- Home
- Protocols
-
Download PDF
Ask a
question
Favorite
Small plates.
Age synchronize animals.
Fresh OP50.
Kimwipes.
Timer.
Video equipment, if needed.
Assay plates were prepared by spreading the E. coli strain OP50-1 in a ring on NGM agar (Brenner 1974) in 5 cm petri plates.
Assay plates were always freshly spread with bacteria, incubated overnight at 37°C, and allowed to cool to room temperature before use.
Plates for measuring locomotory rate in the absence of bacteria were also incubated at 37°C. Only synchronized young adult hermaphrodites (16 h after the late L4 larval stage) were tested.
In all cases, plates were coded so that the experimenter was blind to the genotype.
For well-fed animals, locomotory rate was measured by removing 5 animals from plates with ample bacteria, washing the animals twice in S basal buffer (Brenner 1974), and transferring them to an assay plate in a drop of buffer using a capillary pipette.
The drop of buffer used to transfer the animals was absorbed with a Kimwipe.
Five minutes after transfer, the number of body bends in 20 s intervals was sequentially counted for each of the 5 animals on the assay plate and then repeated the same thing for next set of animals in a different assay plate.
Sawin E. R., Ranganathan R. & Horvitz H. R. C. elegans locomotory rate is modulated by the environment through a dopaminergic pathway and by experience through a serotonergic pathway. Cell press 26: 619-631 (2000).
Brenner S. The genetics of Caenorhabtiditis elegans. Genetics 77: 71-94 (1974).
Do you have any questions about this protocol?
Post your question to gather feedback from the community. We will also invite the authors of this article to respond.
Post a Question
