Fluorescence Imaging of Worms

Worms tagged with fluorescence were imaged under DIC and fluorescence using an Axio Imager M2 microscope (ZEISS). Images were processed and viewed using ZEN 2 pro software (ZEISS). An Immersol 518F oil (Zeiss) was used. All the images were captured at 20°C (Gan et al., 2019 (link)).
Time-lapse imaging of HIS-24::mCherry in N2 and trim-21 mutants was performed at 20°C under a ×100 oil objective using an Axio Imager M2 microscope (ZEISS). Images were focused on specific corpses and were taken every few minutes until the corpses disappeared.

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Yuan L., Li P., Jing H., Zheng Q, & Xiao H. (2022). trim-21 promotes proteasomal degradation of CED-1 for apoptotic cell clearance in C. elegans. eLife, 11, e76436.

Publication 2022

Axio Imager M2 microscope ZEN 2 pro software Immersol 518F oil

Corpses Fluorescence Microscope Worms

Corresponding Organization :

Other organizations : Shaanxi Normal University

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Variable analysis

independent variables

Genotype (N2 and trim-21 mutants)

dependent variables

Localization and dynamics of HIS-24::mCherry in cell corpses

control variables

Temperature (20°C)
Microscope (Axio Imager M2, ZEISS)
Objective (×100 oil)
Imaging medium (Immersol 518F oil, Zeiss)

controls

Positive control: N2 strain (wild-type)
Negative control: trim-21 mutant strain

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