Spatial Firing of Hippocampal Place Cells in Blind Rats

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The Journal of Neuroscience, March 1, 1998, 18(5):1818-1826

Spatial Firing of Hippocampal Place Cells in Blind Rats
Etienne Save, Arnaud Cressant, Catherine Thinus-Blanc, and Bruno Poucet
Centre for Research in Cognitive Neuroscience, Centre National de la Recherche Scientifique, 13402 Marseille Cedex 20, France

  ABSTRACT

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

The rat hippocampus contains cells that are characterized by location-specific firing. Previous work has shown that the angularposition of hippocampal place cell firing fields is accuratelycontrolled by the position of visual cues, suggesting that visionplays a important role in triggering place cell activity. However,a role for other types of information has also been suggestedbecause place cell activity can be recorded while animals aremoving in the darkness. In this study, we asked whether placefields can get established in rats that have never seen theirenvironment. We studied place cell activity in early blind ratsand found that these rats had place cells very similar to thoserecorded from sighted rats. This result suggests that early visionis not necessary for normal firing of hippocampal place cells.Dynamic, motion-related information in conjunction with stimulusrecognition seems to be sufficient.

Key words: hippocampus; unit recordings; place cells; spatial learning; spatial memory; vision; path integration; rat

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

One of the most intriguing features of the rat hippocampus is the existence of place cells. First discovered by O'Keefe andDostrovsky (1971), such cells, when recorded extracellularly froma freely moving rat, have the remarkable characteristic of beingactive only when the animal is in a specific region of its environment.Thus, a given place cell fires in a spatially delimited area calledthe place (or firing) field (O'Keefe and Nadel, 1978; Muller,1996). Together with the well documented impairments in navigationalabilities after lesions of the hippocampus, the existence of placecells provides strong evidence of some important contributionof the hippocampus to the processing of spatial information (O'Keefeand Nadel, 1978; see also Nadel, 1991; Poucet, 1993; Poucet andBenhamou, 1997).

For the last 20 years, the nature of the sensory information that triggers the firing of place cells has been a topic of considerableinterest. Previous work has shown that the location of the placefields can be controlled by visual landmarks (Hill and Best, 1981;Muller and Kubie, 1987; O'Keefe and Speakman, 1987). For example,when a single white cue card attached to the wall of a recordingcylinder is rotated, fields rotate equally, suggesting that placecell firing is under the control of visual cues (Muller and Kubie,1987). Nevertheless, place field positions may also stay stablefor some time when relevant visual cues are removed or the roomlights are switched off (Muller and Kubie, 1987; O'Keefe and Speakman,1987; Quirk et al., 1990), thus suggesting that place cells alsouse nonvisual information to fire in relation to the locationof the animal in space.

One type of information that has been suggested to trigger place cell activity in the absence of visual cues is motion-relatedinformation (O'Keefe, 1976; Hill and Best, 1981; Quirk et al.,1990; Sharp et al., 1995; McNaughton et al., 1996). Accordingto this hypothesis, the rat would update its position by keepingtrack of its movements in space based on signals stemming fromthe proprioceptive and vestibular systems as well as from motorefference copy (McNaughton et al., 1996). However, this strategy,known as path integration (Mittelsteadt and Mittelsteadt, 1980),tends to accumulate errors so that if no recalibration occurs,the cumulative error becomes so large that any further computationis hopeless (Mittelsteadt, 1983; McNaughton et al., 1991; Etienneet al., 1996; Gothard et al., 1996).

Although such calibration supposedly involves the gathering of information from many different sensory systems, it is oftenassumed that visual information plays a key role in this process(e.g., McNaughton et al., 1991). The emphasis on visual informationprobably occurs because vision allows for the simultaneous collectionof a large amount of spatial information, thus enabling organismsto cope rapidly with the major features of their environment.As a result, current thinking about the information primarilyused by the hippocampal place cell system puts strong emphasison the visual system in one way or another. According to thisview, one might expect that visual deprivation would induce profounddisturbances of place cell activity. The present study tests thishypothesis by recording place cell activity from the hippocampusof rats made blind shortly after birth and thus never exposedto any visual stimulus. Place cell activity was recorded whilerats were freely moving in a circular apparatus in which the onlyavailable cues were three-dimensional objects set at the periphery(Cressant et al., 1997). We found that hippocampal place cellsrecorded from blind rats were very similar to place cells recordedfrom sighted rats under the same circumstances, suggesting thatvisual information is not necessary for the spatial firing propertiesof place cells.

  MATERIALS AND METHODS

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

The methods were primarily the same as those used by Cressant et al. (1997), who showed that a set of three three-dimensionalobjects placed in the cylinder standing at the cylinder wall exertedcontrol on the angular position of place fields.

Subjects. Single-unit recordings were obtained from 11 Long-Evans male rats born in the laboratory. Six rats underwent surgicalremoval of their eyes when they were 1 week old. Pups were separatedfrom their littermates when they were 3 weeks old, at which timethey were housed one per cage in a temperature-controlled colony(20 ± 2°C) on a natural light/dark cycle. Electrode implantationand screening for unit activity in both sighted and blind ratsstarted when they were ~90 d old and weighed between 300 and 350gm. They had water ad libitum during all phases of the experiment.Before electrode implantation, the rats were food-deprived to85% of the ad libitum body weight and then trained in a "pellet-chasing"task for 10 d to permit estimation of positional firing rateseverywhere in the cylinder. In this task, the rat had to retrieve20 mg food pellets scattered into the cylinder. The pellets weredelivered through an automatic food dispenser located 2 m abovethe cylinder. The dispenser was equipped with five small tubesthrough which the pellets could drop onto the floor. Because thefood pellets landed in unpredictable places, the rat learned torun almost constantly over the whole floor surface. After trainingwas complete, the rat visited the entire floor area in just afew minutes and so covered the accessible area several times duringa 16 min recording session. The objects that were used duringthe recording were in place during the presurgery training period.

Apparatus. The recording apparatus was a gray cylinder 50 cm in height and 76 cm in diameter. The cylinder was visually isolatedfrom the rest of the laboratory by a concentrically placed cylindricalcurtain 250 cm in diameter and in height. The floor of the cylinderwas a piece of gray paper that was replaced between recordingsessions, so that olfactory cues were made irrelevant to the spatialposition of the rat. During both screening and recording sessions,an FM radio tuned to a music broadcasting station was fixed tothe ceiling in a central position relative to the cylinder tomask possible directional sounds. The rats were introduced intothe recording cylinder from one of four equally spaced positionsaround the circumference. The entry position for a given sessionwas chosen from a list of random numbers.

Three landmark objects were used. The objects differed from each other in color, size, shape, and texture. The objects werea black wooden cone (height, 25 cm; diameter, 11 cm), a whiteplastic cylinder (height, 25 cm; diameter, 10 cm), and a bottleof French red wine (height, 28 cm; diameter, 9 cm). Their locationsrelative to each other were fixed. Each was against the wall ofthe cylinder, forming an isosceles triangle, oriented with thecone at 12 o'clock, the bottle at three o'clock, and the cylinderat six o'clock.

Surgery. Surgery and care after the surgery were conducted according to institutional guidelines. One week after birth (i.e.,before eye opening), six pup rats underwent surgical removal oftheir eyes under halothane anesthesia, after which they were returnedto the cage of their mother. Electrode implantation in both sightedand blind rats was made when they were 90 d old. An injectionof 0.3 ml of atropine was given to prevent respiratory distress.Next, rats were anesthetized with pentobarbital (45 mg/kg) andplaced in a Kopf stereotaxic apparatus. After a midline incisionof the scalp was made, the skin and the muscles were retracted,and holes were drilled in the skull at appropriate locations.A movable array of 10 25 µm electrode wires (Kubie, 1984) wasstereotaxically implanted in the dorsal hippocampus at the followingstereotaxic coordinates: 3.8 mm posterior and 3.0 mm lateral tobregma and 1.5 mm below the dura (Paxinos and Watson, 1986). Miniaturescrews were placed over the right olfactory bulb, the left frontalcortex, and the left cerebellar hemisphere to anchor the headstage.To improve stability, an additional T-shaped screw was loweredupside down into the left parietal bone and turned 90° beforebeing tightened with a small nut. For protection from the dentalcement, sterile petroleum jelly was applied to the exposed brainsurface and the guide tubing of the electrode array. Dental cementwas applied over the jelly and around the guide tubing. The exposedskull was covered with dental resin cement (Ivoclar). The screwsand nut were then embedded in dental cement, and the bottoms ofthe assemblies of the three drive screws were cemented to theskull.

At the completion of the experiment, animals were killed with a lethal dose of pentobarbital and perfused intracardially with0.9% saline followed by 4% formalin. Just before death, positivecurrent (15 µA for 30 sec) was passed through one of the microwiresto deposit iron that could be visualized after reaction with potassiumferrocyanide (Prussian blue). The brains were removed and storedfor 1 d in 3% ferrocyanide. Later, frozen coronal sections 40µm in thickness were taken. Every fifth section was stained withcresyl violet for verification of electrode placements.

Recording methods. Beginning 1 week after surgery, the activity from each microwire was screened daily while the rat chasedpellets in the cylinder. The electrodes were lowered over a periodof several weeks while we searched for unit waveforms of sufficientamplitude to be isolated. Once a unit was isolated, it was recordedduring several 16 min pellet-chasing sessions. Such multiple sessionsare possible because the same cell can be reliably recorded fordays or even weeks (Muller et al., 1987). This makes it possibleto compare the firing of an individual cell after the environmenthas been changed many times.

Screening and recording were done with a cable attached at one end to a commutator that allowed the rat to turn freely. Theother end of the cable was connected to a light-emitting diode(LED) for tracking the head position of the rat, a headstage witha field effect transistor amplifier (FET) for each wire, and finallya connector that mated with the electrode connector cemented tothe skull of the rat. The FETs were used to amplify signals beforethe signals were led to the commutator via the cable. The fixedside of the commutator was connected to a distribution panel.From the panel, the desired signals were amplified 1000-fold withlow-noise differential amplifiers and were bandpass filtered from0.3 to 10 kHz. The signals were then sent to two time-and-amplitudewindow discriminators (model DIS-1; Bak Electronics) arrangedin series for unit isolation. Accepted spikes were converted todigital pulses that were counted for 20 msec intervals. At theend of each such interval [the end of a television frame (seebelow)], the spike count for one or more cells was sent as a fourbit binary number to a computer.

The head position and head direction of the rat were tracked by locating two colored LEDs that were secured to the animalheadstage. The red LED was positioned on the midline ~1 cm abovethe head and somewhat forward of the eyes of the rat. The greenLED, also on the midline, was set ~5 cm behind the red LED. Thetwo LEDs were independently tracked with a television-based digitalspot follower that received the red and green RGB signals froma CCD color camera fixed to the ceiling of the experimental room.Each LED was detected in a grid of 256 × 256 square regions (pixels)6.25 mm on a side, permitting a resolution of ~6° for head direction.For head position tracking, the resolution was reduced by twobits in each dimension, yielding a 64 × 64 grid of pixels 25 mmon a side. The x and y coordinates at the end of each frame werestored in parallel with the number of spikes counted during the20 msec frame.

Testing protocol. The 10 electrodes in each rat were checked several times a day while the rat was in the cylinder. If nocell could be isolated, the electrode bundle was advanced 25-50µm. Cells selected for recording were well discriminated complex-spikecells that showed clear location-specific firing. Activity fromeach microwire was screened daily while the rat was in the recordingapparatus until unit waveforms of sufficient amplitude (>80 µV)could be isolated. Once a unit was well isolated, several recordingsessions were run consecutively to establish whether the positionalfiring patterns were controlled by the position of the set ofobject landmarks in the recording arena.

Before each session, the waveform and the firing pattern were inspected to check for constancy. Between sessions, rats werereturned to their home cages, the objects were removed from theapparatus, and the floor paper in the cylinder was replaced. Next,the objects were placed at appropriate locations in the cylinder.The positions of the objects relative to each other were heldconstant so that the objects could act as reliable spatial cues.

Recordings were made first with the objects in a "standard" position relative to the laboratory frame and next with the objectsrotated as a rigid set around the center of the cylinder. Usually,two sessions with the objects in the standard position were made.The purpose of these standard sessions was to ensure that theposition of the place field of the cell was stable under constantconditions. If this was the case, a first "rotation" session wasdone during which the set of objects was rotated 90° clockwisefrom the standard position. Finally, a second rotation sessionwas conducted with the object set rotated 90° counterclockwiseback to the initial standard position.

Data presentation and analyses. To obtain a positional firing rate distribution, we accumulated the total time that the redlight was detected in each pixel (dwell time) and the total numberof spikes in each pixel for the session duration (usually 16 min).The rate in each pixel was the number of spikes divided by thedwell time. Color-coded firing rate maps were used to visualizepositional firing rate distributions. In such maps, yellow pixelsrepresent locations in which the firing rate was exactly 0.0 Hzfor the whole session. The highest firing rate category is codedas purple. Intermediate firing rates are shown as orange, red,green, and blue pixels (low to high). Pixels that were never visitedduring a session are encoded white. Because the in-field firingrates of place cells can vary over a large range, the values usedas boundaries between color categories were autoscaled for themap of the first sessions recorded for a given cell. To permitcomparisons among positional firing distributions across severalsessions for a cell, we used rate categories for subsequent sessionsthat were the same as that for the first session.

To estimate numerically place field rotation between session pairs, we calculated a pixel-by-pixel cross-correlation as thepositional firing pattern for the second session was rotated in6° steps relative to the positional firing pattern for the firstsession. That is, the pixel-by-pixel cross-correlation was calculated60 times, at rotations of 0, 6, 12, ... 354°. The rotation associatedwith the highest correlation (R_Max) was taken as the rotationof the place field between the two sessions. Counterclockwiserotations were taken as positive; clockwise rotations were takenas negative. The difference between the observed rotation andthe rotation expected if the angular field position were perfectlycontrolled by the stimulus ensemble was the estimate of rotationerror for a pair of sessions. If the field rotated less than expected,the error was taken as negative; if the field rotated more thanexpected, the error was taken as positive.

A place field was defined as a set of at least nine contiguous pixels with a firing rate above the mean firing rate (i.e.,above the total number of spikes during a recording session dividedby session duration). Several numerical measures were used todescribe the positional firing patterns. (1) In-field mean firingrate was the total number of spikes emitted by the cell whilethe rat was in the place field divided by the total time spentby the rat in this field. (2) In-field peak firing rate was thenumber of spikes emitted by the cell in the nine contiguous pixelsof the place field associated with the most activity divided bythe total time spent by the rat in these pixels. (3) Positionalinformation content measured the amount of information (in bits)conveyed about spatial location by a single action potential emittedby a single cell (Skaggs et al., 1993) and was calculated accordingto the formula: I = $Sigma$ _i ( $lambda$ _i/ $lambda$ ) × log₂ ( $lambda$ _i/ $lambda$ )× P_i. In this formula, $lambda$ _i is the mean firing rate ineach pixel, $lambda$ is the overall mean firing rate, and P_i is the probabilityof the animal to be in pixel i (i.e., dwelling time in pixel i/totaldwelling time). The minimal value of positional information contentis 0 for a cell the firing of which does not provide any informationabout location.

To obtain a directional firing rate distribution, we calculated the head direction of the animal from the relative coordinatesof the red and green LEDs (Taube et al., 1990). Head directionanalysis was performed at a resolution of 9°. The total time andthe number of spikes discharged at each head direction for thesession were summed from the collected samples. The directionalfiring rate of the cell was determined by dividing the total numberof spikes in each head direction bin by the total time spent inthe corresponding head direction bin. Because the recorded cellswere place cells and thus had little if any directional selectivity,only a single measure was used to characterize their directionalfiring patterns. Directional information content (in bits) wascalculated according to the formula: I = $Sigma$ _i ( $lambda$ _i/ $lambda$ )× log₂ ( $lambda$ _i/ $lambda$ ) × P_i, where $lambda$ _i is the mean firingrate in each 9° head direction bin, $lambda$ is the overall mean firingrate, and P_i is the probability of the animal to face directioni.

  RESULTS

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

General characteristics of place cells in blind animals

Place cells were first recorded during a session with the objects in a standard position. Figure 1 shows color-coded typicalfiring rate maps for place cells recorded from sighted and blindrats. Inspection of such maps shows that the positional firingproperties of place cells in blind rats were very similar to thoseof place cells in sighted rats. This similarity was confirmedby the measure of positional information content (which characterizesthe positional firing distribution) that yielded similar valuesfor cells recorded from blind and sighted rats (t = 1.51; df =105; NS; Table 1). Similarly, there was no statistically significantdifference in place field size for cells recorded from blind andsighted rats (t = 1.67; df = 105; NS).

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Figure 1. Top. Firing rate maps for four place cells recorded from sighted rats (top) and eight place cells recorded from blindrats (middle and bottom). In each color-coded firing rate map,yellow represents locations in which the firing rate was 0.0 Hz.The highest firing rate category is coded as purple. Intermediatefiring rates are shown as orange, red, green, and blue pixelsfrom low to high. Pixels that were never visited during a sessionare encoded white. The three landmark objects are indicated bythe filled, gray, and open circles. For the cells recorded fromsighted rats shown here, in-field peak firing rate f (in Hz) andpositional information content P (in bits) were f = 7.4 and P= 1.7 (a), f = 2.5 and P = 1.5 (b), f = 15.4 and P = 1.2 (c),and f = 2.7 and P = 2.7 (d). For cells recorded from blind rats,in-field peak firing rate and positional information content weref = 9.6 and P = 1.5 (e), f = 3.7 and P = 1.7 (f), f = 5.4 andP = 2.1 (g), f = 9.0 and P = 2.2 (h), f = 8.2 and P = 1.7 (i),f = 5.0 and P = 2.3 (j), f = 3.2 and P = 1.3 (k), and f = 4.8and P = 1.5 (l).

Figure 2. Bottom. Firing rate maps for two place cells from blind rats across four successive sessions. Rotation errors for Unit#1 (top) were $-$ 5° (R_Max = 0.68) between sessions 1 and 2, $-$ 9°(R_Max = 0.65) between sessions 2 and 3, and $-$ 2° (R_Max = 0.56)between sessions 3 and 4. Rotation errors for Unit #2 (bottom)were +7° (R_Max = 0.46) between sessions 1 and 2, $-$ 1° (R_Max = 0.49)between sessions 2 and 3, and +7° (R_Max = 0.40) between sessions3 and 4.


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Table 1. Main parameters of cell firing in sighted and blind rats

In contrast, place cells from blind rats were slightly more directional than were those from sighted rats as shown by thestatistically significant difference in directional informationcontent, a measure of the directional firing distribution (t =2.74; df = 105; p < 0.001). However, the very low values of directionalinformation content (<1.0) compared with the high values of positionalinformation content suggest that the direction in which the headof the rat pointed was not an important factor of place cell firingin either sighted or blind rats. This was confirmed for placecells from blind rats by additional analyses that rely on themethod of Muller et al. (1994). This method rests on the hypothesisthat directional firing is accurately predicted from the direction-independentpositional firing distribution and the fact that different portionsof place fields tend to be visited with different heading directions.We therefore measured the directional firing rates of place cellspredicted on the basis of these assumptions and compared themwith the observed firing rates. As was found previously for hippocampalplace cells in sighted rats (Muller et al., 1994), very strongagreement was found between predicted and observed firing ratesfor cells from blind rats (all correlations > 0.7; df = 39). Thismeans that the directional selectivity observed in some cellswas perfectly explained by the fact that the rats tended to enterthe place field through stereotypic trajectories. This was particularlytrue for place fields near the wall that can be traversed onlyat restricted head directions. In short, in both sighted and blindrats, location was by far the strongest correlate of place celldischarge. Head direction alone or in combination with positionwas not an important predictor.

In contrast to the similarity in location-selective firing properties, place cells recorded from blind rats tended to dischargeat considerably lower rates compared with place cells recordedfrom sighted rats. The firing rate of place cells in blind ratswas lower according to the three estimates of unit firing (seeTable 1), including overall firing rate (t = 4.54; df = 105;p < 0.0001), mean rate in the place field (t = 7.63; df = 105;p < 0.0001), and peak rate in the place field (t = 3.89; df =105; p < 0.0001). Because mean spike amplitude was comparablefor units recorded from both blind and sighted rats (t = 0.02;df = 105; NS; see Table 1), the differential firing rates canbe hardly seen as resulting from differences in waveform discrimination(in general, a lower amplitude of unitary waveforms makes it necessaryto be more selective about which waveforms are accepted, therebylowering acceptance rates).

Place field distribution

Because, in the absence of visual information, place fields are likely to rely more on close investigation of the object landmarks(although some information about their olfactory and other propertiescan be gathered at some distance), we examined the possibilitythat place field locations in blind and sighted rats might bedifferently distributed in space. For example, place fields inblind rats might tend to cluster around the objects more thando those in sighted rats. However, the proportion of place fieldswith at least one boundary touching an object and of place fieldsthat were away from the objects was not significantly differentin blind and sighted rats (chi-square = 0.02; NS; Table 2).


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Table 2. Proportion of place field locations relative to the objects

Last, fields away from the objects in blind rats were as precise as place fields near the objects, as measured by their positionalinformation content (1.94 for both types of fields). Also therewas no statistically significant difference in positional informationcontent for fields away from the objects between blind and sightedrats (blind rats, 1.94; sighted rats, 1.78; t = 0.8; df = 32;NS). In short, blindness did not induce hippocampal over-representationof locations near the objects.

Cue control of place fields

To establish whether the positional firing patterns of place cells in blind rats were controlled by the position of the setof object landmarks in the recording arena, we usually conductedseveral additional recording sessions (see Materials and Methods).The usual sequence included two sessions with the objects in thestandard position relative to the laboratory frame, followed bya rotation session (during which the objects were rotated 90°clockwise as a rigid set around the center of the cylinder), andfinally ending with a session with the object set rotated 90°counterclockwise (and therefore returned to the initial standardcondition).

Twenty-seven place cells from blind rats were recorded for the whole sequence of sessions, and the results were clear-cut.All place fields were found to be stable under stable conditions(i.e., across the first two standard sessions), to rotate by 90°when the object set was rotated by 90°, and to return back totheir original angular location when the object set was movedback to the standard position (Fig. 2).

In all cells, angular positions of place fields were almost ideally controlled by the position of the object set. This isshown in the scatter plots of Figure 3 in which are summarizedthe results of rotation sessions for the 27 cells recorded forthe whole session sequence. The expected angular position of afiring field (plotted on the x-axis) was derived by adding theangle of rotation of the three objects to the observed angularposition of the firing field for the previous (baseline) session.The y-axis was the observed angular position of the fields forthe next session. As can be seen in Figure 3, the points all liealong the 45° line. In addition, the circular correlation coefficients(Batschelet, 1981) for the 27 points were > 0.98, showing thatthe position of the object set predicted the angular firing fieldlocation with great precision.

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Figure 3. Scatter plots of expected versus observed angular positions of firing fields. A, 1st rotation. B, 2nd rotation. Expected angularposition of a firing field (x-axis) is derived by adding the amountof object rotation to the observed angular position of the firingfield for a baseline session. The observed angular position isplotted on the y-axis.

On average, the absolute rotation error of cells recorded in blind rats was <6° during both the first $-$ 90° rotation (betweensessions 2 and 3) and the second +90° rotation (between sessions3 and 4). This was true both for fields that were close to anobject (i.e., with at least one boundary touching an object; n= 17) and for fields that were some distance away (n = 10). Therewas no exception to this observation for cells recorded in blindrats, just as there was no exception in cells recorded from sightedrats in a previous study that used an identical arrangement ofobjects (Cressant et al., 1997). These results show that evenin blind rats the object set was used as a polarizing stimulusfor the environment.

That the object landmarks were indeed used by the place cell system of blind rats to anchor place field positions was furtherevidenced by complementary analyses of cell firing during thevery first minute of recording sessions. To examine the influenceof previous exploration on cell firing, we started some recordingsessions at the exact moment when the rat was put on the floorat the center of the cylinder facing a randomly chosen direction.Individual paths were analyzed until the occurrence of firingin the place field was observed. At this time, the analysis washalted. In-field cell firing was counted if the cell fired a shortseries of action potentials during a single pass through the field(the exact number of action potentials in the series dependedon the overall firing activity of the cell but was never fewerthan two). Only rotation sessions were examined to eliminate thepossibility that in-field cell firing was inadvertently controlledby static background cues rather than by the landmark objects.Also, only the cells with clearly delineated place fields andwith mean in-field firing rates of >1 Hz were analyzed to removecells with unreliable firing from the analysis.

The timing of action potentials and their locations were analyzed to relate the first occurrence of cell firing in the placefield to the previous behavior of the rat. Specifically, we lookedat how many objects had to be investigated by the rat before apass through the field resulted in cell firing. The results shownin Table 3 indicate that most cells recorded from sighted ratstended to fire from the first moment of entry into the environment.This result strongly suggests that their firing relied on visionof the environment. In contrast, no cell recorded from blind ratswas observed to fire in the field when the rat had not made physicalcontact previously with at least one object. Only 60% of the cellsfired action potentials in the place field after the blind rathad explored one object. All cells were found to fire in the fieldafter the rat had explored all three objects previously (Table3). The failure of cells to fire before the rat had exploredsome significant portion of space was discarded as an explanationfor the reduced overall firing rates of place cells in blind rats;a simulation of the decrease expected on the basis of the timerequired by the rat to contact the three objects revealed thatthis parameter could account only for a 4% decrease in firingrate, whereas the observed mean firing rates in blind rats weredecreased by >57%.


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Table 3. Number and proportion of initial passes through the place field resulting in cell firing as a function of the number of objectsexplored by the rat before cell firing

Behavior

The results reported above suggest that place cell firing in blind rats depended on previous exploration of the objects. Accordingly,it was reasonable to look at whether exploratory behavior of blindrats would differ from that of sighted rats. More specifically,we looked at how rats moved in the cylinder and how they madecontacts with the objects. These behavioral analyses were conductedonly on initial recording sessions so as not to bias the resultswith other confounding factors. For example, between-group differentialsusceptibility to behavioral fatigue across time might resultin different rates of slowing down across sessions for blind andsighted rats.

As expected, blind rats were found to move more cautiously and therefore more slowly in the cylinder than did sighted rats.For each recording session, the change in position of the rat(based on the red LED) was calculated at each 0.5 sec interval,summed over the entire session, and finally divided by the sessionduration. The results shown in Table 4 show that sighted ratsmoved faster than did blind rats (t = 3.97; df = 87; p < 0.0001).As an aside, we note that this difference in speed might be anexplanation for the reduced firing rates of place cells in blindrats. However, the latter hypothesis received little support fromadditional analyses that were made by looking at place cell firingrates during sessions in which blind rats were moving at motionspeeds in the range of the motion speeds observed in sighted rats(10-15 cm/sec). Even under those circumstances, a significantdifference in mean firing rate was still found (blind, 0.52 ±0.07 Hz; sighted, 1.36 ± 0.26 Hz; t = 2.76; df = 35; p < 0.01),thus suggesting that motion speed was not the major cause of lowerplace cell firing rates in blind rats.


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Table 4. Behavioral results

Object exploration was first measured by accumulating the total time the rat spent in the close vicinity of the objects duringthe initial recording session. The area for accumulating timewas a circular region around each object (set to one pixel aroundthe object). A statistical analysis revealed no tendency for blindrats to spend more time near the objects compared with sightedrats (t = 0.98; df = 87; NS; see Table 4).

The total number of contacts with the objects was also analyzed for each session. To do so, the trajectory of the rat wasreplayed and superimposed on a map of the apparatus showing thethree object locations. The occurrence of a contact with an objectwas defined as the red light being within one pixel of the objectradius (i.e., the snout of the rat actually touching the object)at the end of a path starting elsewhere in the cylinder. Successivecontacts to an individual object were counted only if the rathad run a distance corresponding to an arc of 90° of the apparatuswall (60 cm) between each contact. On average, blind rats didnot make more contacts with the objects than did sighted rats(t = 0.47; df = 87; NS), nor did they spend more time exploringthe objects during each contact (t = 0.96; df = 87; NS; see Table4).

Because the number of contacts possibly made during a session depended on the speed of motion of the rat (Fig. 4), an indexwas calculated by dividing the total number of contacts duringa given session by the total distance (in meters) covered by therat during that session to take into account the lower speedsof blind rats. This index was found to be greater in blind ratsas compared with sighted rats (t = 6.09; df = 87; p < 0.0001;see Table 4), showing that, for trajectories of similar length,blind rats made more contacts with the objects than did sightedrats. Figure 4 clearly shows the relation between the speed ofthe rat and the number of contacts with the objects. There wasa clear difference in slopes between blind and sighted rats (blind,slope = 7.9 and R² = 0.84; sighted, slope = 2.56 and R² = 0.25), suggesting that the increase in the number of contactsas a function of the speed of the rat was markedly greater inblind rats than in sighted rats.

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Figure 4. Scatter plot of motion speeds versus numbers of contacts with the objects. In blind rats, the slope of the linear regressionline was 7.9, and speed accounted for 84% of the variance in thenumber of contacts with the objects. In contrast, the slope wasonly 2.56 for sighted rats, with speed accounting for 25% of thevariance in the number of contacts with the objects.

  DISCUSSION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Our results indicate that in spite of early blindness, the rat hippocampal system contains fully functional place cells. Overallthe characteristics of these cells do not seem to make them differentfrom place cells recorded from sighted rats under identical circumstances.The positional firing properties of place cells recorded fromblind rats were very similar to those of place cells recordedfrom sighted rats, and if firing rate was ignored, place cellsfrom blind and sighted rats were virtually indistinguishable.

One major deviation from this similarity concerns firing rates that were markedly lower in cells from blind rats. Becausespike parameters were very similar for cells recorded from bothblind and sighted rats, these lower rates cannot be attributedto some recording bias caused by differential adjustment of windowparameters during recording. Also, the hypothesis that cells fromblind rats were discharging at lower rates because these ratsneeded to contact objects before the first occurrence of firingin the field was discarded as a likely explanation. Last, becauseprevious data suggest the existence of a positive relation betweenthe instantaneous velocity of the animal and the firing activityof place cells (McNaughton et al., 1983), the difference in averagemotion speed that was found between blind and sighted rats inthe present study was examined as a possible explanation of thelower firing rates of place cells in blind rats. Although thishypothesis is attractive, it received little support from additionalanalyses that looked at place cell firing rates in blind ratsduring sessions in which they moved at average speeds similarto those of sighted rats. Even under those circumstances, lowerfiring rates were found in blind rats. Finally, a possible, althoughspeculative, explanation relies on the fact that location-specificactivation of hippocampal place cells normally relies on convergentexcitatory inputs from several sensory systems including vision,proprioception, and vestibular information (McNaughton et al.,1996). In the absence of visual input, activation of hippocampalplace cells relies on a reduced number of sensory sources. Ifone assumes that activation of a given place cell is triggeredby the total net amount of excitatory and inhibitory activitiesit receives (with such activities being determined as well bythe sensory information reaching the hippocampus), then the observeddecrease in place cell firing rates in blind rats might resultfrom the reduced amount of excitatory inputs. An alternative versionof this hypothesis would be that inhibitory modulation by localinterneurons ( $theta$ cells; see Fox and Ranck, 1981) would be increased.Unfortunately, because no attempt was made to record $theta$ cells inthe present study, it is difficult at present to provide supportfor the latter hypothesis.

As seen in sighted rats (Cressant et al., 1997), place cells in blind rats were demonstrated to use three-dimensional objectsintentionally placed into the recording cylinder as spatial landmarks.This was shown by the almost ideal control exerted by the objectset on place field locations. Rotation of the objects was followedby equivalent rotation of place fields. The ability of the placecell system to use the objects as landmarks implies knowledgeof their positions. Because such knowledge cannot be acquiredat a distance by blind rats (contrary to sighted rats who can"sample" the environment visually), it was expected that cellfiring would depend on previous exploratory behavior of the rat.

Clear support for this hypothesis was provided by additional analyses that revealed that, contrary to place cells in sightedrats, no cell in blind rats was observed to fire in the firingfield if the rat had not made physical contact with an objectpreviously. In many cells recorded from blind rats, knowledgeof one landmark position was enough to activate firing in theplace field. This confirms that, to produce coherent firing, thehippocampal place cell system needs information about the locationof objects. This result additionally suggests that the systemis able to use the intrinsic (e.g., olfactory, tactile) propertiesof objects to recognize which object the animal has encountered.However, the fact that in-field cell firing was seen more oftenafter the rat had explored several objects also suggests thatreliability of spatial localization was increased when furtherexploration confirmed the geometrical stability of the environment(Poucet et al., 1986; Gallistel, 1990; Biegler and Morris, 1996;O'Keefe and Burgess, 1996).

Because place fields were also found at locations that were some distance away from the objects, one must imagine that thesystem is able to compute a position everywhere in the environmentand not just at object locations. One possibility is that, oncelandmark positions are known, the place cell system relies onthe dynamic use of internally generated, motion-related informationto update the position of the system throughout the environment.Such information includes kinesthetic signals from the vestibularsystem, proprioceptive cues, and motor efference copy signals(McNaughton et al., 1996). Although motion-related signals areknown to accumulate errors across successive movements in space,such errors can be corrected at each contact with an object byusing the fixed object locations as a means for recalibratinga calculated position. In our experiment, this process is likelyto occur many times during a recording session because of thecombined effects of the small size of the cylinder and of thenumber of objects. Clear behavioral evidence was found in supportof this hypothesis. In fact, detailed analyses of exploratorypatterns revealed that blind rats tended to make exploratory contactswith the objects more often than did sighted rats. Such a patternof exploration is highly suggestive of a compensatory strategythe result of which is to provide blind rats with additional spatialinformation allowing them to recalibrate their position in thearena.

In conclusion, our data provide evidence that, although they can be anchored by visual information when such is available(Muller and Kubie, 1987; Quirk et al., 1990; Sharp et al., 1990),place cells also receive strong inputs from motion-related systemsand other nonvisual modalities (e.g., tactile) that are sufficientto trigger spatially coherent firing. In addition, place celllocation-specific firing does not seem to depend on early visualexperience because it was observed in rats that had never seentheir environment.

The latter observation leads us to make a last point relating to the observation that early visual deprivation in animalsand humans induces behavioral deficits in many spatial tasks (Teesand Midgley, 1978; Dale and Innis, 1980; Lockman et al., 1981;Tees et al., 1981, 1990; Dodds et al., 1982; Tees, 1990). Thisissue has been controversial, however, because some studies reportvery little impairment after visual deprivation (e.g., Lindneret al., 1997; for thorough discussions of human data, see Strelow,1985; Thinus-Blanc and Gaunet, 1997). At any rate, our study suggeststhat the spatial impairments of blind animals, if any, are notthe consequence of a decreased ability of the hippocampal placecell system to keep track of movements in space. Whether suchsparing in location-specific firing of hippocampal place cellswould still be observed had blindness occurred at a later developmentalstage cannot be appreciated at present. Evidence from a previousstudy indicates that the spatial reliability of place cell firingin sighted rats is decreased in the dark relative to normal lightingconditions (Markus et al., 1994). However, several methodologicaldifferences [e.g., in the study of Markus et al. (1994), ratscould see the environment before the lights were turned out, anda disorientation procedure was used before each entry into theexperimental room] preclude drawing any strong conclusion. Therefore,the idea that the unaltered spatial firing patterns in the blindrats of the present study might result from early adaptation tothe absence of vision will require further research.

  FOOTNOTES

Received Oct. 1, 1997; revised Dec. 4, 1997; accepted Dec. 8, 1997.

This work was supported by the Centre National de la Recherche Scientifique and by Centre National de la Recherche Scientifique/NationalScience Foundation Grant 96/0690 and NATO Collaborative ResearchGrant 940777. We thank B. Arnaud and E. S. Hawley for help inconstructing various parts of the unit recording system and L.Eberle and R. Fayolle for electronics. We are grateful to A. Fenton,C. Kentros, R. U. Muller, M. Stead, and S. Wiener for helpfuldiscussions and suggestions. Parts of this paper have been presentedpreviously at the 25th Annual Society for Neuroscience Meeting.
Correspondence should be addressed to Dr. Bruno Poucet, Center for Research in Cognitive Neuroscience, Centre National dela Recherche Scientifique, 31 chemin Joseph-Aiguier, 13402 MarseilleCedex 20, France.

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Materials & Methods
Results
Discussion
References

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