Similarity between rat brain nicotinic α-bungarotoxin receptors and stably expressed α-bungarotoxin binding sites

The present results demonstrate stable expression of α-bungarotoxin (α-BGT) binding sites by cells of the GH 4 C 1 rat pituitary clonal line. Wild-type GH 4 C 1 cells do not express α-BGT binding sites, nor do they contain detectable mRNA for nicotinic receptor α2, α3, α4, α5, α7, β2, or β3 subunits. However, GH 4 C 1 cells stably transfected with rat nicotinic receptor α7 cDNA (α7/GH 4 C 1 cells) express the transgene abundantly as mRNA, and northern analysis showed that the message is of the predicted size. The α7/GH 4 C 1 cells also express saturable, high-affinity binding sites for 125 I-labeled α-BGT, with a K D of 0.4 nM and B max of 3.2 fmol/10 6 intact cells. 125 I-α-BGT binding affinities and pharmacological profiles are not significantly different for sites in membranes prepared either from rat brain or α7/GH 4 C 1 cells. Furthermore, K D and K i values for 125 I-α-BGT binding sites on intact a7/GH 4 C I cells are essentially similar to those for hippocampal neurons in culture. Sucrose density gradient analysis showed that the size of the α-BGT binding sites expressed in α7/GH 4 C 1 cells was similar to that of the native brain α-BGT receptor. Chronic exposure of α7/GH 4 C 1 cells in culture to nicotine or an elevated extracellular potassium concentration induces changes in the number of α-BGT binding sites comparable to those observed in cultured neurons. Collectively, the present results show that the properties of α-BGT binding sites in transfected α7/GH 4 C 1 cells resemble those for brain nicotinic α-BGT receptors. If the heterologously expressed α-BGT binding sites in the present study are composed solely of α7 subunits, the results could suggest that the rat brain α-BGT receptor has a similar homooligomeric structure. Alternatively, if α-BGT binding sites exist as heterooligomers of α7 plus some other previously identified or novel subunit(s), the data would indicate that the α7 subunits play a major role in determining properties of the α-BGT receptor.