Formicis: A Study In Behavioral Componentry

The Formicis Project translates the natural structure-building phenomena of ant-bridges into architectural componentry that intuitively self-aggregates into goal-oriented structures.

Ultraviolet radiation sensitivity of proliferating and differentiated human neuroblastoma cells

The effects of ultraviolet (U.V.) radiation were studied on a cloned line of human neuroblastoma cells in proliferative and differentiated growth modes, the latter being induced by serum deprivation. The neuroblastoma cells were found to be unusually sensitive in comparison with HeLa cells when survival was measured by colony formation in soft agar, the differentiated mode being the most sensitive. Ultraviolet radiation sensitivity was associated with very low DNA repair capacity as measured by DNA repair synthesis and by removal of M. luteus endonuclease-sensitive sites from irradiated DNA. The greater sensitivity of the differentiated cells appeared to be related to a greater degree of DNA damage at a given U.V. dose, resulting from altered cell geometry in the growth mode. The neuroblastoma cells showed little or no post-irradiation inhibition of DNA replication at low U.V. doses, suggesting that it is the repair process rather than the DNA damage which is responsible for inhibiting replication

Heterologous expression and topography of the main intrinsic protein (MIP) from rat lens

AbstractWild type rat lens main intrinsic protein (MIP) and MIP mutated (F73I, F75L) to resemble the glycerol facilitator of Escherichia coli in the region of the NPA1 box were used to investigate the topology of MIP in the membrane of Spodoptera frugiperda (Sf21) cells using the baculovirus expression system and expression in mouse erythroid leukaemia cells (MEL C88). Differential fixation for staining was used, with paraformaldehyde for externally exposed antigenic sites, and acetone for both externally and internally exposed protein antigenic sites. Immunofluorescence using antibodies to synthetic MIP peptides showed that wild type MIP had a six transmembrane topography. The N- and C-termini were intracellular in both expression systems, and both NPA boxes were found to be extracellular. These results show that residues around the NPA1 box can influence the folding of the MIP in the membrane, and provide structural evidence for the poor water transport properties of MIP, as the NPA boxes lie outside the plane of the membrane