Amacrine Cells In Turtle Retina Research Articles

Colocalization of enkephalin-, glucagon-, and corticotropin-releasing factor-like immunoreactivity in GABAergic amacrine cells in turtle retina

The large number of amacrine cells which contain γ-aminobutyric acid (GABA) in the turtle retina makes it difficult to examine specific GABAergic cell types. In order to seletively label subpopulations of GABAergic neurons, we have used fluorescent double-labeling immunocytochemical techniques to examine the localization of GABA-like immunoreactivity (LI) in amacrine cells which contain antigens resembling the neuropeptides glucagon (GLUC), corticotropin-releasing factor (CRF) or enkephalin (ENK). GABA-LI was found in 41% of the cells with GLUC-, 100% of the cells with CRF-, and 69% of the cells with ENK-LI. There were regional differences in the presence of GABA-LI in amacrine cell populations with ENK-LI. GABA-LI was present in about 80% of the cells with ENK-LI outside of the visual streak, while only 37% of the cells within the streak had GABA-LI. Based on the distinct morphologies and regional distributions of these peptidergic amacrine cells, we conclude that they represent different subpopulations of GABAergic amacrine cells in the turtle retina. Future studies can now utilize existing information regarding the synaptic connectivity of these peptidergic amacrine cells to help delineate the functions of GABAergic amacrine cells in the turtle retina.

Neurons immunoreactive to choline acetyltransferase in the turtle retina

Light microscopic immunocytochemistry using anti-choline acetyltransferase (ChAT) was performed to stain putative cholinergic amacrine cells in turtle retina. ChAT-immunoreactive somata lie in the inner nuclear (INL) and ganglion cell (GCL) layers. Three types of amacrine cells were found according to the location of their somata and their dendritic stratification pattern in the inner plexiform layer (IPL). Type I amacrines lie in the row of cells closest to the INL/IPL limits and they branch along the s1/s2 border of the IPL. Type II amacrines are displaced to the GCL and they ramify along the s3/s4 border of the IPL. Type III amacrines lie in the middle of the INL, 2-3 rows away from the IPL limits and their dendrites appear to be bi- or tri-stratified in s1 and s3-s4 of the IPL. The turtle ChAT-IR amacrines are thus similar to the types described in chicken retina. A regular, non-random mosaic formed by stained type II amacrine cells was observed in the GCL. Their density in mid-central retina was 750 cells/mm2, tapering off to 393 cells/mm2 in peripheral retina. Our study indicates that a pair of cholinergic amacrine cell types in turtle retina is arranged in mirror-image symmetry contributing to sublamina "a" and sublamina "b" of the IPL, like in other vertebrate retinas.

Characterization and quantification of peptidergic amacrine cells in the turtle retina: enkephalin, neurotensin, and glucagon.

Immunocytochemical methods were used for selective labeling and characterization of amacrine cells of the turtle (Pseudemys scripta elegans) retina which contained neuropeptide-like immunoreactivity (leu-enkephalin, glucagon, and neurotensin). Processes of amacrine cells arborized in specific strata of the inner plexiform layer (IPL). Different strata were defined in relation to the boundaries of the IPL. Zero represented the strata nearest the inner nuclear layer and 100 represented the strata nearest the ganglion cells. Antisera directed against leu-enkephalin labeled approximately 7,300 amacrine cells in a single turtle retina which were concentrated in the region of the visual streak and decreased in density toward the periphery. In retinal regions outside the visual streak the labeled neurons were similar in size and shape with dendritic arbors which lacked a particular orientation. In contrast, in the visual streak, there were particular neurons which were labeled with enkephalin antiserum which had elongated dendritic arbors that ran parallel to the streak. Both types of amacrine cells with enkephalinergic immunoreactivity sent their dendrites into the 0-20 region and the 65-100 region of the IPL. Antisera directed against glucagon labeled approximately 2,500 amacrine cells in a single turtle retina. These cells were concentrated in areas near the visual streak. Amacrine cells labeled with glucagon antiserum had dendritic arbors which were asymmetrically skewed toward one end of the cell and ramified in the 0-20 strata with sparse projections at the 40 and 80 strata of the IPL. Antisera directed against neurotensin labeled 12,800 amacrine cells in a single turtle retina. These cells were concentrated in the region of the visual streak. Two distinct amacrine cell types were labeled selectively. One type had a large, vertically oriented cell body (10 X 14 micron) which gave rise to a single 2-micron-thick process that branched and ramified within the 45-70 strata. The other amacrine cell type with neurotensin-like immunoreactivity had a smaller cell body (8 micron) that sent numerous thin dendrites into the same 45-70 strata. The present results indicated that various neuropeptides were present in amacrine cells of the turtle retina and that a specific neuropeptide could be found in more than one anatomical type of amacrine cell. Each anatomical type of amacrine cell had a unique dendritic arborization which ramified within particular strata within the IPL.