The nuclear translocation of STAT1 and STAT2 is a key process in

The nuclear translocation of STAT1 and STAT2 is a key process in IFN-α transduction signaling. We and others have shown that STAT1 translocation is impaired in Pol-expressing and HBV-infected hepatocytes.6, Opaganib price 7 We further examined whether Pol interferes with IFN-α–induced STAT2 nuclear accumulation. In the absence of IFN-α, STAT2 was predominantly localized in the cytoplasm, whereas STAT1 was found in both the cytoplasm and nucleus; upon IFN-α stimulation, strong nuclear accumulation of both STAT1 and STAT2 was

observed, but only in cells without Pol expression (Fig 4A). Furthermore, the protein levels of STAT1/2 in the cytoplasmic and nuclear fractions of Dox-treated or Dox-free HepAD38 cells were determined via immunoblotting. As shown in Fig. 4B, the accumulation of STAT1/2 in the nucleus following IFN-α treatment was significantly detained in Dox-free (Pol-expressing) cells. Impaired nuclear translocation

DAPT research buy of STAT1/2 was also observed in HepG2.215 cells compared with HepG2 cells (Supporting Fig. 6). Importin-α5 (also known as karyopherin α1), a nuclear localization signal receptor, has been shown to specifically interact with the STAT1-STAT2 heterodimer and to be responsible for the nuclear transport of the complex.17, 18 We thus investigated whether Pol interferes with the interaction between importin-α5 and activated STATs. As shown in Fig. 5A, STAT1 and STAT2 were clearly detected in the importin-α5 immunoprecipitation 上海皓元医药股份有限公司 complex when IFN-α was added, however, the STATs decreased in a dose-dependent manner, with increased expression of Pol. A similar inhibition was observed using the HepAD38 model (Supporting Fig. 5C). Moreover, impaired colocalization of STAT2 and importin-α5 was observed in HepG2.215 cells compared with that in HepG2 cells by immunofluorescence

(Fig. 5B). To investigate whether Pol directly interacts with importin-α5, GST pull-down assays were conducted, and Flag-Pol was pulled down by GST–importin-α5 (Fig. 5C). Furthermore, colocalization of Pol and importin-α5 in the cytoplasm was detected (Fig. 6D). The C-terminal arm repeats 8 and 9 of importin-α5 have been reported to form a unique binding site for activated STAT1-STAT2.19 Thus, we aimed to determine whether Pol binds to this region of importin-α5. Hemagglutinin-tagged full-length importin-α5 and several truncated constructs were transfected along with Flag-Pol, and the co-IP results showed that Pol was able to coprecipitate with all the truncations except importin-α5-1-406 (Fig. 5D), implying that Pol binds to importin-α5 through a region (407-504) that is also required for the importin-α5-STAT1/2 interaction.

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