In the visual system of arthropods histamine (HA) is the neurotransmitter for stimulus transmission from retina photoreceptor neurons to downstream postsynaptic neurons. We propose a recycling pathway for this neurotransmitter in Drosophila melanogaster (D. melanogaster) in which the two enzymes Ebony and Tan together with yet to be identified transporters hold key functions: HA from the synaptic cleft is fused to β-alanine by Ebony in the surrounding epithelial glia for inactivation. After transfer into photoreceptor neurons, β-alanyl-histamine or carcinine (CA) is hydrolyzed by Tan thereby replenishing the HA pool for vesicle loading. This working model strongly depends among others on the cata-lytic efficiency of Ebony. To verify the proposed recycling pathway with a key function of Ebony in neurotransmitter inactivation, it is essential to determine its reaction kinetics. Furthermore, enzyme structure will be solved to understand how specific recruitment of β-alanine and peptide bond formation can be performed in concert with fast HA transport into epithelial glia. As a prerequisite new expression systems and purification strategies will be employed that overcome the hitherto limited capability in preparing pure and active Ebony protein.

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