114 A Highly Sensitive and Specific Universal Mirna Profiling Method

helminthic infections, and allergy. They are closely associated with recruiting and amplifying T helper 2 (Th2) lymphocyte response in contrast to Th1asscoiated CAMs. Wide donor-to-donor variability of human primary monocytes and their limited life span in vitro is a current impediment to investigating human AAM biology and their contribution to enhancing Th2mediated pathologic inflammation found in asthmatic lungs. Methods: Using the human promonocytic cell line, THP1, we have successfully established a THP1-derived and committed CAM and AAM populations demonstrating typical macrophage-oriented morphological characteristics. Results: Quantitative PCR and ELISA demonstrated that THP1-AAM cell model express classic pathogen neutralizing dectin receptors such as scavenger type mannose receptor (MRC1) and Th2-associated signature chemokines including CCL13, 17, 18 and 22, and are tolerant to TLR4 challenge by LPS treatment in contrast to THP1-CAM which expressed an LPS enhanced expression of pro-inflammatory mediators such as TNF-a, CXCL10 and -11. Furthermore, THP1-AAM cell model expressed 50to 100-fold lower expression IFN-alpha 4, IFN-beta, and IFN-lambda1 compared to THP1-CAM. Quantitative PCR array revealed that a select group of interferon regulatory factors (IRFs), antiviral genes such as Mx1, and interferon stimulated genes such as ISG15 are down-regulated only in THP-1 AAM cell model upon differentiation or LPS treatment emphasizing its classic infection tolerant phenotype. In addition, IRF4 was found to be upregulated only in the THP1-AAM model which may point towards its critical role in orchestrating the macrophage lineage commitment towards an alternatively activated phenotype as well as governing its unique cytokine and chemokines expression profile. Conclusions: Compared to the donor variability of primary human monocytes, establishing THP1-AAM and CAM cell models will enable a more rapid and efficient investigation of a spectrum of molecular mechanisms governing innate, classic, and alternative phenotypes in macrophage populations and their role in pathologic processes, in particular allergic inflammation of the upper airways.