Insulin, glucagon and somatostatin in fetal rat islets maintained free‐floating in culture: immunocytochemistry and radioimmunoassay

Summary— Fetal rat islets maintained free‐floating in tissue culture represent a source of B‐cells. Because we recently noted the occurrence of other cell types during long‐term tissue culture, this in vitro model was used to examine the possible development of non B‐cells. The changes in the numbers and percentages of B, A and D‐cells in vitro were estimated by counting the hormone‐positive cells after immunocytochemical staining. Insulin, glucagon, and somatostatin contents were determined in extracts of the cultured tissue. The experiments described here showed that the cultured islets maintained their viability over a two‐week culture period, as evidenced by the increase of both the number of B‐cells per islet and the DNA content per islet. During the first few days of culture, immunocytochemically stained free‐floating islets indicated the presence of rare A‐ and D‐cells at the periphery of B‐cells; thereafter, numerous A‐ and D‐cells were seen interdigitating with B‐cells. Expressed per islet, the number of A‐ and D‐cells increased during the culture; within the endocrine cell population, the percentage of these cells increased with time, at the expense of the percentage of B‐cells. The glucagon and somatostatin contents of the free‐floating islets were also increased. These converging observations suggest that additional non B‐cells may have been produced by free‐floating islets during long‐term tissue culture.