Fluid compartmentation and electrolytes of cat cerebral cotex in vitro. 3. Ontogenetic and comparative aspects

Studies on swelling and fluid compartmentation have been carried out in vitro on incubated slices of cerebral cortex from kittens 1.5-120 days post-natal age and on incubated sections of corpus callosum and slices of liver and kidney cortex from adult cats. The findings have been compared with analogous data for incubated slices of adult cat cerebral cortex, studied under identical conditions (Bourke and Tower , 1966a, b), in order to identify the probable morphological correlates of fluid and electrolyte distribution. Incubated cortical slices from neonatal (1.5-4-day-old) kittens exhibit none of the relevant characteristics of slices from adult cerebral cortex. By 1 month post-natal age, K⁺-dependent swelling of slices becomes demonstrable, and the K⁺ and Na⁺ contents of slices approximate adult levels. Both these developments coincide with the morphological and physiological maturation of cortical neurons. At 3 months post-natal age, slice swelling accessible to C1^? but not to sucrose becomes observable and the dependence of sucrose space size on time, during incubation, of solute addition becomes demonstrable. Both these developments follow completion of axonal myelination in the cortex but coincide with the period of cortical glial cell proliferation. Incubated sections of corpus callosum from adult cats exhibit none of the relevant characteristics observed for cortical slices under identical conditions. Tissue swelling is minimal and uninfluenced by K⁺ concentrations of incubation media. Tissue fluid spaces accessible to sucrose are approximately twice the size of spaces accessible to inulin. In general, qualitatively similar results have been obtained for incubated slices of cat liver or kidney cortex or for incubated sections of rat diaphragm under the same conditions. A behaviour for glial cells (? astrocytes) in cerebral cortex under such in vitro conditions distinctly different from behaviour of subcortical glial cells is suggested.     

Ultrastructural organization of the neuropil in layer I of the cat cerebral cortex

The ultrastructure of layer I in the middle ectosylvian gyrus (area 22) of the cat's cerebral cortex was investigated. Beneath the subpial astrocytic layer most of the neuropil in layer I was shown to be occupied by nerve fibers and their terminals, terminal branches, dendritic spines, and astrocytic processes surrounding them. More than 90% of the presynaptic terminals contained spherical synaptic vesicles. The predominant types of interneuronal junctions are axo-spinous and axo-dendritic synapses of asymmetrical type. Presynaptic terminals, which contain flattened and pleomorphic synaptic vesicles, take part in the formation of all symmetrical junctions, accounting for 6% of the total number of synapses. Large polymorphic outgrowths filled with vacuoles — so-called multivacuolar sacs — are described. These structures were invaginated into varicose expansion of the terminal branches of apical dendrites of pyramidal neurons. They are shown to be outgrowths of presynaptic terminals. Dependence of synaptic function on the shape of the synaptic vesicles is examined.I. S. Beritashvili Institute of Physiology, Academy of Sciences of the Georgian SSR, Tbilisi. Translated from Neirofiziologiya, Vol. 15, No. 1, pp. 50–55, January–February, 1983.     

Synaptosomal fractions of cat cerebral cortex after hypo-osmotic and detergent treatment.

Different synaptosomal fractions were prepared by subcellular fractionation from cat cerebral cortex. The seperated nerve ending fractions differed in both density and osmotic sensitivity. Synaptosomal ghosts were obtained by hypo-osmotic treatment. In the synaptosomal ghost fractions the synaptic areas seemed to be intact morphologically. The morphology of the "synaptic triad" (pre- and postsynaptic membranes and the synaptic cleft) was not affected even by treatment with Triton X-100 non-ionic detergent (0.6%). The solubilizing effect of different concentrations of the detergent was checked in the supernatants and in the insoluble residues. The homogeneity of various subcellular fractions and the effect of the osmotic and detergent treatments are discussed.     

After-effects of anodal polarization in the cat cerebral cortex

Functional changes in neurons and their glial satellites in the cat motor cortex were studied after surface de polarization. An increase in the frequency of spontaneous and evoked unit activity in deep layers of the cortex was demonstrated by a microelectrode method and shown to continue for 0.5 h after the end of polarization. Layer by layer investigation of the cortex by cytophotometry using visible light of two wavelengths on sections stained with gallocyanin and chrome alum revealed an increase in the number of reactive phosphate groups of nucleic acids after polarization for 15 min and a decrease in their content 20 min after the end of polarization in pyramidal neurons of layer V, followed by an increase in the interneurons of this layer after 75 min. The number of glial satellites in the same layer was increased near the pyramidal neurons 20 min after the end of polarization and near the interneurons 75 min after its end. In layers II, III, and VI no statistically significant changes in these indices could be found. The results show that the cell population activated by surface polarization is formed of neurons in layer V. Prolonged activation of interneurons and their distinguishing structural features are considered to reflect their organizing role in trace processes.Institute of Higher Nervous Activity and Neurophysiology, Academy of Sciences of the USSR, Moscow. Translated from Neirofiziologiya, Vol. 4, No. 3, pp. 256–263, May–June, 1972.     

Phosphorylation of ribosomal proteins in rat cerebral cortex in vitro.

Incubation of cerebral cortical tissue from immature rats in the presence of [32P]orthophosphate resulted in similar rates of incorporation of radioactivity into the proteins of free and membrane-bound ribosomes. Incorporation of label into ribosomal proteins of both species continued actively for at least 3 hours. Since recovery of membrane-bound ribosomes from rat cerebral cortex is quite low, further analyses of the radioactive phosphoproteins were restricted to the free ribosome population. A significant fraction of the radioactivity which was precipitated with trichloroacetic acid was not removed by heating in trichloroacetic acid at 90 degrees or extracted with organic solvents and therefore was presumed to be covalently bound to protein. The radioactive phosphoryl groups present in the ribosomal proteins were mainly in ester linkages since they were readily removed by exposure to 1 N NaOH, relatively unaltered by 1N HCl, and unaffected by hydroxylamine. This conclusion was supported by the isolation of labeled o-phosphoserine and o-phosphothreonine residues from hydrolysates of ribosomal proteins. A significant fraction of the labeled phosphoproteins in the purified ribosomes appeared to be bound tightly to the ribosome structure since only 40% of the radioactivity could be removed by extraction of these ribosomes with 1 M KCl. Phosphorylation of proteins of cerebral monoribosomes was more rapid than the same process in polyribosomes from the same source. Eight radioactive phosphoprotein bands could be detected by electrophoresis of proteins obtained from unfractionated cerebral ribosomes on unidimensional polyacrylamide gels containing sodium dodecyl sulfate. The protein nature of these materials was confirmed by pronase digestion. Proteins of subribosomal particles isolated from the total free ribosomal population were labeled differentially. When dissociation was carried out in the presence of EDTA, the small subunit contained four radioactive phosphoprotein bands, whereas the large subunit contained five. Three of the radioactive phosphoprotein components of the small subunit were removed when dissociation of cerebral ribosomes which were previously washed with high salt media was carried out in the presence of puromycin and high salt. However, only the largest labeled phosphoprotein band of the large subunit was removed by this procedure. This component exhibited the same electrophoretic mobility as one of the radioactive phosphoprotein bands which was removed from the small subunit by high salt treatment..     

Prostaglandin D synthase in microvessels from the cat cerebral cortex

Microvessels, a mixture composed predominantly of small arterioles and capillaries (7–80μ diameter), were isolated from the rat cerebral cortex by selective nylon sieving and glass bead elutriation. The morphology and purity of the microvessel and cerebral cortex filtrate (virtually free of vascular contamination) were monitored by light microscopy and by the activity of several enzymes: γ-glutamyl transpeptidase, GSH-transferase, prostacyclin synthase and PGD synthase. Prostacyclin and PGD synthesizing activities as well as γ-glutamyl transpeptidase activity were localized to the microvessels of the rat cerebral cortex whereas GSH-S-transferase was restricted to the non-vascular filtrate function. The characteristics of the PGD synthase were similar to those of the purified enzyme previously described for the rat brain. The microvessel (MV) PGD synthase was localized to the cytosol fraction of the microvessels and did not require reduced glutathione for activity. The enzyme was inhibitd by pre-incubation with p-hydroxymercuribenzoate (lmM) or N-ethylmaleimide (lmM). The MV PGD synthase saturated at 15–20μM PGH₂, exhibited an apparent K_M of 9.6μM, and a pH optimum of 8.0–8.1. These findings suggest roles for both prostacyclin and PGD synthesis by the rat cerebral vasculature in the autoregulation of cerebral blood flow and/or function. These studies also indicate that the major source of PGI₂ and PGD₂ synthesis by rat brain homogenates is the microvasculature.     

Some data on postnatal maturation of the cerebral cortex in cat

This paper describes the neurons in different cortical areas and traces their postnatal changes. Rapid Golgi and Golgi--Kopsch impregnation were carried out in 1-day-old and 9-day-old kittens. The maturation of the pyramidal neurons can be observed mainly on their basal dendritic orientation and on development of the dendritic spines. The differentiation of the interneurons (non-pyramidal) also proceeds on the first postnatal days. These, though slightly less mature than the associated pyramidal neurons, are identifiable already on the first postnatal day. It is concluded that there are significant differences in the maturation of the neurons in the various cortical areas.     

The connectional organization of neural systems in the cat cerebral cortex

BACKGROUND: The mammalian brain consists of the cerebral cortical sheet, which is composed of many distinct areas, the cerebellar cortex, and many non-cortical nuclei. Powerful neuroanatomical techniques have revealed a large number of connections between these structures. The large number of brain structures and the very many connections between them form a strikingly complex network. The complexity of this network has made it difficult to understand how the central nervous system is organized. Recently, however, optimization analysis of an important subset of central nervous connections that occur between the different areas of the cerebral cortex has produced understandable and quantitative representations of the organization of cortical systems of the primate brain. RESULTS: Here we briefly report the extension of this approach to the cortical systems of the cat. There were four connectional clusters of cortical areas in the cat. These clusters of areas corresponded to the visual, auditory, and somato-motor systems, and to the frontal and limbic areas, which we call the fronto-limbic complex. All the major sensory systems were hierarchically organized, and their 'higher' stations were more closely associated with the fronto-limbic complex than were their 'lower' stations. CONCLUSIONS: Features of the organization of the cat brain, together with earlier primate results, suggest that there may be a common cortical plan in mammals. We suggest that this common plan may involve relatively discrete, hierarchically organized, cortical sensory systems and a topologically central fronto-limbic complex. Specific variations on this wiring plan may relate to evolutionary history and selection for particular ecological niches.     

Anoxia-induced changes in cAMP contents in the cat cerebral cortex]

Effect of the cessation of oxygen supply on cAMP content and neuronal spike activity (NSA) in the cortex brain was studied. The interruption of oxygen supply during in first decades of seconds evoked changes in the pattern of NSA, followed with the decrease of cAMP content (to 56 +/- 10%). Then the phase of neuronal hyperactivity and increase of cAMP level (to 198 +/- 26%) took place. The content of cAMP approximated the basal one in 2.5 min anoxia. Anoxia during 5 min resulted in direct opposite shifts of cAMP content in two groups of cats (an increase up to 223 +/- 11%, and decrease up to 75 +/- 8%, respectively, which correlated with individual features of NSA recovery in postanoxic period and values of cAMP basal level in the cortex of different animals. Upon 30 min reoxygenation after 2.5 min anoxia a decline of the content of cAMP (to 63 +/- 12%) accompanied enhance of NSA. This period of reoxygenation after 5 min anoxia demonstrated two types of reactions, observed in different groups of cats: the first type--NSA tended to normalization with the level of cAMP 44 +/- 8% below basal level, and the second type--insufficient recovery of NSA attended by value of cAMP 90 +/- 13% above basal level.