Table 1:
Troubleshooting of procedure.
| Step | Problem | Cause | Suggestion |
| 1.2. | Failure of trypsinisation | Inhibitory FBS in residual media | Ensure entire media is washed away with HBSS before trypsin |
| 2.1. | DMSO pools at centre of well & is toxic to the cells located at center | Dense DMSO sits at center of well when added directly to well | Add DMSO(-solubilized drugs) to media in tube, mix and add media/DMSO mixture to well |
| 2.5. | Loss of formazan | Insoluble formazan crystals lost in MTT | Do not agitate plate or disturb formazan when removing MTT |
| 3.3./13.2. | Hyper-exposed calcein-AM staining | Incubation of live cells with calcein-AM > 2 h | Ensure calcein-AM stained cells are imaged in < 2 h |
| 3.5. | Underestimation of neurite length | Gridlines with too large distance between lines | T of 25 µm is recommended for SH-SY5Y cell neurite analysis |
| 4./9./14. | Poor cell survival following transfection | Excessive time taken for electroporation protocol | Perform electroporation protocol in > 30 min |
| 4./9./14. | Poor transfection efficiency & survival | Transfection protocol not optimized | See ‘Transfection of Cultured Neural Cells Optimization’ |
| 5./10. | Low protein yield | Excessive lysate dilution | Use 150 µl lysis buffer per well |
| 5./10. | Absence of activated signaling pathway(s) | Phosphorylation of proteins lost | Use phosphatase inhibitors in lysis buffer |
| 6.3. | Meninges on VM tissue | Inefficient removal of meninges from VM | Peel VM tissue from meninges. Do not attempt to cut meninges |
| 7.4. | Unanalysable/misplaced neurons at edge of well | 50 µl of plated cells spills to edges of well | Ensure 50 µl of plated cells remains at center of well |
| 8.3./13.3. | Underestimation of neurite length | Gridlines with too large distance between lines | T of 50 µm is recommended for primary neuron growth analysis |
| 9.4. | GFP-positive cells lost | Fixing can quench GFP | Use anti-GFP antibody |
| 11.5. | Wrong ganglia dissected for cell culture | SCG & nodose ganglia similar & close together | SCG is distinctly larger than nodose ganglion |
| 11.6. | Loss of dissected SCG | ‘Sticky’ SCG stuck in pipettes &/or tubes | Use unplugged Pasteur pipette that can wash out with trypsin |
| 3./4./8./9./13./14. | Incorrect visualization of target neurons | Inappropriate labeling/identification of neurons | See ‘Visualization of Cultured Neural Cells’ |