Table

Table 3. Optimal conditions for culturing Drosophila tissues during imaging

Tissue Optimized culture conditions Notesa
Early- to mid-stage egg chambers dissected from well-fed females Halocarbon oil (series 95) Avoids dehydration/hypoxia
Early stages: problem of activation and loss of MT organization in aqueous media
Oil has higher RI than water
Good environment for injection
Late-stage egg chambers dissected from well-fed females Grace’s medium (Sigma) Provides ionic and osmotic balance and nutrients
Late stages not susceptible to problems of early stages
Embryos, dechorionated and dehydrated Halocarbon oil (series 700) RI similar to glycerol
Halocarbon oil prevents excess dehydration while avoiding hypoxia (which causes changes to the cell cycle)
Good environment for injection
Halocarbon oil with breathable Teflon membrane Better dehydration prevention for long-term development studies
Better bright-field imaging
Can help squash specimen for greater optical clarity (reduced spherical aberration)
Aqueous medium Can use WI objectives, which have longer working distance with high NA
Spread macrophages from third instar larvae Culture-slide-mounted coverslips treated with ConA in a humidified overchamber Inverted microscope, 100X 1.4-NA oil objective
Six-well tissue-culture plate Upright microscope, 60X 0.9-NA dipping objective
Schneider’s insect medium with 5% FCSb
Neuronal cell cultures from larval brains, overnight culture Dissociation by enzyme cocktail (Kraft et al. 1998) Inverted microscope, 100X 1.4-NA oil objective
Schneider’s insect medium with 5% FCS
Coverslips treated with ConA (16 μg/mL) and laminin (5 μg/mL)
Whole larval fillet Schneider’s insect medium with 5% FCS Upright microscope, 60X 0.9-NA dipping objective
Sylgard mounting chamber
aAbbreviations: MT: microtubule; RI: refractive index; WI: water immersion; FCS: fetal calf serum; NA: numerical aperture.
bFrom Sigma-Aldrich.
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  1. doi:10.1101/pdb.tab3top75 Cold Spring Harb Protoc 2010: pdb.tab3top75-

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