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Cation binding sites on synaptic vesicles
Authors:W Hoss  K Okumura  M Formaniak  R Tanaka
Institution:1. Center for Brain Research, University of Rochester School of Medicine and Dentistry, Rochester, New York 14642 USA;2. Department of Biochemistry, Nagoya City University School of Medicine, Nagoya 467, Japan
Abstract:The protein-sensitized fluorescence of Tb3+ was used as a probe for cation binding sites on synaptic vesicles. Competition studies show that the order of affinity for the sites is Cu2+ > Mn2+ > Ca2+ > Mg2+ and Zn2+ is inactive. Fluorescence quenching studies indicate that the site is superficial and the effect of pH suggests that histidine is involved in the binding. Measurements of enzyme activities in the presence of lanthanides reveal that the metal binding site identified by Tb3+ fluorescence is not the Cu2+ site associated with dopamine-β-hydroxylase. Terbium inhibits Ca2+-stimulated ATPase but not Mg2+-stimulated ATPase activities of the synaptic vesicle fraction. A kinetic analysis indicates that the site monitored by Tb3+ fluorescence may be a component of the Ca2+-stimulated ATPase. It is also suggested that Mg2+ and especially Cu2+ may bind to the sites in vivo, serving as a bridge between vesicles and other synaptic components such as the presynaptic plasma membrane.
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