Glutamine synthetase heterogeneous expression as a marker for the cellular lineage of preneoplastic and neoplastic liver populations

Abstract

The distribution of glutamine synthetase (GS) in rat liver and in putative preneoplastic and neoplastic lesions was studied at stages of hepatocarcinogenesis induced by diethylnltros amine (DEN), 2-acetylaminofluorene (AAF) and aflatoxin B₁ (AFB₁) using immunohistochemistry. in control rats, GS was localized entirely to rings 1–3 cells deep surrounding the central veins. Exposure to DEN or AAF resulted in a reduction of these GS-positive (GS⁺) zones by 96 and 61% respectively, due to necrosis of the cells in this compartment, while AFB₁ had little effect (+ foci, adenomas and carcinomas developed in animals exposed to DEN or AAF, but not AFB₁ corresponding to the acute effects. Small GS⁺ foci also identified by other phenotypic abnormalities (e.g. γ-glutamyltransferase) were exclusively associated with the regenerating GS⁺ zone as were a few collections of GS⁺ hepatocytes, the nature of which was uncertain. Although accounting for a very small fraction (+ foci or GS⁺ hepatocytes apparently gave rise to a substantial fraction of adenomas that were GS⁺ (DEN: 43% and AAF: 33%) and an even higher percentage of GS⁺ carcinomas (DEN: 59% and AAF: 39%). No GS⁺ neoplasms were induced by AFB₁ Statistical evaluation of these data strongly suggests that GS⁺ neoplasms originate through initiation of hepatocytes which possess this particular phenotype. Thus, GS might serve as a specific marker for tracing cell lineage relationships dur ing hepatocarcinogenesis. The GS⁺ phenotype which confers glutamine independence may also provide a growth ad vantage.