6 Despite their highly specialized microvascular differentiation, LSECs retain a remarkable phenotypic and functional plasticity. In liver cirrhosis, for example, endothelial plasticity results in morphological transdifferentiation
of LSEC, collectively termed sinusoidal “capillarization.” Unfortunately, not much is known about the mechanisms that Y-27632 control regular LSEC differentiation and LSEC transdifferentiation during pathogenic processes. LSEC-hepatocyte interactions have been recognized to be of special importance due to unidirectional cytokine crosstalk between LSEC and hepatocytes mediated by hepatocyte growth factor (HGF) and vice versa between hepatocytes and LSEC by way of EG-VEGF.7 Recently, we have been able to show that LSEC-derived Wnt2 acts as a cell type-specific autocrine growth factor in LSEC cross-stimulating the VEGF pathway.8 A major setback in deciphering LSEC-specific differentiation is the Cilomilast datasheet fact that LSECs are not amenable to long-term cultures in vitro. LSECs rapidly lose their characteristic morphology as well as some of their specialized functions in culture. Hitherto, attempts to improve LSEC culture conditions have had limited success,9, 10 indicating that a better understanding of the molecular programs underlying
LSEC-specific differentiation in vivo and dedifferentiation in vitro is urgently needed. Dedifferentiation of EC in culture is not unique to LSEC. Both blood vascular as well as lymphatic microvascular EC undergo marked transdifferentiation over time upon culture.11 High endothelial venule endothelial cells (HEVEC) from tonsil are a striking example of highly specialized ECs
that lose their specific gene signature as soon as 48 hours after isolation.12 Thus, even short-term cultures of primary EC do not adequately mimic the respective differentiated EC phenotypes in situ. These results suggest that organ-specific EC differentiation and function is maintained by the respective tissue microenvironments. For a comprehensive analysis of the molecular programs mediating LSEC-specific differentiation, we chose a similar, two-sided, MCE公司 comparative gene expression profiling approach. Selection of the genes that were both overexpressed in LSEC in comparison to LMEC and down-regulated in LSEC upon short-term cultivation resulted in identification of an LSEC-specific gene signature including genes in several functional categories. Among these molecules, liver endothelial differentiation-associated protein (Leda)-1 was identified as a novel homolog of adherens junction-associated protein-1 (Ajap-1/Shrew-1) involved in cell adhesion and polarity.13, 14 This LSEC-specific gene signature may comprehensively determine the special functional program of liver sinusoidal endothelium.