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Deltavision core deconvolution imaging system

Manufactured by Cytiva

The DeltaVision Core is a deconvolution imaging system designed for high-resolution microscopy. It utilizes a unique optical design and advanced image processing algorithms to enhance image quality and resolution. The system is capable of capturing and processing images with a high level of detail and clarity.

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2 protocols using deltavision core deconvolution imaging system

1

Microscopic Imaging of C. elegans Neurons

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Animals were immobilized with 10–100 mM sodium azide dissolved in M9, depending on developmental stage, mounted on a 2% agarose pad, and covered with a No. 1.5 coverslip. Spherical aberration was minimized using immersion oil matching. Z-stacks were acquired using a DeltaVision Core deconvolution imaging system (Applied Precision) with the InsightSSI light source; UApo 40×/1.35 NA oil immersion objective, PlanApo 60×/1.42 NA oil immersion objective, or UPlanSApo 100×/1.40 NA oil immersion objective (Olympus); the standard DeltaVision live cell excitation and emission filter set; and a Photometrics CoolSnap HQ2 CCD camera (Roper Scientific). Images were acquired and deconvolved with Softworx 5.5 (Applied Precision). Images are displayed as maximum intensity projections generated in Priism [32 (link)]. Images were pseudocolored and image brightness was linearly adjusted using Adobe Photoshop. IL2 dendrite lengths were measured using the Segmented Line tool in Fiji (NIH) [33 (link)]. To control for differences in head size, dendrite lengths are normalized to the distance from the cell body to the nose tip. p-values were generated using the Wilcoxon Rank-Sum (Mann-Whitney U) test in RStudio and adjusted using the Bonferroni correction.
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2

Imaging Caenorhabditis elegans Embryos and Larvae

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Animals were prepared for imaging by mounting on a 2% agarose pad with a #1.5 coverslip. Larval animals were immobilized with sodium azide, young embryos (prior to twitching, ~1.5-fold) were simply imaged live, and older embryos were arrested to prevent movement as described in Cebul, McLachlan, and Heiman, 2020 (link). Early-stage embryos were acquired by dissecting adult hermaphrodites.
Image stacks were collected on a DeltaVision Core deconvolution imaging system (Applied Precision) with the InsightSSI light source; UApo 40×/1.35 NA oil immersion objective, PlanApo 60×/1.42 NA oil immersion objective or UPlanSApo 100×/1.40 NA oil immersion objective (Olympus); the standard DeltaVision live cell excitation and emission filter set; and a Photometrics CoolSnap HQ2 CCD camera (Roper Scientific). Image stacks were acquired and deconvolved with Softworx 5.5 (Applied Precision).
Representative images were generated as follows: Maximum intensity projections were created from contiguous optical sections in Fiji, then linearly adjusted for brightness in Adobe Photoshop. Multicolored images were generated by placing each channel in a separate false-colored screen layer in Photoshop. Adobe Illustrator was used to assemble final images.
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