Decoupling Eye-Specific Segregation from Lamination in the Lateral Geniculate Nucleus

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The Journal of Neuroscience, November 1, 2002, 22(21):9419-9429

Decoupling Eye-Specific Segregation from Lamination in the Lateral Geniculate Nucleus
Andrew D. Huberman¹, David Stellwagen², and Barbara Chapman¹
¹ Center for Neuroscience, University of California, Davis, California 95616, and ² Department of Psychiatry and Behavioral Sciences, Stanford University School of Medicine, Palo Alto, California 94304

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

To determine whether there is a critical period for development of eye-specific layers in the lateral geniculate nucleus (LGN),we prevented the normal segregation of retinogeniculate afferentsand then allowed an extended period of time for recovery. Afterrecovery, both anatomy and physiology revealed strictly nonoverlappingterritories of input from the two eyes. However, the normal stereotypedpattern of eye-specific afferent and cellular layers never developed.Instead, the eye-specific territories of afferent input emergedas variable and disorganized patches with no corresponding interlaminarspaces in the LGN. These findings reveal a critical period forcoordinating the development of three processes in the LGN: thesegregation of afferents from the two eyes, the spatial organizationof those afferents into layers, and the alignment of postsynapticcytoarchitecture with the afferent inputs. We also assessed thephysiological consequences of preventing normal lamination andfound normal single-cell responses and topographic representationof visual space in the LGN. Clusters of ON-center and OFF-centerLGN cells were segregated from one another as in normal animals.However, the organization of ON and OFF sublaminas in the treatedanimals wasdisrupted.

Key words: visual system; development; lateral geniculate nucleus; activity; lamination; eye-specific; critical period

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The adult LGN is characterized by its stereotyped organization into discrete eye-specific layers. These layers are evidentboth as nonoverlapping regions of afferents from the two eyesand as corresponding cellular laminas formed by LGN neurons (Jones,1985). The mechanisms underlying the development of the afferentand cellular LGN layers are not wellunderstood.

During normal development, the retinogeniculate afferents from the two eyes initially overlap before gradually segregatinginto eye-specific layers (Fig. 1A,B) (Linden et al., 1981; Cucchiaroand Guillery, 1984; Hutchins and Casagrande, 1990; Penn et al.,1998; Hahm et al., 1999). Previous experiments suggest that theformation of afferent layers in the LGN occurs via a competitionbetween the two eyes for postsynaptic space. If one eye is removedbefore eye-specific segregation, axons from the remaining eyeexpand into regions of the LGN normally occupied only by the othereye (Lund et al., 1973; Rakic, 1981; Guillery et al., 1985a; Sretavanand Shatz, 1986; Garraghty et al., 1988; Thompson et al., 1993).Furthermore, this competition between the two eyes in normal developmentis mediated by spontaneous retinal activity. If activity fromboth eyes is pharmacologically silenced, axons from the two eyesdo not segregate (Fig. 1C-E) (Shatz and Stryker, 1988; Penn etal., 1998; Rossi et al., 2001). If activity is silenced in oneeye, there is an expansion of the territory of the active untreatedeye at the expense of the projection from the inactive eye (Pennet al., 1998; Stellwagen and Shatz, 2002). Conversely, if thelevel of activity in one eye is elevated, there is an expansionof the territory of the more active eye at the expense of thenormally active untreated eye (Stellwagen and Shatz, 2002).

The formation of eye-specific cellular layers in the LGN is proposed to be driven by the retinal afferents themselves. Normally,the development of cellular layers occurs after afferents fromthe two eyes segregate (Linden et al., 1981; Cucchiaro and Guillery,1984; Hutchins and Casagrande, 1990). If the pattern of retinogeniculateafferents is abnormal, the cytoarchitecture of the LGN directlyreflects these abnormal inputs. For example, in monocularly orbinocularly enucleated animals (Brunso-Bechtold and Casagrande,1981; Rakic, 1981; Guillery et al., 1985a,b; Sretavan and Shatz,1986; Garraghty et al., 1988; Morgan and Thompson, 1993), eye-specificcellular laminas also do not develop. Moreover, in coat-colormutants, in which the density of the ipsilateral-eye projectionto the LGN is reduced, the cellular laminas mirror the abnormaltopography of the retinal projections (Guillery, 1969, 1971).

Our experiment was designed to further study the developmental interaction between afferents from the two eyes and betweenthese retinal afferents and the cytoarchitecture of the LGN. Specifically,we sought to determine the role of spontaneous retinal activityin these interactions and to look for a critical period for developmentof LGN lamination. To do so, we prevented the normal eye-specificsegregation of retinogeniculate inputs by silencing spontaneousretinal activity in both eyes and then allowed these animals anextended period of recovery, during which spontaneous retinalactivity returned to normal. We then assessed the effects of thismanipulation on the pattern of retinogeniculate inputs, the cytoarchitectureof the LGN, and the physiology of LGN neurons, including theirreceptive field properties and spatialorganization.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animals. Timed pregnant Fitch-coat ferrets were obtained from Marshall Farms (New Rose, NY). All experimental procedures wereperformed in accordance with approved animal use protocols atUniversity of California Davis. Postnatal day 0 (P0) correspondsto the day of birth. Animals in all treatment groups gained weightnormally throughout the course of the study (Chapman and Godecke,2000).

In vivo intravitreal application of epibatidine. Surgical and drug injection procedures were similar to those described previously(Penn et al., 1998; Chapman, 2000; Stellwagen and Shatz, 2002).Briefly, every 48 hr from P1 until P10, animals were anesthetizedwith inhalant isofluorane and 1-2 µl of epibatidine HCl (1 mMdissolved in sterile saline) (dose of 1 µl on P1, increased by0.25 µl for each subsequent injection; Sigma, St. Louis, MO),or an equivalent volume of control solution (sterile saline) wasinjected into the vitreous humor of each eye at a rate of 0.5µl/min using a 33 gauge needle attached to a Hamilton (Reno, NV)microsyringe.

Labeling of retinogeniculate afferents and cytoarchitecture in the LGN. Ferrets received intravitreal injections of choleratoxin- $beta$ subunit (CT $beta$ ) conjugated to fluorescein (green label)in the right eye and CT $beta$ conjugated to rhodamine (red label) intothe left eye (3-8 µl depending on the age of the animal; 0.5%in sterile saline; List Biochemical) (CT $beta$ has no biological activity).One day later, animals were transcardially perfused with 4% paraformaldehyde(ages in text correspond to age at which animals were killed),and tissue was postfixed overnight and sectioned at 50 µm. Afterimaging of retinal afferents (see below), LGN sections were dehydratedand stained with Thionin (0.45%) to revealcytoarchitecture.

Retinal histology. Retinal flatmounts were prepared by dissecting out the retina whole from the eyecup and placing four relievingcuts along the major axis, radial to the optic nerve. The entireretina was stained with 4',6'-diamidino-2-phenylindole (VectorLaboratories, Burlingame, CA) to reveal cell nuclei; CT $beta$ labelallowed identification of nuclei and, for ganglion cells, an axon.For retinal cross sections, eyes were hemisected, embedded, sectionedat 15 µm, and processed withThionin.

Image quantification. All images were digitally acquired with a CCD camera (SPOT Diagnostic); universal gains were establishedfor each label at a given magnification. Raw images of the LGNwere imported to PhotoShop (Adobe Systems, San Jose, CA) and croppedto exclude the optic tract and medial intralaminar nucleus. Imageswere then thresholded to 30% above background (designated as anonretinorecipient portion of the tissue slice 1 mm lateral tothe midline of the thalamus). The 30% value is based on previousstudies (Stellwagen and Shatz, 2002) and evaluation of signal:noisein tissue from animals of different ages. Thresholded images werethen set to black (<30% above threshold) or white (>30% abovethreshold). Measurements of the area of the LGN occupied by thecontralateral or ipsilateral eye projections were calculated byautomatically selecting all white pixels within the image frame(Scion Image; Scion Corp., Frederick, MD). Measurements of overlapwere calculated by multiplying the thresholded image of the contralateraleye inputs to the LGN with the thresholded image of the ipsilateraleye inputs to the same LGN. In the resulting image, white pixelsthus correspond only to locations at which the contralateral andipsilateral afferents were both present; overlap area was calculatedby automatically selecting all of the white pixels within theimage frame (Scion Image). To quantify the extent of the ipsilateralprojection to the LGN, the boundary of the total ipsilateral projection(including A, A1, and C laminas in normal animals and all ipsilateraleye label in epibatidine-recovery animals) was delineated by connectingthe edges of the outermost ipsilateral projections with straightlines; then the total area contained within the resulting polygonwas divided by the total area of the LGN in that section. Threeto six sections through the middle 200-300 µm portion of the LGNwere analyzed for each animal (depending on the age of the animal).LGNs from animals in which retinal ganglion cell or retinogeniculatelabeling appeared incomplete were excluded from allanalyses.

Measurements of both total cell and ganglion cell density were performed from matched locations in the central and peripheralretina for all four retinal quadrants. Morphological criteriadescribed previously were used to identify different cell types(Henderson et al., 1988; Stellwagen and Shatz, 2002). Quantificationwas limited to retinas P25 and older (P25+) (after ganglion cellgenesis and apoptosis in the ferret retina is complete) (Hendersonet al., 1988; Reese et al., 1994; Cusato et al., 2001). The entireretinas from ferrets of all ages were carefully inspected fordamage.

Preparation of photomicrographs. Images were imported to PhotoShop (Adobe Systems) for cropping, resizing, and alignment.In some cases, artifact was removed from outside the boundariesof theLGN.

Imaging of spontaneous retinal activity. Imaging of spontaneous retinal activity was performed according to protocols describedpreviously (Feller et al., 1996; Penn et al., 1998; Stellwagenet al., 1999; Wong et al., 2000; Stellwagen and Shatz, 2002).Ferrets were deeply anesthetized with halothane and then decapitated.Retinas were then rapidly dissected from the eye and incubatedin 10 µM fura-2 AM (Molecular Probes, Eugene, OR) in artificialCSF [ACSF (in mM): 119 NaCl, 2.5 KCl, 1.3 MgCl₂, 1 KH₂PO₄, 2.5CaCl₂, 26.2 NaHCO₃, and 11 D-glucose] containing 1% DMSO and 0.02%pluronic acid for 4-8 hr in an oxygenated chamber at 28°. Opticalrecording was performed on an inverted microscope (Diapshot 300;Nikon, Tokyo, Japan) using a 5× objective (to assess activityacross an entire quadrant of the retina) or 40× objective (toassess correlations between individual neighboring cells; averageof 20 cells per field). Retinas were perfused continuously with32° ACSF throughout the imaging session. In some cases, retinaswere perfused with 100 nM epibatidine (in ACSF) during the imagingsession. Images were acquired with a pentamax cooled CCD camera(Princeton Instruments, Trenton, NJ), using Metamorph software(Universal Imaging, West Chester, PA). Difference images werecalculated from an initial background frame. Fluorescence dataare presented as $Delta$ F/F versus time, where F is the amount of directcurrent fluorescence corrected for bleaching and $Delta$ F is the deviationfrom this baseline. Wave frequency was determined by dividingthe total number of $>=$ 1% $Delta$ F/F events/time. Wave domain sizes werecalculated by measuring the contiguous extent of an area wherea propagating >1% $Delta$ F/F eventoccurred.

Extracellular recordings of visual responses in the LGN. LGN recordings were performed using protocols described previously(Stryker and Zahs, 1983; Zahs and Stryker, 1985; Chapman, 2000;Chapman and Godecke, 2000). Ferrets were anesthetized using amixture of acepromazine (0.4 mg/kg) and ketamine (40 mg/kg, i.m.)and placed in a modified kitten stereotax. Animals were intubatedand anesthesia was maintained using 1-2% inhalant isoflurane inoxygen (volume and rate to maintained peak inspiratory pressureat 1.5 kPa and end-tidal carbon dioxide at 3.5-5%). End-tidalcarbon dioxide, core body temperature, and electrocardiogram weremonitored throughout the experiment. In cases in which retinotopywas mapped, animals were paralyzed with vecuronium bromide (0.2mg · kg¹ · hr¹, i.v.) and ventilated mechanically. A 4 × 4 mm craniotomy wasmade over the LGN, lacquered tungsten electrodes (Micro Probe,Potomac, MD) were advanced through the depth of the LGN usinga microdrive, and visual responses were recorded every 100 µm.To map retinotopy and the organization of ON- and OFF-center cells,LGN activity was assessed with an audio monitor and oscilloscope,and receptive fields were mapped onto a tangent screen using ahandheld light. Electrode penetrations were spaced in a 300 µmgrid across the rostrocaudal and mediolateral extent of the LGN.To obtain peristimulus time histograms (PSTHs) and receptive fieldmaps, visual stimuli were created using a VSG 2/5 visual stimulator(Cambridge Research Systems, Rochester, UK) and were displayedon a Sony monitor with a mean luminance of 40-50 candelas/m². Single units were discriminated, and spike times and waveformswere recorded using a Spike 2 system (Cambridge Electronic Design,Cambridge, UK). Receptive field maps were calculated by reversecorrelation from responses to white noise (m-sequence) stimuli(Reid et al., 1997). The white noise stimulus consisted of a 25× 25 grid of squares that were white or black 50% of the time,as determined by an m-sequence of length 2¹⁵-1. The stimulus was updated every 7.14 msec. PSTHs show averagedresponses from 40 presentations of an alternating black/whitedisk on a neutral graybackground.

At the end of the experiment, animals were injected intraocularly with anterograde tracers to visualize retinogeniculate afferents(see above); the animals were killed 24 hr later, and LGN andretinal tissue was harvested for anatomical assessment of theepibatidine treatment (see above) and reconstruction of the electrodetracks. Recording positions along electrode tracks were reconstructedby matching the locations where visually responsive neurons werefirst and last encountered with the dorsal and ventral anatomicalborders of LGN. Positions along the tracks were also verifiedby matching where the physiological responses changed from oneeye to the other, with the borders of eye-specific retinogeniculateCT $beta$ -fluorescein/rhodamine.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Activity blockade prevents segregation of eye-specific inputs to the LGN

In normal P1 ferrets (n = 6), ganglion cell axons from the two retinas overlap extensively (Fig. 1A) (Linden et al., 1981;Cucchiaro and Guillery, 1984; Hutchins and Casagrande, 1990; Pennet al., 1998; Hahm et al., 1999), with ~50% of the LGN receivinginputs from both eyes (Fig. 1C). By P10, axons from the two eyesare segregated (Fig. 1B) (Linden et al., 1981; Cucchiaro and Guillery,1984; Hutchins and Casagrande, 1990; Penn et al., 1998; Hahm etal., 1999; Chapman, 2000) with <1% of the LGN receiving overlappingcontralateral and ipsilateral retinal axons (Fig. 1C). The segregationof eye-specific inputs to the LGN can be prevented by silencingspontaneous retinal activity (Fig. 1C,E) (Penn et al., 1998; Rossiet al., 2001). In P1-P10 ferret retinas, spontaneous retinal activityis completely silenced by application of epibatidine (Fig. 1D)(Penn et al., 1998; Stellwagen et al., 1999). Immediately afterthe binocular epibatidine treatment from P1 to P10 (n = 6), inputsfrom the two eyes overlap throughout ~50% of the LGN (Fig. 1E,C),similar to the overlapping pattern seen in normal P1 ferrets (Fig.1A,C) and unlike the segregated pattern seen in control P10 ferrets(n = 3 untreated; n = 4 saline injected) (Fig. 1B,C). Two featuresunderlie the overlap seen in both normal P1 ferrets and P10 epibatidine-treatedferrets: the contralateral eye projects to the entire retinorecipientarea of the LGN (Fig. 1A,E, top panels), and the ipsilateral retinalprojection is significantly expanded (Fig. 1A,E, middle panels,C).

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Figure 1. Effect of epibatidine on spontaneous retinal activity and development of eye-specific segregation in the LGN. A, B, E, Contralateral (top panels) and ipsilateral (middle panels) retinal inputs to the LGN and their merged representation (bottom panels) from a normal P1 ferret (A), a normal P10 ferret (B) (arrows indicate lamina A, A1, and C), and a P10 ferret that received intravitreal injections of epibatidine every 48 hr from P1 to P10 (E). Tissue sections are in the horizontal plane; rostral is to the top, and medial is to the center of each panel. Scale bar: A, 50 µm; B, E, 75 µm. C, Percentage of LGN area occupied by overlapping projections from both eyes (overlap) or the ipsilateral eye on P1 (n = 6 LGNs) and P10 after normal/saline or epibatidine treatment (***p < 0.0001) (N.S., not significantly different) (overlap, p = 0.5; ipsilateral, p = 0.49; t test; n = 6 normal/6 saline, n = 12 epibatidine). PND, Postnatal day. D, Epibatidine abolishes early spontaneous retinal activity. Top trace, Normal P5 ferret retina showing spontaneous periodic increases in intracellular Ca²⁺ (downward deflections); bottom trace, P5 ferret retina showing one initial Ca²⁺ wave and then complete, sustained elimination of wave activity after application of 100 nM epibatidine (arrow).

Recovery restores eye-specific segregation but not afferent lamination

To determine whether there is a critical period for the development of the normal pattern of eye-specific inputs to the LGN,a group of ferrets received binocular intravitreal injectionsof epibatidine every 48 hr from P1 to P10 (n = 15) but were thenallowed to survive until P25 (n = 8), P36 (n = 4), or P65-P100(n = 3), at which time retinogeniculate afferents were visualized.In control ferrets P25 and older (P25+) that received either notreatment (n = 6) or binocular intravitreal injections of salinefrom P1 to P10 (n = 8), retinogeniculate afferents are completelysegregated into eye-specific A and A1 laminas (overlap area of<1%; n = 22 LGNs) as well as into ON and OFF sublaminas (see Figs.2A, 4B,C) (Linden et al., 1981; Stryker and Zahs, 1983; Cucchiaroand Guillery, 1984; Zahs and Stryker, 1985; Hutchins and Casagrande,1990; Hahm et al., 1999). The pattern of retinal inputs to theLGN of the epibatidine-treated animals that were allowed to recoveruntil P25+ (hereafter referred to as epibatidine-recovery animals)is dramatically different (compare Figs. 2A, 4B,C with Figs. 2B,4F,G,J,K,N,O). Although inputs from the two eyes achieved normallevels of segregation in these animals (overlap area of <1%; n= 26 LGNs; p = 0.48 recovery animals vs controls), the patternof eye-specific inputs is highly aberrant, with multiple ipsilateralprojections of various shapes, positions, and sizes distributedover a significantly greater-than-normal extent of the LGN (Fig.2C). These abnormal projections often extend into the region ofthe nucleus normally occupied only by afferents from the contralateraleye (compare Fig. 2A with 2B and Fig. 4B,C with 4F,G,J,K,N,O)and can even be displaced to the medial border of the nucleus(Fig. 2B, arrows in middle and bottom panels).

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Figure 2. Intravitreal epibatidine from P1 to P10, followed by recovery, disrupts normal patterning of eye-specific laminas in the LGN. A, B, Contralateral (top panels) and ipsilateral (middle panels) retinal inputs to the LGN and their merged representation (bottom panels) from a P25 ferret treated with saline from P1 to P10 (A) [arrows indicate ON and OFF sublaminas of laminas A (A_on, A_off) and A1 (A1_on, A1_off); C laminas are also seen] and a P25 ferret injected with epibatidine from P1 to P10 (B) (arrows indicate afferents from the ipsilateral retina that extend to ectopic locations along the medial border of the LGN). Tissue sections are in the horizontal plane; rostral is to the top, and medial is to the center of each panel. Scale bar, 100 µm. C, Quantification of the extent of ipsilateral retinal afferents across the LGN in the two treatment groups (***p < 0.0001) (t test; n = 11 controls; n = 13 epibatidine). D, Quantification of the LGN area occupied by ipsilateral retinal afferents in the two treatment groups (*p < 0.05; **p < 0.01) (t test; n = 11 control LGNs; n = 13 epibatidine). PND, Postnatal day.

Discontinuities in the contralateral-eye and ipsilateral-eye layers have been shown previously to accompany reductions inthe density of the ipsilateral retinogeniculate projection incoat-color mutants (Guillery, 1969, 1971). However, a simple reductionin the ipsilateral projection cannot explain the multiple eye-specificpatches seen in the epibatidine-recovery animals, because thearea of the LGN occupied by the ipsilateral projections is notreduced but is in fact slightly increased relative to controls(Fig. 2D).

Epibatidine treatment does not damage the retina, and spontaneous retinal activity re-emerges after the drug treatment

Damage to the developing retina caused by the drug or tracer injections cannot explain the abnormal pattern of afferents seenin the epibatidine-recovery animals. Total retinal area does notdiffer between the treatment groups, and cell density is normalacross all four quadrants of the treated retinas (total cell density,100 ± 1.4% of controls; ganglion cell density, 100 ± 1.8% of controls;n = 8 controls and n = 8 epibatidine-treated retinas). The thicknessof the nuclear and synaptic layers of the retina is also normalin the treated group (Fig. 3A,B). In addition, there are no ectopicpatches in the retinogeniculate projection of the treated animalsat P10 (Fig. 1E) or regions devoid of retinogeniculate afferentsat any age after the drug treatment (Figs. 1E, 2B, 4F,G,J,K,N,O),either or both of which would be expected if lesions of the earlypostnatal retina had occurred (Jeffrey, 1985; Hanson and Reese,1993). Deliberate needle-induced lesions to the retina performedon P4 or P34, followed by subsequent labeling of retinal ganglioncells on P36, confirm that after both long and short survivalperiods, needle-induced damage to the early postnatal ferret retinais easily detected (Fig. 3C,D). No such damage was evident inany of the animals included in this study.

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Figure 3. Epibatidine injections from P1 to P10 do not disrupt the structural integrity of the retina or the patterns of spontaneous retinal activity that re-emerge after treatment. A, B, Cross sections of the retina from a normal P36 ferret (A) and a P36 ferret that was treated with epibatidine from P1 to P10 (B). Scale bar, 50 µm. C, D, Low-magnification view of the ventral retina from a P36 ferret that was treated with epibatidine from P1 to P10 (C) and a P36 animal that received a needle-induced lesion to the retina on P4 (D) (arrow indicates site of degeneration in the ganglion cell layer). CT $beta$ -rhodamine label of cell bodies is shown. Scale bar, 250 µm. E, Quantification of the frequency of retinal waves present in normal and epibatidine-treated retinas on P10-P12 (N.S., not significant; p = 0.69) (t test; n = 12 controls, n = 9 treated retinas). PND, Postnatal day. F, Examples of spontaneous retinal activity recorded from a normal (top trace) and epibatidine-treated (bottom trace) P10-P12 retina; values for each trace represent an area of the ganglion cell layer encompassing ~20 cells.

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Figure 4. Relationship between afferent projection patterns and cytoarchitecture in epibatidine-recovery animals. A-D, Bilateral representation of cytoarchitecture (A, D) and retinal afferents (B, C) to the LGN of a saline-treated P25 ferret; lamina A and A1 and their respective ON (A_on, A1_on) and OFF (A_off, A1_off) sublaminas are clearly present from the pattern of both afferent and cytoarchitectural labeling (arrowheads indicate the border between layers A and A1, separated by an intralaminar space). E-P, LGNs of epibatidine-treated P25+ ferrets labeled to reveal cytoarchitecture (E, H, I, L, M, P) and retinogeniculate afferents (F, G, J, K, N, O). E, F, I, J, Adjacent sections (50 µm each) through the depth of the same LGN. M, N, O, P, Bilateral LGNs from the same animal; arrowheads in E and F indicate ectopic intralaminar spaces. Scale bar, 100 µm.

Because cholinergic agents fail to suppress spontaneous retinal activity in ferret retinas older than P12 (Wong et al., 2000),it is unlikely that residual blockade of spontaneous retinal activityafter cessation of the drug treatment could have contributed tothe abnormal pattern of afferents seen in the epibatidine-recoveryanimals. In fact, in ferrets that received binocular injectionsof epibatidine every 48 hr from P12 to P25, the LGN appeared normal(data not shown). However, to determine whether normal patternsof spontaneous retinal activity re-emerge after the epibatidinetreatment, and to further determine that the drug and/or injectionprocedure did not render portions of the retina dead or permanentlyinactive, we analyzed patterns of spontaneous retinal activity(Feller et al., 1996; Penn et al., 1998; Stellwagen et al., 1999;Wong et al., 2000; Stellwagen and Shatz, 2002) present in control(untreated, n = 8 retinas; saline, n = 9 retinas) or epibatidine-treated(n = 9 retinas) P10-P12 ferret retinas that received injectionsevery 48 hr from P1 to P10. Fluorescence imaging of intracellularCa²⁺ confirmed that by P10-P12, ganglion cells in the epibatidine-treatedretinas exhibited highly correlated, periodic bouts of spontaneousactivity with propagation patterns characteristic of normal P10-P12"retinal waves." Low-magnification imaging across all four retinalquadrants confirmed that the spontaneous retinal activity thatre-emerges from P10-P12 tiles the entire surface of the ganglioncell layer and is indistinguishable from that of normal or saline-treatedcontrols in terms of frequency, duration, or amplitude (Fig. 3E,F).Wave domain size was also normal in the epibatidine-recovery retinas(0.31 ± 0.05 mm²; n = 19 waves, vs 0.30 ± 0.06 mm² in control retinas; n = 19 waves), indicating that retinal ganglioncells in both groups are well correlated in theirfiring.

Epibatidine treatment followed by recovery abolishes the normal patterns of cellular lamination in the LGN

In control ferrets, LGN cells form cytoarchitectural layers that lie in direct registration with the layers formed by theterminals of retinal afferents; they are concentrated into distinctA and A1 laminas, as well as ON and OFF sublaminas, each separatedby a cell-sparse interlaminar space (Fig. 4A-D, arrowheads) (Lindenet al., 1981; Stryker and Zahs, 1983; Cucchiaro and Guillery,1984; Zahs and Stryker, 1985; Hutchins and Casagrande, 1990; Hahmet al., 1999). In contrast, the LGNs of the epibatidine-recoveryanimals completely lack normal patterns of cellular lamination(Fig. 4E,H,I,L,M,P). Clusters of cells, surrounded by cell-sparseregions, are occasionally visible, but comparison of these clusterswith the pattern of retinogeniculate afferents in the same tissuesections reveals that they do not correspond to eye-specific terminationzones of ganglion cell axons (for example, compare arrowheadsin Fig. 4E,F).

Although the spatial organization of afferent and cellular laminas seen in each LGN of control animals is remarkably stereotyped(Figs. 2A, 4A-D) (Linden et al., 1981; Stryker and Zahs, 1983;Cucchiaro and Guillery, 1984; Jones, 1985; Zahs and Stryker, 1985;Hutchins and Casagrande, 1990; Hahm et al., 1999), a strikingfeature of the pattern of retinogeniculate inputs of the epibatidine-recoveryanimals is their variability between animals (compare Figs. 2B,4G-N), between the two LGNs of the same animal (Fig. 4M-P), andeven across short distances (<100 µm) through the depth of thesame LGN (Fig. 4F,J).

Effects of early epibatidine treatment on visual responsiveness and functional organization of the LGN

To determine whether disrupting the pattern of retinal afferent lamination alters the physiology of LGN neurons, we performedextracellular recordings in epibatidine-recovery animals. LGNneurons responded vigorously to visual stimuli, confirming thatthe drug treatment did not disrupt the overall health of the retinogeniculatepathway (epibatidine, n = 425 recording sites, n = 4 ferrets agedP52-P71; controls, n = 383 recording sites, n = 9 ferrets agedP37 to adult). All cells encountered were monocular, indicatingthat functional as well as anatomical segregation of eye-specificinputs to the LGN occurred after the termination of the epibatidinetreatment. Cells in the LGN of the treated animals exhibited ON-or OFF-center responses typical of normal ferrets (Fig. 5) (Strykerand Zahs, 1983; Zahs and Stryker, 1985; Chapman and Gödecke,2000). Both sustained (Fig. 5A,E,C,G) and transient (Fig. 5B,F,D,H)responses of both center types were present in both epibatidine-and saline-treated animals. The cells in the treated animals showednormal center-surround organization (compare Fig. 6A-D, salinetreated, with Fig. 5E-H, epibatidine treated), typical of ferretsat this stage of development (Tavazoie and Reid, 2000). The relativepercentage of sites at which exclusively ON- or OFF-center unitsversus both center-type units were recorded along each electrodepenetration was normal (Table 1). As in normal animals, whena mixture of ON and OFF responses was encountered, this alwaysoccurred within a limited region (100-300 µm) adjacent to theoptic tract, where the C layers are typically found (Fig. 7) (Strykerand Zahs, 1983). Multiple vertical electrode penetrations wereused to map the distribution of responses in each animal. In normalanimals, this always reveals four sublaminas in the same sequence:contralateral-ON, contralateral-OFF, ipsilateral-ON, and ipsilateral-OFF(Stryker and Zahs, 1983; Zahs and Stryker, 1985). In the epibatidine-recoveryanimals, there was much more variation in the number of ON orOFF regions within a single penetration; anywhere from two tosix distinct ON or OFF regions were detected. Reconstruction ofadjacent penetrations revealed that these ON or OFF regions werepresent in varying sequence from one penetration site to the next(Fig. 7). In addition, although eye-specific borders always correspondto receptive field center-type borders in normal animals, regardlessof the angle of the electrode penetration (Stryker and Zahs, 1983;Zahs and Stryker, 1985), in the treated animals, exclusively ON-or OFF-center cells often straddled the boundaries of eye-specificlayers (for example, see arrows in Fig. 7). Thus, disrupting thepattern of eye-specific layers disrupts the organization of ONand OFF sublaminas in the LGN but has little effect on the receptivefield properties of the individual cells.

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Figure 5. PSTHs showing ON or OFF responses of single LGN neurons from saline-treated (A-D) and epibatidine-recovery (E-H) ferrets. Sustained (A, E) and transient (B, F) ON responses and sustained (C, G) and transient (D, H) OFF responses were present in both groups of animals.

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Figure 6. Receptive field organization of LGN neurons in saline-treated (A-D) and epibatidine-recovery (E-H) ferrets. Both OFF- (A, B, E, F) and ON- (C, D, G, H) center surround receptive fields were present in both treatment groups. Areas of the receptive fields of the cells excited by light stimuli (ON subregions) are shown in red, and areas excited by dark stimuli (OFF subregions) are shown in blue. Brightness corresponds to the strength of the responses of the cells. Yellow square, 2 × 2 degrees of visual angle.


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Table 1. Relative proportion of sites where exclusively ON- or OFF-center versus both-center-type inputs were recorded in the LGN

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Figure 7. Photomicrograph of the LGN showing the relationship between eye-specific and ON-OFF organization from an epibatidine-recovery ferret. Green represents inputs from the contralateral eye, and red represents inputs from the ipsilateral eye. Four electrode penetrations, spaced 300 µm apart across the rostrocaudal axis of the medial portion of the LGN, are shown; responses were recorded every 100 µm along each penetration. Solid ovals encompass regions along the electrode track in which cells with ON-center receptive fields were recorded. Dashed ovals encompass regions along the electrode tracks in which cells with OFF-center receptive fields were recorded. Rectangles encompass regions in which cells with mixed ON and OFF receptive fields were recorded. Arrows indicate one case in which a region of ON-center cells traverses several eye-specific borders. Tissue section is in the parasagittal plane; at the age shown (P65), rostral is to the right, and dorsal is to the top of the image. Scale bar, 200 µm.

Surprisingly, in the epibatidine-recovery animals, the topographic representation of the binocular visual field was mappedsmoothly in a given penetration, even across the boundaries ofeye-specific borders (Fig. 8). As in normal ferrets, peripheralazimuths were represented rostrally, whereas higher elevationswere represented dorsally (Fig. 8) (Stryker and Zahs, 1983; Zahsand Stryker, 1985). Thus, dramatically disrupting the organizationof eye-specific and ON and OFF lamination does not affect thegross topographic representation of visual space in the LGN. Thisfinding is especially unexpected given the widely varying patternof eye-specific layers both between and within the LGNs of thetreated animals.

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Figure 8. Retinotopic organization of the LGN in a saline-treated (A) and an epibatidine-recovery (B) ferret. Receptive fields recorded from two electrode penetrations spaced 300 µm apart along the rostrocaudal axis of the LGN are shown for both animals. Numbers indicate the order that cells were recorded in each experiment. Recording sites were 100 µm apart along the electrode penetration. Green corresponds to contralateral eye responses, and red corresponds to ipsilateral eye responses. In A, receptive fields 1-16 were recorded in one electrode penetration, whereas receptive fields 20-30 were recorded in a separate electrode penetration positioned 300 µm more rostral. Three additional cells (17-19) were recorded at the bottom of the more caudal penetration, but their responses were too weak to plot reliably. In B, receptive fields 1-12 were recorded in one electrode penetration, whereas receptive fields 20-29 were recorded in a separate electrode penetration positioned 300 µm more rostral. Seven additional cells (13-19) were encountered at the top of the more rostral penetration, but their receptive fields were located above and peripheral to the tangent screen, so they could not be carefully plotted; they are not included here.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Our results show that the development of lamination in the LGN reflects three processes: the segregation of retinogeniculateafferents, the patterning of those afferents into layers, andthe emergence of cellular layers that correspond to the patternof afferent layers. During normal development, the segregationof retinal afferents into eye-specific territories and the patterningof those territories into afferent layers of stereotyped shape,size, and position occur in parallel. Eye-specific afferent layersemerge from a state in which inputs from the two eyes overlapextensively and then segregate directly into layers A and A1;they never segregate into patches within the region of initialoverlap (Fig. 1A-C) (Linden et al., 1981; Shatz, 1983; Cucchiaroand Guillery, 1984; Hutchins and Casagrande, 1990; Penn et al.,1998; Hahm et al., 1999). This has suggested that afferent segregationand afferent lamination are the same process. Cellular laminascorresponding to the pattern of afferent layers emerge soon aftersegregation is complete (Rakic, 1976; Linden et al., 1981; Shatz,1983; Cucchiaro and Guillery, 1984; Hutchins and Casagrande, 1990).Previous experiments show that removal of one eye early in developmentresults in an expansion of the inputs from the remaining eye tofill almost the entire LGN and a corresponding loss of eye-specificcellular lamination (Rakic, 1981; Guillery et al., 1985a; Sretavanand Shatz, 1986; Garraghty et al., 1988; Morgan and Thompson,1993). Moreover, in coat-color mutants in which abnormal retinogeniculateprojections develop, the cellular laminas mirror those abnormalprojections (Guillery, 1969, 1971; Guillery et al., 1985a). Theseresults, in which the pattern of cellular lamination mirrors thatof the afferents, suggested that cellular lamination is drivenby the projection pattern of theafferents.

Here we show, however, that eye-specific afferent segregation can develop without normal afferent lamination, demonstratingthat these are in fact distinct processes. We also show that wheneye-specific afferent segregation is not accompanied by normalafferent lamination, interlaminar zones corresponding to the patternof inputs from the two eyes failed to develop. Therefore, cellularlamination is also decoupled from afferentsegregation.

Our results reveal a critical period for normal development of the LGN. Preventing spontaneous retinal activity during thiscritical period prevents the formation of normal afferent andcellular layers. This indicates that there is something specialabout the developmental time window in which retinogeniculatesegregation normally occurs for proper patterning of laminas inthe LGN. Surprisingly, however, axons from the two eyes remaincapable of segregating into nonoverlapping termination zones afterthe end of this critical period for lamination. Thus, the exacttiming of lamination is crucial, but eye-specific segregationcan occur even if it begins after the developmental stage in whichit normally would be complete. It is unclear what factors areessential for normal lamination of the LGN and why these are limitedto the developmental period in which eye-specific segregationnormallyoccurs.

It is possible that the pattern of spontaneous retinal activity present from P1 to P10 could be instructive toward developmentof lamination. The pattern of spontaneous retinal activity isdifferent from P1 to P10, when eye-specific segregation normallyresults in lamination, than it is from P10 to P25 (Wong et al.,1993), when we show that eye-specific segregation results in patches.However, it is unlikely that activity is sufficient to instructthe development of lamination. First, during the same developmentalstage when retinogeniculate afferents segregate into eye-specificlaminas, retinal activity also induces contralateral and ipsilateralganglion cell afferents to segregate into clusters rather thanlayers in the rostral superior colliculus (Thompson and Holt,1989). Second, in studies in which retinal inputs were rewiredinto the medial geniculate nucleus, afferents from the two eyesinitially overlapped and then segregated into eye-specific patchesinstead of layers (Angelucci et al., 1997). Spontaneous retinalactivity was normal throughout development in these animals, andyet this did not produce normal lamination. These results indicatethat layer formation is controlled by cues that are intrinsicand unique to the LGN, rather than by patterns of retinal activity.Moreover, it is hard to imagine how activity could give rise tohighly stereotyped eye-specific layers, because activity is likelyto differ across animals, and yet eye-specific laminas in theLGN always form in the same positions as layers of essentiallyinvariant size, shape, and orientation (Figs. 1B, 2A, 4A-D) (Lindenet al., 1981; Stryker and Zahs, 1983; Cucchiaro and Guillery,1984; Zahs and Stryker, 1985; Hutchins and Casagrande, 1990; Pennet al., 1998; Hahm et al., 1999; Stellwagen and Shatz, 2002).

Theoretically, the timing of fiber ingrowth could influence the final pattern of eye-specific layers in the LGN. Axons fromthe contralateral eye arrive before axons from the ipsilateraleye (Linden et al., 1981; Cucchiaro and Guillery, 1984), raisingthe possibility that layers are patterned such that earliest arrivingaxons terminate in the medial-most LGN (future location of layerA). However, axons from the two eyes do not segregate as theygrow into the LGN; they overlap extensively throughout the LGNearly in development (Fig. 1A,C) (Linden et al., 1981; Cucchiaroand Guillery, 1984; Penn et al., 1998). The overlap seen in normalP1 ferrets is similar to that seen in epibatidine-treated ferretsat P10 (Fig. 1A,C,E) (Penn et al., 1998). Therefore, differencesin the timing of ingrowth cannot explain the normal patterningof eye-specific laminas in the LGN or the lack of normal laminasseen in the epibatidine-recoveryanimals.

Patterning of layers thus almost certainly relies on the presence of signals that bias the location and boundaries of theregions into which afferents from one or the other eye segregate.Recent studies have demonstrated a critical role for the ephrinfamily of axon guidance cues in directing nasal and temporal retinalaxons to different regions in the optic tectum and LGN (for review,see Feldheim et al., 1998; Flanagan and Vanderhaeghen, 1998),making the ephrins premiere candidates for patterning of the contralateralA (nasal-retina derived) and ipsilateral A1 (temporal-retina derived)layers in the LGN. However, it is important to note that silencingretinal activity from P1 to P10 prevents normal afferent laminationfrom developing (Fig. 1E) (Penn et al., 1998). Thus, if ephrin-likecues do in fact guide contralateral and ipsilateral retinal afferentsto their appropriate regions in the LGN, activity appears to berequired to "read out" these cues. Additionally, the eye-specificsegregation without normal afferent and cellular lamination seenin the LGN of epibatidine-recovery animals suggests that the abilityof guidance cues to direct incoming axons to their appropriateregions in the LGN is restricted to the phase of development whenaxons normally segregate in this target. This would explain whyin the epibatidine-recovery animals, inputs from the two eyessegregate into a variable projectionpattern.

Our physiological data show that, just as eye-specific retinogeniculate connections can emerge in the absence of normal eye-specificlayers, segregated ON- or OFF-center LGN neurons can develop withoutaccompanying normal ON and OFF sublamination. Nevertheless, disruptingthe spatial organization of eye-specific layers appears to havea profound impact on the overall arrangement of ON and OFF segregationin the LGN. This is surprising in light of a previous report showingnormal ON-OFF lamination in the expanded projection from the remainingeye of monocularly enucleated animals (Morgan and Thompson, 1993).The disruption of ON and OFF sublaminas in epibatidine-recoveryanimals occurs despite the fact that they experienced normal patternsof retinal waves from P12 to P25, when the differential activityof ON- versus OFF-center ganglion cells in the retina drives functionalsegregation of ON and OFF pathways in the LGN (Wong and Oakley,1996; Bisti et al., 1998; Myhr et al., 2001). Because we did notrecord from individual ganglion cells in the epibatidine-recoveryanimals, we cannot be sure that the firing patterns of these neuronsare completely normal; thus, we cannot rule out a role for P12-P25retinal activity in forming normal ON and OFF sublaminas. However,our data suggest that delaying eye-specific segregation untilafter P10 influences the organization of ON-OFF sublaminas, afeature that, based on its later timing during normal development,had appeared independent of the formation of eye-specificlaminas.

Apart from the disruption in ON and OFF patterning, the physiology and functional organization in the LGN of animals in whichafferents are segregated but lamination is disrupted are remarkablynormal. The presence of normal retinotopy in these animals indicatesthat, despite the large degree of overlap in the retinogeniculateprojections from each eye at P10 (Fig. 1C,E), axons from ganglioncells in the two eyes that view identical regions in visual spacesegregated into neighboring domains during the recovery period.This is especially surprising given the highly variable patternof eye-specific inputs to the LGN of the epibatidine-recoveryanimals, and it indicates that binocular, retinotopically organizedmaps of visual space can be organized in many different ways.The relatively normal physiology and functional architecture ofthe LGN in epibatidine-recovery animals also raises the questionof the functional significance of the highly stereotyped LGN laminationin normalanimals.

  FOOTNOTES

Received April 15, 2002; revised Aug. 13, 2002; accepted Aug. 23, 2002.

This work was supported by National Institutes of Health (NIH) Grant EY11369 (B.C.), Core Grant EY12576, and an NIH SystemsNeuroscience Training Fellowship (A.D.H.). We thank B. Reese foradvice on retinal histology; R. Berman and B. Barres for use oftheir imaging facilities; S. Sabo for advice on image quantification;A. Haines and P. Nguyen for expert technical assistance; W. Usrey,M. Sceniak, O. Collins, and H. Alitto for assistance with white-noisereceptive field mapping; and L. Stone for helpful comments onthismanuscript.

Correspondence should be addressed to Dr. Barbara Chapman, Center for Neuroscience, 1544 Newton Court, Davis, CA 95616. E-mail:bxchapman{at}ucdavis.edu.

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DISCUSSION
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