During the critical period for development of eye-specific preferencein the VC, an activity-dependent component of cpg15 expressionemerges, and the effect of retinal action potential blockade becomesprogressively more pronounced with age.

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Figure 6. Quantification of cpg15 expression in the SC after 3 d of monocular TTX blockade initiated at different developmental times. Data from three in situ experiments are shown, of which Figure 5 is representative. After background subtraction, the net average pixel value in superficial layers of the SC was normalized by the net average pixel value of the MGB. cpg15 expression in the SC is depressed by retinal TTX blockade soon after eye opening. Solid circles, SC contralateral to TTX blockade; open circles, SC contralateral to citrate control. Error bars indicate SEM. Points marked with asterisks are significantly different between the SC of control and TTX-treated rats (at 4 weeks, p = 0.026; at 5 weeks, p = 0.0003; at 6 weeks, p = 0.027; at 8 weeks, p = 0.011; unpaired Student's t test).

Effect of monocular deprivation on cpg15 expression

It has been shown that total blockade of retinal activity produces a smaller shift in ocular dominance plasticity than thatproduced by MD (Rittenhouse et al., 1999). To investigate whetherthe effect of monocular activity blockade on cpg15 expressionis less extreme than that of MD, we monocularly deprived normallyraised rats for 3 d periods, starting at different developmentaltimes. cpg15 levels in the VC and the SC contralateral to thesutured eye were compared with the VC and the SC in normal animals.As in both DR and TTX-treated animals, there was no change inthe onset of cpg15 expression in the VC of MD rats (Fig. 3c).During the next 4 weeks of development, cpg15 expression in theVC contralateral to the MD eye was significantly less than innormal animals. Unlike animals whose retinally driven action potentialsare blocked by TTX, at the peak of the critical period (P28) MDanimals exhibit levels of cpg15 expression that are significantlyless than those of controls. With maturation, the effect of MDbecomes less significant, and at 8 weeks after birth, cpg15 expressionin the deprived VC is no longer different from controls. Thistrend is opposite to the effect of TTX, which becomes more significantas the animals mature. As in DR animals and in contrast to animalswith retinal activity blockade, monocular deprivation did notaffect cpg15 levels in the contralateralSC.

Effect of early visual experience on adult cpg15 expression

Previous studies suggest that early periods of visual experience are sufficient to trigger closure of the critical perioddespite later visual deprivation (Mower et al., 1983; Mower andChristen, 1985). To determine the window of early visual experiencerequired for the development of normal adult regulation of cpg15expression in the VC, animals were raised in a normal 12 hr light/darkcycle to 2, 3, 4, or 5 weeks after birth and then transferredto a dark environment until adulthood at 8 weeks. Animals werekilled without seeing any additional light or after 24 hr of re-exposureto light, to assess their ability to regulate cpg15 expression.In normally raised adult rats, cpg15 mRNA expression in the VCis downregulated after a 2 week period in the dark. After re-exposureto light for 24 hr, such dark-adapted rats will upregulate cpg15levels (Nedivi et al., 1996) (Figs. 7h and 8h). In contrast, ratsraised in darkness to 8 weeks show abnormally high levels of cpg15expression in the VC; after exposure to 24 hr of light, the levelsof expression are decreased (Figs. 4, 7a, and 8a). These two extremeswere compared with animals exposed to visual experience at restrictedwindows during development. Animals exposed to visual experiencefor 2 or 3 weeks before being placed in the dark until they hadreached adulthood displayed a regulation of cpg15 expression thatwas essentially the same as that seen in DR animals (Figs. 7b,c,and 8b,c). Animals reared with normal visual experience for thefirst 4 or 5 weeks after birth and then placed in darkness until8 weeks of age regulate cpg15 expression in the VC similarly tonormal animals (Figs. 7d,e and 8d,e). These results suggest that1 week of visual experience at the outset of the critical periodis sufficient to confer normal patterns of adult cpg15 regulation.To test this prediction, animals were raised to 8 weeks in darknessexcept for 1 week of light either between weeks 3 and 4 or betweenweeks 4 and 5. cpg15 expression in the VC was assayed at 8 weeks.cpg15 mRNA levels in animals allowed just 1 week of visual experienceduring the critical period are strikingly similar to those seenin normally raised animals and are dramatically induced on re-exposureto light for 24 hr (Fig. 8f,g). Our results show that a restricted1 week window of visual experience during the critical periodis sufficient to determine adult patterns of cpg15 regulationin the VC.

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Figure 7. Early visual experience confers normal adult patterns of cpg15 regulation. Representative dark-field photomicrographs of in situ hybridizations for cpg15 mRNA on coronal sections through the VC are shown. Animals were raised to different ages with normal visual experience and then transferred into a dark environment until 8 weeks of age (left), followed by a 24 hr re-exposure to light (right). Animals raised normally to 4 or 5 weeks of age (d, e) and then dark-reared to 8 weeks show the normal decline in cpg15 levels with maturation as well as the normal adult regulation (h) of cpg15 expression by light (arrowheads delineate the VC). Similar to DR animals from birth (a), animals raised normally to 2 and 3 weeks of age (b, c) and then dark-reared to 8 weeks fail to downregulate cpg15 as adults and do not reinduce cpg15 in response to light. Panels were not normalized for montage assembly. Scale bar, 1 mm.

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Figure 8. One week of visual experience during the critical period is sufficient to confer the normal adult patterns of cpg15 regulation. Quantification of cpg15 expression in the VC of rats with early visual experience. Measurements and calculations were done as described in Figure 3. The treatment legend is identical to Figure 7. A 1 week window of light during the critical period, either between weeks 3 and 4 (f) or weeks 4 and 5 (g), confers normal adult patterns of cpg15 regulation. Gray bars, cpg15 expression levels without re-exposure to light; black bars, levels after 24 hr of light exposure. Error bars indicate the SEM. Points marked with asterisks are significantly different between animals killed in the dark or after 24 hr of light exposure (e, h, p < 0.0001; f, p = 0.0049; g, p = 0.0022; d, p = 0.009; unpaired Student's t test).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The experiments described here address the temporal and spatial expression patterns of cpg15 in the developing visual systemof the normal rat and in response to visual manipulations. cpg15expression was monitored in relation to the critical period fordevelopment of eye-specific preference in the VC. We comparedexpression during normal development with that seen in responseto dark rearing, monocular retinal action potential blockade,or MD. The regulation of cpg15 expression patterns suggests thatit may serve as a molecular indicator of the potential for visualsystemplasticity.

Activity-independent and activity-dependent phases of cpg15 expression

We found that in the visual system of rats, the onset of cpg15 mRNA expression in the VC occurs 2 weeks after birth. cpg15expression levels gradually rise and peak 2 weeks later, in themidst of the electrophysiologically mapped cortical critical periodfor shifts in eye preference. After its peak expression, cpg15mRNA levels in the VC decline to a lower basal level in adults,concomitant with critical period closure at ~6 weeks of age (Fagioliniet al., 1994; Gordon and Stryker, 1996). Although the onset ofcpg15 expression is coincident with eye opening, it is unaffectedby dark rearing, blockade of retinally driven action potentials,or MD. This is consistent with previous studies of cpg15 expressionin the visual system of cats, which demonstrated that early cpg15expression in the VC is activity independent (Corriveau et al.,1999). Therefore, the initial timing of cpg15 expression is likelyto be controlled by a developmentally regulated activity-independentmechanism. This fits with electrophysiological and optical imagingstudies that demonstrate that the basic structure of corticalmaps is innate and develops in the absence of visual experience(Crair et al., 1998).

These studies also show that experience is necessary at a later stage of development for the refinement of ocular selectivityand to maintain responsiveness (Crair et al., 1998). We find thatafter the peak of the critical period, as the levels of cpg15in the VC begin to decline, a component of cpg15 expression thatis dependent on retinally driven action potentials becomes evidentand is progressively more pronounced with age. Activity-dependentregulation of cpg15 expression in the SC and the LGN can be detected1 week earlier than in the VC, perhaps because of the earliermaturation of these visual structures. Our results indicate thatthe regulation of cpg15 expression is biphasic in all visual structures.Early cpg15 expression is independent of retinally driven actionpotentials. With maturation during the critical period, an activity-dependentcomponent of cpg15 expression emerges, and the effect of the blockadeof retinally driven action potentials becomes progressively morepronounced with age. Activity-dependent regulation of cpg15 arisesrelatively late in development and may represent an adult featureof visual systemplasticity.

Effect of visual experience on cpg15 expression

The aspects of cpg15 regulation that we found to be dependent on normal visual experience were its peak levels in the VC atP28 and its subsequent downregulation after the end of the criticalperiod. Although cpg15 levels in the VC of DR rats are indistinguishablefrom those in control rats within the first 3 weeks after birth,the expression at P28 is lower than in controls. Rats DR beyondP28 maintain the same peak level of cpg15 expression through adulthood,levels that are significantly higher than in their control counterparts.There is a crossover of the cpg15 expression profiles in normaland DR rats, such that at the peak of the critical period expressionis higher in normal animals, whereas after the critical periodcpg15 is higher in DR animals. This crossover can also be seenin the developmental profiles of susceptibility to MD in normaland DR cats (Mower, 1991). In rodents, there have been no studiesthat examine the effects of dark rearing on susceptibility toMD during the height of the critical period. Studies at laterages show that similar to cats, DR rats also retain a prolongedcapability to respond to MD, even at P90 (Guire et al., 1999).

With respect to dark rearing, we show here two additional cases in which cpg15 regulation closely parallels plasticity asmeasured by susceptibility to MD. Electrophysiological studieshave demonstrated that a short exposure to light can trigger theend of the delayed plasticity that results from dark rearing (Moweret al., 1983; Philpot et al., 2001). Similarly, early visual experiencein DR kittens attenuates the effects of later dark rearing sothat there is no delayed plasticity (Cynader, 1983). These resultsshow that the effect of dark rearing can be negated by a shortperiod of light exposure in DR adults, or with sufficient earlyvisual experience. We find that a 24 hr exposure to light returnscpg15 levels in DR rats to those found in normally raised adults,and that 1 week of visual experience during the critical periodis sufficient to confer normal adult patterns of cpg15regulation.

Our results show that even 1 week of visual experience during the critical period is sufficient for establishing adult patternsof cpg15 regulation. This suggests that visual experience is notpersistently required during development for normal functionalmaturation of the visual system to occur. Rather, exposure topatterned vision for at least 1 week during the critical periodcan irreversibly trigger the molecular machinery that is requiredfor maturation; this will likely result in normal adult responsesto visual manipulations. Because cpg15 expression is abnormallyhigh in the adult in the absence of visual experience, the moleculartrigger for maturation may involve a general downregulation ofplasticity genes such as cpg15.

Differences in the effect of DR on cpg15 from effects of activity blockade and MD

The effect on cpg15 expression of binocular elimination of patterned vision during the critical period is profoundly differentfrom the effect of retinal action potential blockade or MD. Darkrearing causes a prolonged upregulation of cpg15 expression startingat the peak of the critical period and continuing into adulthood,whereas retinal action potential blockade at the same developmentaltimes causes a decrease in cpg15 expression. The effect of darkrearing is exclusive to the VC, whereas blockade of retinallydriven action potentials affects cpg15 expression in the LGN andthe SC as well as in the VC. This result corresponds well withthe observation that the delayed plasticity seen in DR cats isnot manifested in the LGN (Mower et al., 1985; Mower and Christen,1985).

During the critical period, downregulation of cpg15 expression in the VC by MD is more severe than that caused by retinalactivity blockade. This is consistent with electrophysiologicalstudies that show that MD during the critical period producesa greater shift of ocular dominance in the VC than monocular blockadeof retinal activity (Rittenhouse et al., 1999). A possible explanationis that during MD the residual activity from the retina activelydepresses the efficacy of synaptic connections driven by the deprivedeye (Bear and Rittenhouse, 1999; Rittenhouse et al., 1999). Despitethe fact that an MD eye is generating some activity as opposedto the total loss of activity caused by the blockade of retinallydriven action potentials, during the critical period cpg15 levelsare lower in the VC of MD animals than in animals after retinalTTX blockade. This could reflect the depression of cortical synapticactivity driven by the deprivedeye.

Taken together, all of this indicates that regulation of cpg15 expression does not correspond directly to levels of activity.Rather, it seems to reflect a propensity for functionalplasticity.

Effect of dark rearing on expression of visually responsive genes

It has been proposed that mechanisms that underlie adult plasticity during learning and memory, or long-term potentiationand long-term depression, also play a key role in developmentalplasticity (Kandel and O'Dell, 1992; Goodman and Shatz, 1993;Constantine-Paton and Cline, 1998; Nedivi, 1999). For this reason,many genes isolated or characterized on the basis of their responseto activity in the adult have been investigated in the contextof developmental plasticity in the visual system. These includeboth regulatory genes that encode transcription factors as wellas effector genes that can directly affect neuronal morphologyand function (for review, see Nedivi, 1999). Multiple genes showa transcriptional response to dark rearing, although the typeof response varies. Whereas growth-associated protein 43 (GAP43),calcium calmodulin-dependent kinase II (CaMKII), and glutamicacid decarboxylase (GAD) all show the same increase in expressionshown by cpg15 in response to dark rearing past the critical period(Neve and Bear, 1989), junB, zif/268, and BDNF show the oppositeresponse and are downregulated (Rosen et al., 1992; Lein and Shatz,2000). In contrast to the light-independent onset of cpg15 expression,dark rearing prevents the normal onset and transcriptional increaseof Homer, zif/268, and BDNF in the VC (Worley et al., 1990; Brakemanet al., 1997; Capsoni et al., 1999; Lein and Shatz, 2000). Subsequentexposure to light causes their rapid induction (Worley et al.,1990; Brakeman et al., 1997; Capsoni et al., 1999; Lein and Shatz,2000). The transcriptional regulation of this latter group providesan accurate "molecular readout" of activity, whereas regulationof cpg15 together with GAP43, CaMKII, and GAD corresponds moreclosely with the capacity forplasticity.

Summary

During the development of the Xenopus visual system, cpg15 concurrently regulates multiple aspects of retinotectal circuitformation (Cantallops et al., 2000). It promotes tectal cell dendriticarbor growth, stabilizes retinal axon arbors, and promotes maturationof retinotectal synapses (Nedivi et al., 1998; Cantallops et al.,2000). Our finding that DR rats fail to downregulate cpg15 raisesthe possibility that perhaps the residual plasticity measuredelectrophysiologically in these animals reflects an extended capacityfor local synaptic remodeling. The prolonged plasticity seen inDR animals may result from failure to downregulate genes suchas cpg15, which could promote structural remodeling and synapticmaturation.

  FOOTNOTES

Received May 14, 2001; revised Nov. 28, 2001; accepted Dec. 7, 2001.

This work was supported by grants from the National Eye Institute, the Ellison Medical Foundation, and the Alfred P. SloanFoundation (E.N.). We are grateful to members of the Nedivi laboratoryand to Drs. Hollis T. Cline, Martha Constantine-Paton, and RachelWong for critical review of this manuscript. We thank MatthewColonnese for help with Elvaxsurgeries.

Correspondence should be addressed to Elly Nedivi, Massachusetts Institute of Technology, E18-670, 50 Ames Street, Cambridge,MA 02139. E-mail: nedivi{at}mit.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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