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Fig. 4

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ZDB-IMAGE-200501-41
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Figures for Zhang et al., 2020
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Figure Caption

Fig. 4 Dram1 deficiency does not affect the capability of macrophages to phagocytose Mm.

a Representative stereo micrographs of macrophages in the whole tail region and quantification of the number of macrophages in this region. 3 dpf dram1∆19n/∆19n and dram1+/+/ mpeg1:mCherryF larvae were obtained from incrossed dram1+/∆19n animals and the number of macrophages for each larva were counted before determining the genotype. Genotyping was performed by PCR and Sanger sequencing (≥28 larvae/group). Data are accumulated from two independent experiments and represented by scatter and boxplots as detailed in the “Methods” section. ns non-significant, *p < 0.05,**p < 0.01,***p < 0.001. b Representative stereo images of the whole tail of 3 dpf dram1∆19n/∆19n and dram1+/+ larvae following an immunohistochemical peroxidase activity detection protocol. The number of neutrophils in this region was quantified per individual larva (≥18 larvae/group). Data are accumulated from two independent experiments and represented by scatter and boxplots as detailed in the “Methods” section. ns non-significant, *p < 0.05,**p < 0.01,***p < 0.001. c Representative confocal micrographs of macrophages located in the blood circulation over the yolk sac of infected dram1∆19n/∆19n and dram1+/+ embryos in mpeg1:mCherryF background at 1 h post-infection (hpi). Scale bars, 10 μm. Quantification of phagocytosis of Mm by macrophages at 1 hpi. dram1∆19n/∆19n and dram1+/+ embryos in mpeg1:mCherryF background were infected with Mm at 30 hpf and fixed at 1 hpi. The percentage of macrophages having phagocytosed Mm clusters was determined per individual larva (≥16 larvae/ group). Results are accumulated from two independent experiments and represented by scatter and boxplots as detailed in the “Methods” section. ns non-significant, *p < 0.05,**p < 0.01,***p < 0.001.

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Acknowledgments
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