Demonstration of an ATPase at the cell surface of intact normal and neoplastic human cells in culture

An ATPase reaction has been studied at the surface of intact normal and neoplastic human cells in culture. For this purpose a sensitive method has been developed which permits repeated monitoring of enzyme activity without interference with cellular viability. Experiments could be performed with the cells cultured in a single dish. The cells were firmly attached to the supporting medium throughout the experiment. The incubation medium could easily be separated from the cells at the end of the reaction. There was no diffusion of the surface-located ATPase into the incubation medium. Another advantage was the possibility of microscopic control of the appearance of the cells during the reaction. High ATPase activity was found in glia-like cells derived from normal adult brain cells while lines from gliomas had very low activity. One SV40 transformed glia line had an extremely low ATPase activity in contrast to the uninfected cells. Normal fibroblasts and sarcoma cells had about the same low activity as the glioma cells.     

Homoserine kinase from Escherichia coli K-12: properties, inhibition by L-threonine, and regulation of biosynthesis

We have partially purified homoserine kinase from a genetically derepressed strain of Escherichia coli K-12. The optimum pH of the enzyme-substrate reaction was 7.8 and the K(m) values for l-homoserine and adenosine 5'-triphosphate were both 3 x 10(-4) M. K(+) (or NH(4) (+)) as well as Mg(2+) were required for its activity. The sedimentation coefficient determined by ultracentrifugation in a sucrose density gradient was 5.0 +/- 0.25S. l-Homoserine was an excellent protector against heat inactivation of homoserine kinase. l-Threonine was a competitive inhibitor of homoserine kinase, suggesting that end-product inhibition of this enzyme plays a role in vivo in the overall regulation of threonine biosynthesis. The specific activity of aspartokinase I-homoserine dehydrogenase I and of homoserine kinase showed a strong positive correlation in extracts from strains under widely varying conditions of genetic or physiological derepression; it was concluded that these two enzymes are coordinately regulated in E. coli K-12.