C. elegans Movement Tracking: A Method to Assess Locomotion in Worms

Overview

This video describes the use of video and tracking software to record worm movement in an arena.  The example protocol measures the effect of ethanol exposure on worm locomotion.

Protocol

The following protocol is an excerpt from Davies et al, An Assay for Measuring the Effects of Ethanol on the Locomotion Speed of Caenorhabditis elegans, J. Vis. Exp. (2015).

1. Steps to Perform on the Day before the Assay

   1. Pick L4 stage worms to fresh nematode growth medium (NGM) plates seeded with a lawn of OP50 E. coli, and culture them at 20 ˚C O/N. Each assay condition requires 10 worms; pick an excess of worms to allow for O/N loss of worms.
      1. Only assay animals that are first-day adults; many mutants grow at a slower speed than wild type. Adjust the timing of picking for strains that have developmental delays so that all animals tested are first-day adults.
2. Steps to Perform on the Day of the Assay
   1. Preparation for the assay:
      1. Perform assays on standard unseeded 60 x 15 mm NGM plates. Dry all of the plates to be used at 37 ˚C for 2 hr, with lids off. For each experimental trial, use four dried NGM plates; these will be the 0 mM and 400 mM ethanol assay plates and their accompanying acclimation plates.
         NOTE: The use of NGM plates is important here; differences in the composition of the plates, in particular their osmolarity, can strongly affect the dose response of ethanol on behavior, this is due, at least in part, to changes in the amount of ethanol accumulated by the animals. NGM agar is 160 mOsm.
      2. After drying, weigh each of the unseeded NGM plates to be used in the assay and note the weight. Determine the volume of media in the plates based on the weight of an empty plate. To approximate the conversion of weight of the agar to volume, assume that the media weighs the same as an equal volume of water.
         NOTE: Our most consistent results have been found with NGM media that has dehydrated sufficiently that an original 10 ml volume has a post-drying volume between 8.3–8.9 ml. An alternative to the 2 hr dry time is to dry until the plates reach this volume range to account for differences in incubators.
      3. Melt 4 copper rings (inner diameter of 1.6 cm) into the surface of each of the plates to act as corrals for the different genotypes or treatment groups of worms. Grasp each ring with forceps, and heat in a flame (a strong flame from a Bunsen burner works well) for approximately 3 sec. Immediately place the ring on a plate while still holding the ring with the forceps to prevent it from ‘skipping’.
         1. Ensure that the ring rests flat against the surface of the agar by pressing down gently with the forceps at several points on the ring. When placing the ring, be careful to leave room for an additional three rings.
         2. Melt the three additional copper rings into the surface of the plate, taking care to place them as close together as possible so that all four will be in the field of view of the camera.
            NOTE: Making a good seal with the agar is essential to keep the worms in the rings during the assay. Rings that skip around on the plate are unlikely to make the correct seal with the agar and may scar the agar, which allows worms to burrow and interferes with visualizing the worms.
         3. For each assay plate prepare an accompanying “acclimation” plate, which should be dried and unseeded and will receive no ethanol. Place four copper rings on these plates.
      4. Label the bottom of the plates next to each ring with the worm strain to be used in the ring, taking care to not write in the field of view of the ring itself. Match the labels on the assay plate with its accompanying acclimation plate.
      5. Calculate the amount of 100% ethanol to add to each assay plate so that the final concentration is 0 mM or 400 mM ethanol (weight to volume). For each experiment (n = 1), there will be one 0 mM and one 400 mM ethanol plate; acclimation plates do not receive ethanol. Add the ethanol, pipetting it around the surface of the plate. Use laboratory film to seal the plate and allow it to equilibrate on the bench top for 2 hr.
      6. When 1.5 hr has elapsed, begin the acclimation step of the assay, step 2.2.
   2. Perform locomotion assay: Assay plates
      1. Carefully transfer 10 worms of each experimental group to the center of a copper ring on the acclimation plate. Remove any food that is visible on the agar at this point by scraping gently with the worm pick. Vary the order in which the experimental groups are put on the plates across experimental trials so that the same strains are not put on the plates in the same order across trials.
         NOTE: The goal is to transfer the animals to the plate with minimal quantities of food, because if food on the acclimation plate is transferred to the assay plate the worms will aggregate around the food and the effect of the drug on locomotion will be obscured.
      2. Be careful not to break the surface of the agar with the pick, as this will allow the worms to burrow and will disrupt the assay. Incubate the worms at RT for 30 min.
      3. Ensure that there is an appropriate interval between the initiations of each plate. An experienced experimenter can move 40 animals, 10/ring for 4 rings in < 1.5 min, but any interval up to 2 min is acceptable. The standard assay has movies recording at 10-12 min and 30-32 min of exposure for both 0 mM and 400 mM ethanol.
      4. Initiate the acclimation plate for the 0 mM exposure and the acclimation plate for the 400 mM exposure approximately 2 min and 30 sec apart to allow for saving of the first movie file before the second movie must begin.
      5. After the 30-min acclimation period, transfer the worms from the acclimation plates to the assay plates. Transfer the worms to the assay plates (0 mM or 400 mM ethanol) in the same order that they were added to the acclimation plate, keeping track of the timing between the completions of each plate. Seal the plate with laboratory film to minimize loss of ethanol to vaporization.
      6. Use a scooping motion with a thin-edged flattened worm pick to collect worms on top of the flattened pick. Perform the transfer of worms from the unseeded acclimation plate to the assay plate without the use of bacteria, which is commonly used in transferring worms as it helps to glue the worm to the pick.
         NOTE: The speed at which animals are transferred at this step is very important because the first worms on the plate will be exposed to ethanol longer than the last worms added to the plate, and earlier time points may show some time-dependent effects. This is the major reason for rotating which strains are placed on a plate first across experimental replicates.
   3. Perform Locomotion Assay: Filming
      1. Use a microscope/camera combination that allows for simultaneous imaging of all four rings in the field of view (approximately 42x42 mm² square), such as a 0.5x microscope objective, 0.8x magnification and a camera with a 2048x2048 7.4 µm pixel CCD.
      2. Use even illumination across the field of view, which aids in object recognition at the intensity threshold step. A 3”x3” backlight works well.
      3. Image the worms on a plate positioned media-side up (lid down), which generates contrast that is lost when using the backlight compared with a traditional microscope transmitted light source.
      4. Prepare the image analysis software to capture time-lapse movies of the moving worms. Set the software to capture 12-bit gray-scale images every 1 sec, as a 2-min (120 frame) movie. To reduce the size of the output file, while still retaining sufficient image resolution, use a 2x2 binning mode to capture 1024x1024 pixel images.
      5. Record the movies. Begin recording a 120-frame movie of the first plate (0 mM ethanol) 10 min after the last worms were placed on that plate. Save the movie file.
      6. Record the second plate (400 mM ethanol). Repeat this process for both plates beginning 30 min after the last worms were placed on the first plate (0 mM ethanol) to capture the 30–32 min time points for each exposure.
         NOTE: Allow sufficient time to save the image files after each capture session before beginning recording of the next plate to be analyzed.
      7. For future-proofing of archived movies and to allow these movies to be opened and analyzed by other public domain open source imaging software programs, such as ImageJ, convert a copy of each movie to 8-bit 256 gray scale TIFF files.
         NOTE: The image analysis software described here uses a proprietary file format.

Materials

Name	Company	Catalog Number	Comments
C. elegans strains	Caenorhabditis Genetics Center
60 x 15 mm Petri plates, triple vented	Greiner Bio-One	628161	Other plate brands will suffice.
NGM agar	Various		NaCl (3 g/L), agar (17 g/L), peptone (2.5 g/L), 1 ml cholesterol (5 mg/ml in ethanol), 1 ml (1 M) MgSO4, 1 ml (1 M) CaCl2, 25 ml (1 M) KPO4, pH=6, 975 ml H2O
Forceps	Various		e.g., Fisher Scientific #10300
37 °C Incubator	Various		For drying agar
Copper rings	Plumbmaster	STK#35583 (48 cap thread gasket)	1.6 cm inner diameter, 1.8 cm outer diameter copper rings
100% ethanol	Various
Parafilm M	Bemis	PM996
CCD camera	QImaging	RET-4000R-F-M-12	This camera has a large field of view.
Stereomicroscope with C-mount and 0.5X objective	Leica	MZ6	Discontinued model, M60 is current equivalent.
Light source	Schott	A08923	3”x3”  backlight for even illumination across the field of view
Imaging and tracking software	Media Cybernetics	ImagePro-Plus v6.0-6.3	Newer versions of the software have tracking functions.