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Membrane lipids bacterial toxins, interactions with

G-protein a-subunits also possess specific residues that can be covalently modified by bacterial toxins. Cholera toxin catalyzes the transfer of ADP-ribose moiety of NAD to a specific arginine residue in certain a-subunits, whereas pertussis toxin ADP-ribosylates those a-subunits that contain a specific cysteine residue near the carboxy-terminus. Modification of the a-subunit by cholera toxin persistently activates these protein by inhibiting their GTPase activity, whereas pertussis toxin inactives Gia protein and thereby results in the uncoupling of receptor from the effector. G-protein a-subunits are regulated by covalent modifications by fatty acids myristate and palmate. These lipid modifications serve to anchor the subunits to the membrane and increase the interaction with other protein and also increase the affinity of the a-subunit for 3y. In this regard, the myristoylation of Gia is required for adenylyl cyclase inhibition in cell-free assay (Taussig et al. 1993). [Pg.6]

Fig. 1 Protein-carbohydrate interactions at the cell surface mediating cell-cell binding, cell-microbe (bacterial, viral, and bacterial toxin) adhesion and cell-antibody binding. The sugar chains can be linked to proteins (ribbons) or anchored in the plasma membrane via a lipid. Reprinted from [6] with permission. Copyright 2005, Macmillan Publishers Ltd... Fig. 1 Protein-carbohydrate interactions at the cell surface mediating cell-cell binding, cell-microbe (bacterial, viral, and bacterial toxin) adhesion and cell-antibody binding. The sugar chains can be linked to proteins (ribbons) or anchored in the plasma membrane via a lipid. Reprinted from [6] with permission. Copyright 2005, Macmillan Publishers Ltd...

See other pages where Membrane lipids bacterial toxins, interactions with is mentioned: [Pg.79]    [Pg.238]    [Pg.190]    [Pg.281]    [Pg.150]    [Pg.241]    [Pg.259]    [Pg.328]    [Pg.338]    [Pg.586]    [Pg.2125]   
See also in sourсe #XX -- [ Pg.150 ]




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