Expression of sli^UAS.cBa under the control of Scer\GAL4^ey-OK107 does not lead to any changes in the development of the optic lobes when compared to controls.

Expression of sli^Scer\UAS.cBa in myocardial cells, driven by Scer\GAL4^tin.CΔ4, does not produce significant cardiac alignment defects. Pan-mesodermal expression of this transgene, driven by both Scer\GAL4^how-24B and Scer\GAL4^twi.PG, produces cardiac alignment defects with low penetrance. In contrast, sli^Scer\UAS.cBa expression in pericardial cells, driven by Scer\GAL4^eve.eme, results in frequent alignment defects.

Embryos expressing sli^Scer\UAS.cBa under the control of Scer\GAL4^tracheal generally have normal dorsal sensory neuron morphology.

When expression of sli^Scer\UAS.cBa is driven by Scer\GAL4^sli.PS, Scer\GAL4^elav-C155 or Scer\GAL4^en-e16E the ventral nerve cord is disrupted with interruption of intersegmental connections and displacement of the axon tracts away from the source of sli protein.

When expression is driven by Scer\GAL4^sim.P3.7 in an otherwise wild type background, fewer than the normal number of axons cross the midline. Longitudinal tracts are thicker within segments and thinner between segments than normal. The position of the SP1 neuron is irregular. When expression is driven by Scer\GAL4^sli.PS, defasciculation of commissural tracts occurs, some commissures are missing and ectopic lateral axon extension occurs. Expression driven by Scer\GAL4^en-e16E results in breaks in the longitudinal tracts, including the MP fascicle and the later-forming SP1 fascicle. Axons inappropriately cross the midline. Expression driven by Scer\GAL4^sca-537.4 results in a reduction in the number of axons traversing the segment boundary in the longitudinal tracts, thinning and delaying development of fascicles.