Time course profile and cell-type-specific production of monokine induced by interferon-gamma in concanavalin A-induced hepatic injury in mice: Comparative study with interferon-inducible protein-10

Citation
Y. Itoh et al., Time course profile and cell-type-specific production of monokine induced by interferon-gamma in concanavalin A-induced hepatic injury in mice: Comparative study with interferon-inducible protein-10, SC J GASTR, 36(12), 2001, pp. 1344-1351
Citations number
48
Categorie Soggetti
Gastroenerology and Hepatology","da verificare
Journal title
SCANDINAVIAN JOURNAL OF GASTROENTEROLOGY
ISSN journal
00365521 → ACNP
Volume
36
Issue
12
Year of publication
2001
Pages
1344 - 1351
Database
ISI
SICI code
0036-5521(200112)36:12<1344:TCPACP>2.0.ZU;2-B
Abstract
Background: We have previously shown that interferon-inducible protein-10 ( IP-10), a chemokine for activated lymphocytes, was specifically induced in the liver of Concanavalin A (Con A)-treated mice. The aim of this study was to investigate the time course profile and cell-type-specific hepatic prod uction of monokine induced by interferon-gamma (MIG), a chemokine which sha res its receptor and most of its activity with IP-10, in Con A-treated mice and to compare them with those of IP-10. Methods: Hepatic mRNA expression of MIG and IP-10 was studied by means of Nor-them blot analysis and in situ hybridization in Con A-treated mice. The levels of MIG and IP-10 in the se rum and culture supernatants of marine hepatoma-, hepatic sinusoidal endoth elial cell-, hepatic stellate cell- and macrophage-derived cell lines were determined by means of specific enzyme-linked immunosorbent assays, Results : The serum level of MIG slowly reached a maximum at 12 h after Con A injec tion and remained elevated for a long time, whereas that of IP- 10 reached a maximum at 3 h and declined quickly, a finding supported by Northern blot analysis. Using in situ hybridization, the mRNA of MIG as well as IP- 10 w as found to be expressed in hepatocytes and hepatic non-parenchymal cells. Similar to IP-10, MIG was produced by hepatoma-, hepatic sinusoidal endothe lial cell-, hepatic stellate cell- and macrophage-derived cell lines in vit ro. Conclusions: Although both MIG and IP-10 were produced by hepatocytes a nd hepatic nonparenchymal cells in Con A-treated mice, the time course prof ile of MIG was distinguish able from that of IP-10. The fact that hepatic M IG and IP-10 were produced sequentially in this hepatitis model may suggest that a non-redundant role is played by these two chemokines in the process of hepatic necro-inflammation.