In previously study, we have reported a primary pulmonary cell cultures. In this culture system, the stem/progenitor cells (Oct-4+/SSEA-1+/Sca-1+ and CCSP+) could proliferate and maintain in undifferentiated stage and formed individual colonies with surrounding stromal cells. When the stem/progenitor cells were plucked away from the primary cultures without stromal cells, and transferred to a new culture dishes, the transferred cells were differentiated into type-2 and then type -1 pneumocytes in a sequential fashion. This result suggested that the stromal cells were important for the growth and maintenance the pulmonary stem/progenitor cells in the primary cultures. The aim was to determine the interaction between the stem/progenitor cells and stromal cells. We adopted a proteomic analysis to identify the key factors which regulated the growth of the cells in the culture. Proteomic profiling reveals that colony cells and their neighboring niche cells, stromal cells, produce a number of cytokines and growth factors. We found that stromal cells secrete cytokine BLC, LIX and MCP-1 while colony cells expressed receptor CXCR5, CXCR2 and CCR2. Addition of BLC, LIX and MCP1 could enhance the expression of Oct-4, Sox2 and Nanog in colony cells. Except the paracrine regulation, the autocrine regulation may also play some role. The pulmonary stem/progenitor cells expressed the pluripotency markers of embryonic stem cells, include the Oct-4 and Sox2.They may have potential to become to embryonic-like stem cells after appropriate induction. We also want to evaluate the stemness of the stem/progenitor cells by in vivo assay.