Neurotransmitter uptake of synaptic vesicles studied by X-ray diffraction

Komorowski, Karlo; Preobraschenski, Julia; Ganzella, Marcelo; Alfken, Jette; Neuhaus, Charlotte; Jahn, Reinhard; Salditt, Tim

doi:10.1007/s00249-022-01609-w

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Neurotransmitter uptake of synaptic vesicles studied by X-ray diffraction

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Preobraschenski, Julia
Emeritus Group Laboratory of Neurobiology, Max Planck Institute for Multidisciplinary Sciences, Max Planck Society;

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Ganzella, Marcelo
Emeritus Group Laboratory of Neurobiology, Max Planck Institute for Multidisciplinary Sciences, Max Planck Society;

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Jahn, Reinhard
Emeritus Group Laboratory of Neurobiology, Max Planck Institute for Multidisciplinary Sciences, Max Planck Society;

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Citation

Komorowski, K., Preobraschenski, J., Ganzella, M., Alfken, J., Neuhaus, C., Jahn, R., et al. (2022). Neurotransmitter uptake of synaptic vesicles studied by X-ray diffraction. European Biophysics Journal, 51, 465-482. doi:10.1007/s00249-022-01609-w.

Cite as: https://hdl.handle.net/21.11116/0000-000B-7BA2-4

Abstract

The size, polydispersity, and electron density profile of synaptic vesicles (SVs) can be studied by small-angle X-ray scattering (SAXS), i.e. by X-ray diffraction from purified SV suspensions in solution. Here we show that size and shape transformations, as they appear in the functional context of these important synaptic organelles, can also be monitored by SAXS. In particular, we have investigated the active uptake of neurotransmitters, and find a mean vesicle radius increase of about 12% after the uptake of glutamate, which indicates an unusually large extensibility of the vesicle surface, likely to be accompanied by conformational changes of membrane proteins and rearrangements of the bilayer. Changes in the electron density profile (EDP) give first indications for such a rearrangement. Details of the protein structure are screened, however, by SVs polydispersity. To overcome the limitations of large ensemble averages and heterogeneous structures, we therefore propose serial X-ray diffraction by single free electron laser pulses. Using simulated data for realistic parameters, we show that this is in principle feasible, and that even spatial distances between vesicle proteins could be assessed by this approach.