Drosophila Nervous System Dissection and Dye-Injection

The procedure for adult Drosophila nervous system dissection and subsequent dye-injection has been previously described in detail [55 (link), 56 (link)]. To visualize the morphology of the GF-TTMn connection either a 10 mM Alexa Fluor 555 Hydrazide (Molecular Probes) in 200 mM KCl or a dye solution of 10% w/v neurobiotin (Vector Labs) and tetramethylrhodamine isothiocyanate (TRITC)-dextran (Invitrogen) in 2 M potassium acetate was injected into the GF axons by passing hyperpolarizing or depolarizing current, respectively. Preparation of GF samples for confocal microscopy has been described previously [55 (link), 56 (link)]. The following antibodies and concentrations were used: Streptavidine-Cy3 conjugate (Jackson; 1:750 dilution), BP104 (Developmental Studies Hybridoma Bank, 1:50 dilution), goat anti-mouse-Cy2 and Cy5 (Jackson ImmunoResearch, 1:500 dilution), anti-GFP A11122 (Invitrogen, 1:500 dilution). Samples were scanned at a resolution of 1024x1024 pixels, 2.5x zoom, and 0.5 μm step size with a Nikon C1si Fast Spectral Confocal system using a 60×/1.4 NA oil immersion objective lens. Images were processed using Nikon Elements Advance Research 4.4 and Adobe Photosuite CS5 software.

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Kudumala S.R., Penserga T., Börner J., Slipchuk O., Kakad P., Lee L.H., Qureshi A., Pielage J, & Godenschwege T.A. (2017). Lissencephaly-1 dependent axonal retrograde transport of L1-type CAM Neuroglian in the adult drosophila central nervous system. PLoS ONE, 12(8), e0183605.

Publication 2017

neurobiotin BP104 anti-GFP A11122 C1si Fast Spectral Confocal system

Adult Alexa fluor 555 Antibodies Axons Confocal microscopy Dilution Dissection Drosophila Goat Hybridoma Hydrazide Immersion Isothiocyanate Lens Molecular probes Mouse Nervous system Neurobiotin Potassium acetate Tetramethylrhodamine dextran Vector

Corresponding Organization : Florida Atlantic University

Other organizations : University of Kaiserslautern

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Variable analysis

independent variables

Type of dye injected into GF axons (Alexa Fluor 555 Hydrazide or neurobiotin + TRITC-dextran)

dependent variables

Morphology of the GF-TTMn connection

control variables

Concentration of dyes (10 mM Alexa Fluor 555 Hydrazide or 10% w/v neurobiotin + TRITC-dextran)
Injection method (passing hyperpolarizing or depolarizing current)
Preparation of GF samples for confocal microscopy
Antibodies and their concentrations used for immunostaining (Streptavidine-Cy3, BP104, goat anti-mouse-Cy2 and Cy5, anti-GFP A11122)
Confocal microscopy settings (resolution, zoom, step size, objective lens)

controls

Positive control: None specified
Negative control: None specified

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