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Notes: A fluorescent dye (usually fast blue or rhodamine tagged latex microspheres) was injected into cortical area 17 (or area 17 and the lateral part of area 18b) of adult and juvenile (15–22 day old) Sprague-Dawley albino rats. Another fluorescent dye (usually diamidino yellow) was injected into cortical areas 17, 18a and 18b of the opposite hemisphere. The injections involved only the cortical grey matter. After postinjection survival of 2–14 days the distribution of retrogradely labelled mesencephalic and prosencephalic cells was analysed. Both small and large injections labelled retrogradely a substantial number of cells in specific and nonspecific dorsal thalamic nuclei (lateral geniculate, lateral posterior, ventromedial, several intralaminar nuclei and nucleus Reuniens) as well as a small number of cells in the preoptic area of the hypothalamus and the mesencephalic ventral tagmental area (VTA). While labelled thalamic cells contained only the dye injected into the ipsilateral cortex, a small proportion of hypothalamic and VTA cells was labelled with the dye injected into the contralateral cortex. Virtually none of the cells in these areas were double labelled with both dyes. Both small and large injections labelled cells in the ipsilateral telencephalic magnocellular nuclei of the basal forebrain and the caudal claustrum. A substantial minority of labelled cells in these structures was labelled by the dye injected into the contralateral cortex. Furthermore, a small proportion (about 1%) of claustral cells projecting to the ipsilateral cortex were double labelled with both dyes. In several cortical areas ipsilateral to the injected area 17, associational neurons were intermingled with commissural neurons projecting to the contralateral visual cortex. A substantial proportion of associational neurons projecting to ipsilateral area 17 also projected to the contralateral visual cortex (associational-commissural neurons). Thus, in visual area 18a, the associational-commissural neurons were located in all laminae, with the exception of lamina 1 and the bottom of lamina 6, and constituted about 30% of the neurons projecting to ipsilateral area 17. In paralimbic association area 35/13, associational-commissural neurons were located in lamina 5 and constituted about 20% of neurons projecting to ipsilateral area 17. In the limbic area 29d, the associational-commissural neurons were located in laminae 4, 5 and the upper part of lamina 6 and constituted about 10% of the associational-commissural neurons projecting to ipsilateral area 17. In oculomotor area 8, double-labelled neurons were located in lamina 5 and constituted about 10% of the neurons projecting to ipsilateral area 17. Thus, it appears that the axons of mesencephalic and diencephalic neurons projecting to the visual cortex do not send collaterals into both hemispheres. The bihemispheric projection to the rat's visual cortex originates almost exclusively in the retinotopically organized cortical area 18a and in integrative cortical areas 35/13, 29d and 8.

Notes: Numerous cortical neurons in the juvenile and adult rat project to visual areas of both hemispheres whereas the vast majority of subcortical structures projecting to the visual cortex send strictly ipsilateral projections (Dreher et al., 1990). In the present study, the authors have sought to determine whether this pattern of axonal bifurcation in the connectivity of the visual areas undergoes a change during postnatal development. Two retrograde fluorescent dyes were used, fast blue (FB) and diamidino yellow (DY). Large multiple injections of one of the dyes were placed in all visual areas of one hemisphere and a small injection of the other dye was placed in area 17 of the opposite hemisphere. Labelled neurons were observed in subcortical and cortical structures on the side of the small injection. The experiments were performed on ten neonatal albino rat pups aged between 3 and 12 postnatal days (p.n.d.) at the time of injection and the results were compared with those obtained in the juvenile and adult animals, as reported in the preceding paper. In the thalamus of newborn animals, neurons belonging to nuclei located away from the midline send strictly ipsilateral cortical projections. However, in the midline nuclei of the intralaminar thalamic complex, a small region of overlap was observed between neurons projecting ipsilaterally and neurons projecting contralaterally in animals aged less than 9 postnatal days. In addition, in these neonatal animals a small number of bilaterally projecting neurons was detected in this region of overlap. In all other subcortical structures examined (ventral tegmental area, diagonal band of Broca, claustrum), the laterality of the projection was the same in the newborn and the adult animals. In particular, in the claustrum of neonatal animals, as in adult animals, there was a large contingent of contralaterally projecting neurons and only a very small number of bilaterally projecting neurons. The results in the cortex contrast with those observed in subcortical structures. Whereas ipsilaterally projecting neurons were distributed in a broadly similar way in newborn and adult animals, the laminar and areal distribution of contralaterally projecting neurons in newborn animals clearly differed from those observed in the adult animals. Furthermore, double labelled neurons were more numerous in animals aged less than 12 days than in adults. The proportions of such bilaterally projecting neurons were computed with respect to the numbers of neurons sending ipsilateral projections to area 17. These proportions are constant at all ages in the claustrum and cortical area 8. In areas 18a, 29 and 35 on the other hand, the proportions of bilaterally projecting neurons increase after 5 days and reach a peak in the period extending from 9 to 11 days of age when more than half of the neurons projecting ipsilaterally also send an axonal branch to the contralateral cortex. In cortical areas 29 and 35, this peak is followed by a sudden drop to the adult level at 12 postnatal days, whereas the return to the adult level is gradual in area 18a. These results demonstrate that, in subcortical structures and in cortical area 8, the laterality of the afferent connections to the visual cortex does not change during postnatal development. By contrast, cortical areas 18a, 29 and 35 go through a stage when numerous cells send bifurcating connections to both hemispheres. The timing of the decrease in proportions of bilaterally projecting neurons in these areas suggests that numerous neurons retract their callosal axonal branch when the adult pattern of callosal connectivity is established at 9–11 days of age.

Notes: Abstract Binocular non-dominant suppression (NDS) in the dorsal lateral geniculate nucleus (LGNd) of the cat was studied by recording from single neurons in the LGNd of anaesthetized, paralysed cats while stimulating the non-dominant eye with a moving light bar. The maintained discharge rate of LGNd neurons was varied by stimulating the dominant eye in various ways: by varying the size or contrast of a flashed spot, by varying the inner diameter of a flashed annulus of large outer diameter, by varying the velocity of a moving light bar, and by covering the eye. Non-dominant suppression was quantified either as the decrease in the maintained discharge rate (the “dip”), expressed as spikes per second, or as the ratio of the dip to the maintained discharge rate (the “dip ratio”). At low maintained discharge rates the dip, although low in value, frequently approached the maintained rate, i.e. the dip ratio approached unity. As the maintained discharge rate increased the dip value also increased, but more slowly than the maintained discharge rate, i.e. the dip ratio decreased. At maintained discharge rates above about 30 spikes/s, in many neurons the dip appeared to be approaching a constant value. This strong dependence of NDS on the maintained discharge rate of the LGNd neuron suggests that the inhibitory input to the cell arises from a region of the brain that receives an input both from the non-dominant eye and from the LGNd cell. Reasons are given for thinking that this region is the perigeniculate nucleus. Because of the strong dependence of dip and dip ratio on the maintained discharge rate, it was necessary to adopt stringent criteria when comparing NDS in two different sets of neurons or of the same set of neurons in different conditions. We recognized a significant difference in NDS between two classes of neurons or between two states only if: (1) there was no significant difference between the maintained discharge rates, and (2) there was a significant difference for both dip and dip ratio between the two classes or states. Using these criteria we found: (1) no difference between non-lagged X (XNL) and non-lagged Y (YNL) cells, (2) no difference between on-centre and off-centre cells for either XNL or YNL cells, (3) no difference between XNL cells and lagged X (XL) cells. However, there was a significant difference between cells in lamina A and those in lamina A1 for both XNL and YNL cells, dip and dip ratio values being about twice as great in lamina A. In cats in which one optic nerve had been pressure-blocked so as to prevent conduction in the largest axons (Y fibres), loss of conduction in Y fibres crossing the chiasm and projecting to the contralateral LGNd did not affect NDS. Loss of conduction in Y fibres projecting to the ipsilateral LGNd caused a complete loss of NDS in the non-lagged Y cells of lamina A and a substantial decrease in the NDS of the nonlagged X cells of lamina A. The latter cells must, therefore, be partly suppressed by non-Y fibres, presumably X fibres. It also follows that all the NDS of cells in lamina A1 is mediated by non-Y fibres, probably X fibres. Thus, NDS in the cat is partly class-specific and partly not. The discharge of retinal ganglion cells also protects the LGNd cells against NDS. The contribution of Y fibres to this anti-suppressive action was also examined. Contralaterally projecting Y fibres make no contribution. Ipsilaterally projecting Y fibres exert an anti-suppressive action on non-lagged X cells in lamina A1. It follows also that the anti-suppressive action on cells in lamina A mediated by contralaterally projecting fibres is due to non-Y fibres, presumably X fibres. Thus, both the suppressive and the anti-suppressive actions of Y fibres are mediated only by the uncrossed pathway.

Notes: Summary Afferent connections of rat primary visual cortex (area 17 or V1 area) and the rostral and caudal parts of areas 18a and 18b were studied, by placing in each of the areas, small electrophoretic injections of enzyme horseradish peroxidase (HRP) or wheat germ agglutinated-HRP. The results indicate that: 1) each of the areas has a distinct pattern of distribution of afferent neurons in the ipsilateral visual thalamus — area 17 receives its principal thalamic input from the dorsal lateral geniculate nucleus, the caudal parts of areas 18a and 18b receive a major thalamic input from the lateral posterior nucleus and a minor input from the posterior nucleus, while the rostral parts of areas 18a and 18b receive a major input from the posterior nucleus, and a minor projection from the lateral posterior nucleus; 2) the rostral and caudal parts of areas 18a and 18b each receive an associational input from area 17; 3) the rostral parts of areas 18a and 18b each receive associational input from three different extrastriate regions, the caudal part of the same extrastriate area, and the rostral and caudal parts of the other extrastriate area, whereas the caudal parts of areas 18a and 18b receive associational inputs only from one or two extrastriate regions; 4) area 17, area 18b and rostral area 18a each receive a substantial associational input from lamina V of the caudal part of the frontal eye field (FEF) in the motor cortex; however the input from the FEF to caudal area 18a (if present) is very small; 5) The extrastriate areas studied receive associational input from the restrosplenial cingulate area 29d; however, the input from area 29d to area 17 appears to be very small. The distinct patterns of distribution of prosencephalic afferents suggest to us that multiple retinotopically organized areas described previously in the rat cortex (cf Montero 1981; Espinoza and Thomas 1983) represent functionally distinct areas.

Notes: Summary The patterns of callosal interconnections between the visual cortices of rats display considerable plasticity in response to various neonatal manipulations. In the present study, many neurones in the principal visual thalamic relay nuclei, the dorsal lateral geniculate nucleus (DLG) and to a lesser extent those in the lateral posterior nucleus (LP) were destroyed by injections of the neurotoxin — kainic acid — on the first day of postnatal life. Four weeks later, as demonstrated with the anterograde and retrograde transport of the enzyme horseradish peroxidase (HRP) injected into the occipital lobe of one hemisphere, callosally projecting neurones and terminals were distributed more widely in the retinotopically organized areas 17, 18a and 18b of the visual cortex ipsilateral to the lesioned visual thalamus than in unoperated control animals of the same age. By contrast, in the visual cortex contralateral to the lesioned visual thalamus the areal distribution of callosally projecting neurones and terminals was similar to that of the controls, that is, largely but not exclusively restricted to the common border of areas 17 and 18a. Both in unoperated and operated animals, cells in lamina V of several cytoarchitectonically defined areas that are not retinotopically organized (area 8 in the frontal lobe, area 29d in the retrosplenial limbic cortex and perirhinal areas 35/13 in the temporal lobe) also project to contralateral visual cortices. In areas 8 and 29d, the total numbers, laminar distributions and densities of labelled callosal cells both ipsilateral and contralateral to the kainate-injected visual thalamus were similar to those in the controls. However, in the temporal lobe, the areal distribution of the labelled callosal neurones was more extensive than that in the controls and labelled cells in areas 35/13 of the cortex contralateral to the kainate-lesioned visual thalamus merged with those in the neighbouring areas 20 and 36. By contrast, the areal distribution of associational neurones in area 18a and in nonretinotopically organized areas projecting to area 17 were very similar in controls and in operated animals (neonatal kainate lesion of the visual thalamus, neonatal section of the corpus callosum or both procedures combined). However, in operated animals, the labelled associational neurones projecting from the supragranular laminae (II/III) of area 18a to area 17 constituted a higher proportion of all cells than did those in the unoperated control animals. Thus, overall the number of associational neurones projecting from area 18a to area 17 was slightly increased by the experimental manipulations performed. The implications of these results concerning the mechanism(s) underlying the developmental changes in the distribution of commissural and associational neurones projecting to the rat's visual cortex are discussed.

Notes: Summary Using tissue from the inner layers of the retina as the immunogen, we have prepared a monoclonal antibody which is selective for two classes of neuron in the cat retina. The antibody, termed 4B2, was generated by intrasplenic injection, demonstrating that neuron-specific antibodies can be elicited by this technique, which requires only micrograms of immunogen. The 4B2 binds to the somas, dendrites and axons of ganglion cells. Double labelling with 4B2 and with a retrograde tracer injected into the retino-recipient nuclei of the brain demonstrates that, of the cell classes in the ganglion cell layer, 4B2 labels only ganglion cells, and that, amongst ganglion cells, 4B2 is strongly selective for large (α-) and medium-sized (β- and perhaps γ-) cells. Double labelling with 4B2 and with markers for amacrine cells confirms tht 4B2 does not label amacrine cells. Double labelling with 4B2 and with anti-GFAP confirms that 4B2 does not label the macroglia of the retina. The 4B2 also labels bipolar cells, showing their somas, dendrites and axons. The axons of the labelled cells terminate in large boutons, in the innermost part of the inner plexiform layer and in the ganglion cell layer. This level of termination suggests that 4B2 labels rod bipolars, and perhaps a subgroup of cone bipolars. Double labelling with 4B2 and with markers for amacrine, horizontal and Müller cells indicates that other cell classes with somas in the inner nuclear layer remain unlabelled. In addition, we have examined the ontogeny of 4B2 labelling in the cat retina. The developmental sequence of labelling with 4B2 follows the sequence in which the cells are born, first ganglion and then bipolar cells.