Fig. S8

Bifunctional compounds do not enhance phagocytosis of conidia by

wild-type zebrafish neutrophils.

A) Diagram of a 72 hpf zebrafish larva indicating the site of inoculation and the site of

analysis (i). (ii) Collapsed z-stack (maximum intensity) representative image showing

conidia (blue, Hoechst) and neutrophils (green, GFP) in the caudal venous plexus of

Tg(mpx:GFP/mpeg1:mCherry) embryos injected with spi1-MO at the one-cell stage

and infected with A. fumigatus conidia at 72 hpi. Scale: 100 μm. iii) highermagnification

of neutrophils and conidia indicating extracellular conidia (open yellow

arrowhead) and examples of phagocytosis by neutrophils (filled yellow arrowheads).

Scale: 20 μm.

B) Graph shows neutrophil (N) and macrophage (M) counts in each caudal venous plexus

field of view (FOV) for spi1-MO morphant larvae injected with treated and control

conidia.

C) Graph shows conidia counts per FOV for each treatment group.

D) Graph shows the percent of neutrophils containing conidia at 2 hpi for each treatment

group.

E) Graph shows the number of phagocytosed conidia per FOV at 2 hpi for each treatment

group. Each point represents an infected larva.