PB2 is a component of influenza A RNA polymerase complex and has been shown to play an important role in influenza A viral transcription and replication. To study the role of PB2 involved in influenza A viral replication, we set to fish out cellular factors that interact with PB2 by using yeast two-hybrid system. We found that eight cellular proteins could interact with PB2 C-terminal region. Among them, HAX-1 was confirmed to interact with PB2 by co-immunoprecipitation and GST pull-down assays. HAX-1, a multifunction protein, has been shown to have an anti-apoptotic function and play roles in regulating mRNA transport. To study the role of HAX-1 in influenza A viral replication, HAX-1 knock-down H1299 cells were established by using lentivirus expressing shRNA against HAX-1. We found that influenza A viral production was significantly increased in HAX-1 knock-down cells, indicating that HAX1 plays an inhibitory role in influenza A viral replication. To study the mechanism underlying HAX-1 inhibition of influenza A replication, we transfected PB2-Flag alone, HA-HAX-1 alone, or PB2-Flag + HA-HAX-1 into 293FT cells and detected the location of PB2-Flag and HA-HAX-1 by confocal microscope. HA-HAX-1 localized in the cytoplasm in the absence of PB2. This data is consistent with the previous reports that HAX-1 mainly localized in the mitochondria. Interestingly, when HA-HAX-1 was co-expressed with PB2-Flag, a protein known to localize in the nucleus, a significant proportion of HA-HAX-1 was found in the nucleus. These data indicate that PB2 may translocate HAX-1 into nucleus by interacting with the latter. The significance of this finding and how PB2 interaction with HAX-1 may facilitate influenza A viral production is discussed.