“…Thus we used it to study the synthesis, assembly, and sealing of tight junctions (TJs) (69,74,75,78,145,183,297), as well as the polarity of Na ϩ -K ϩ -ATPase (61,62,96,102); Enrique Rodriguez-Boulan introduced the use of viruses that bud either apically (e.g., Flu) or basolateraly (e.g., stomatitis) to track the fate of specific proteins during apical or basolateral polarity (283, 284, 379 -382), and Carlos A. Rabito analyzed the onset of polarized cotransporters (368,370,371). M. Taub perfected the approach by developing totally defined culture media (440 -442), and complementary procedures were refined to open and reseal the TJs by removing and restoring Ca 2ϩ (69,97,101,184,186), follow the cascades of phosphorylation involved (20,21,85), the role of the cytoskeleton (311, 312), the participation of protein synthesis and sorting (196,376,379,381), the polarized distribution of ion channels (317,359,360,361,421,439), the involvement of E-cadherin (199 -201), the effect of agents that induce differentiation (280), and the vectorial movement of receptors (302). A distinct advantage of cultured monolayers is derived from the possibility of labeling beforehand a given cell type, and then mixing them with other types from different epithelia and even different animal species (98,…”