Liver receptor homolog-1 (LRH-1) is a transcription factor and belongs to nuclear receptor 5A subfamily. LRH-1 is mainly expressed in liver､intestine and in ovary. LRH-1 has been shown to enhance the tanscriptional activity of several steriodogenic promoters including CYP11A1. Our previous studies indicated that PIASy markedly inhibited the mLRH-1-stimulated activity of the human CYP11A1 promoter. This study investigates the molecular mechanism of the expression of PIASy on mLRH-1-mediated transcription. A series of fusion proteins of Gal4-mLRH-1 and VP16-PIASy were constructed. Mammalian two-hybrid assay demostrates the protein-protein interaction between mLRH-1 and PIASy. In addition, the C-terminal residues 193-560 of mLRH-1 and C-terminal of PIASy are invovled in this interaction. We futher tested whether PIASy inhibits mLRH-1 transactivity by interfering the interaction between mLRH-1 and coactivators. We found that SRC-1 can partially rescued the PIASy inhibition of mLRH-1 transactivity. Furthermore, mammalian two-hybrid assay recealed that PIASy reduced the interaction between mLRH-1 and SRC-1.It suggests that PIASy may function as a repressor of mLRH-1 by interfering the action of SRC-1. In addition, we found that both β-catenin and TBP can inhibit the mLRH-1 sitimulated CYP11A1 promoter activity. Our previous studied indicated that the DNA binding domain of mLRH-1 may contain two nuclear localization signaling peptides (117-168 and 169-193). In this study, we examined the location of mutated by immunocytochemistry. Deletion of residues 116-169 or 169-193 has no effect on nuclear localization of mLRH-1. However, removal of residues 116-193 results in a evenly distribution of mLRH-1 in nucleus and cytoplasm. It suggested that either 116-169 or 169-193 is sufficient for nuclear localization of mLRH-1.