Determination of the Spontaneous Locomotor Activity in Drosophila melanogaster

Summary

Drosophila melanogaster are useful in studying genetic or environmental manipulations that affect behaviors such as spontaneous locomotor activity.  Here we describe a protocol that utilizes monitors with infrared beams and data analysis software to quantify spontaneous locomotor activity. 

Abstract

Drosophila melanogaster has been used as an excellent model organism to study environmental and genetic manipulations that affect behavior. One such behavior is spontaneous locomotor activity. Here we describe our protocol that utilizes Drosophila population monitors and a tracking system that allows continuous monitoring of the spontaneous locomotor activity of flies for several days at a time. This method is simple, reliable, and objective and can be used to examine the effects of aging, sex, changes in caloric content of food, addition of drugs, or genetic manipulations that mimic human diseases.

Introduction

Fruit flies, Drosophila melanogaster, have been used as a valuable model organism to study mechanisms underlying complex behaviors, such as learning and memory, social interaction, aggression, drug abuse, sleep, sensory function, courtship, and mating^1,2. One behavior that has been studied through multiple protocols is spontaneous locomotor activity. Negative geotaxis was one of the first methods developed for measuring Drosophila activity, and this protocol involves measuring the percentage of flies that reach a certain height of the vial after flies were shaken to the bottom of the container^1,3.  This method has advantages of being straightforward, inexpensive, and since it does not require any special equipment it can be performed in any laboratory. It has been used as a valuable screening tool to study effects of different genetic manipulations on fly mobility³. However, it is time and labor intensive and has the possibility of bias due to variable shaking of the vials and human recordings. 

The negative geotaxis method was improved upon by development of the Rapid Iterative Negative Geotaxis (RING) method^4,5, which takes photographs of the fly vials following shaking of the flies to the bottom. The advantage of this protocol is its sensitivity and the possibility of testing a large number of fly vials at the same time. However, this protocol still has the potential for human error, and only measures negative geotaxis. Other laboratories have used simple observation in culture vials to determine locomotor activity⁶.

Recently several video recording systems for measuring fly locomotor activity have been developed.  One video monitoring protocol provides time for adjustment before recording⁷.  The method described by Slawson et al. also uses an air pulse to stop movement until the start of recording, which could potentially be a stressor to the animals⁷.  This method provides information on average speed, max speed, time spend in motion, etc.  Another three-dimensional tracking system measures the maximal velocity of individual flies during ~0.2 seconds of free flight takeoff⁸. A three-dimensional video monitoring protocol uses flies expressing GFP and multiple cameras fitted with filters allowing for detection of fluorescence to determine fly mobility⁹. Flies in this protocol tend to exhibit cylindrical flight patterns, which is potentially due to the shape of Drosophila culture vials¹⁰. This method was improved by using a dome that allows measuring spontaneous movement of two flies¹¹. A high-throughput method that uses a camera to automatically monitor and quantify the individual and social behavior of Drosophila has been also described¹².  Zou et al. developed a behavioral monitor system (BMS) that uses two computer-assisted cameras to record lifetime behavior and movements such as resting, moving, flying, eating, drinking, or deaths of individual tephritid fruit flies¹³. Several other video systems have been developed to monitor fly behavioral activity^14,15.  

Here we describe a method for quantifying Drosophila activity that utilizes population monitors. These monitors are housed in temperature- and humidity-controlled incubators at 25 °C on a 12 hour day-night light cycle. Each population monitor has infrared beams placed in rings positioned at three different heights. Every time a fly moves across the rings it interrupts the infrared beam, which is recorded by a microprocessor that independently records and counts the activity of flies within the vial. A microprocessor uploads the total activity within the vial to the computer at user-defined intervals that could vary from 1 second to 60 minutes. The method described here provides ample time for flies to adjust to the new environment and allows for simultaneous measuring of the spontaneous locomotor activity of as many as 120 populations of flies. In addition, we describe preparation of the food, fly maintenance, setting up the mobility population monitors in temperature controlled incubators, and potential factors that may affect results. This method can be used to study how different environmental or genetic modifications affect spontaneous locomotor activity of the flies.

Protocol

Note: The Canton-S strain is the standard wild-type background line obtained from the Bloomington Stock Center.

1. Food Preparation and Recipe for 1,000 ml of Food

Note: This section describes the protocol for food preparation. Large metal pots are used to prepare about 18 L of food at a time. The protocol described here is downsized and uses 1,000 ml H₂O. Food is autoclaved twice.

1. Mix 113 g sucrose and 28 g brewers yeast in 643 ml water. Leave ingredients on a hot plate set at 25 °C with a stir bar to mix throughout for 15 minutes.
2. Autoclave food solution for 20 min.
3. Mix 49 g cornmeal and 8.1 g agar in 268 ml water and add to the autoclaved food mixture described in step 1.2. Mix well with a large spoon or a whisk.
4. Autoclave food mixture for another 20 min.
5. Place the food on a plate and let cool down with constant mixing with a stir bar. If additional solutions should be added to food, such as mifepristone (RU486), keep the food on a hot plate set up at 60 °C and add solution when the food reaches the required temperature.
6. Dissolve 2.4 g tegosept in 10.7 ml 100% EtOH and keep on a cold plate with a stirrer to completely dissolve and mix for about 15 min.
7. Add tegosept solution to food when the temperature of food is 60 °C and mix well.
8. Use a pump or a food dispenser to pour about 10 ml of food into a wide vial. By using a food dispenser one can pour food simultaneously into 100 wide, plastic vials (1 tray) at a time.
9. Cover the vials with Kimwipes and cheese cloth and leave food at room temperature for 12-24 hr to cool down. Keep the food at 4 °C and use within 3-4 weeks. Warm up the food to room temperature before use for fly work.

2. Preparation of Glass Vials

1. Prepare food according to the protocol listed in step 1.
2. Aliquot 5 ml of food into each narrow, glass vial, which is the correct size for the population monitors. This amount of food should be low enough to be below the lowest ring of the population monitor.
3. After the food cools down to room temperature cover the vials with sponge plugs and keep them at 4 °C for up to 2 weeks. Because the amount of food in a vial is rather low, it is best to use the food within a week or two to prevent any drying.
4. Warm up the vials to room temperature before use.

3. Maintenance of the Parental Flies

1. Grow the flies in wide plastic vials with standard laboratory food and keep the vials in a humidified, temperature-controlled environmental chamber at 25 °C on a 12 hr light/dark cycle. The daylight period starts at 6:00 AM in this laboratory.
2. In the morning clear adult flies from the vials from which parental flies will be collected.
3. Collect newly eclosed flies and separate them by gender on a CO₂ pad within 8 hr after eclosion to make sure that the female flies are virgins. Flies start to mate 8 hr after eclosion.
4. When the virgin male and female flies are between 5 and 10 days of age, put 10 males and 10 female flies in a vial with standard food and several grains of active yeast on top.
   Note: Control the density of the larvae by using the same number of flies and keeping them in a vial for two days. Addition of active yeast promotes egg production.
5. Keep the flies to mate and lay eggs in a temperature-controlled environmental chamber at 25 °C with a 12 hr light/dark cycle for 2 days. Set up 5-10 vials of parental flies.
6. Pass the flies to a new plastic vial every other day and keep the vials with the eggs in an incubator at 25 °C.

4. Collection of Experimental Flies

1. After 9 days flies will start to eclose from the vials where the parental flies laid eggs (described in step 3.6.). Clear and discard the flies that eclosed during the first day and return the vials to incubator. Most of the flies eclosed on day 1 are females. A more synchronized population of flies will eclose on day 2.
2. Within 24 hr place newly eclosed flies on CO₂ pads and collect 25 male and 25 female flies per vials with a paintbrush or metal spoon. Keep flies on CO₂ pads for a short period of time to minimize any effects of CO₂. Write down the day of eclosion on the vial. Assemble at least 5 replicate vials for experimental and for control groups.
3. Keep the vials in temperature-controlled environmental chambers at 25 °C with a 12 hr light/dark cycle.
4. Pass the flies to a new plastic vial every other day using a funnel.
5. Age the flies until the desired age for experimentation is reached.

5. Setting Up the Mobility Monitors

1. Place the population monitors in a temperature-controlled incubator.
2. Connect each monitor with a 4-wire telephone cable to the Power Supply Interface Unit (PSIU) via 5-way splitters (multi-line), which can connect up to 5 individual monitors to one opening in the PSIU. See Figures 1A and 2B.
3. Connect the PSIU to a line power outlet (100-240 V). Plug the power supply output connector into one of the 2 mating PSIU jacks. The adjacent green light illuminates green when connected properly.
4. Connect the PSIU to the Universal Serial Bus (USB) hardware. Connect the USB cable between the USB hardware with a Macintosh or a Windows PC for data recording. It would be best to have a computer dedicated only for data collection since collection runs for days at a time.
5. Download the USB software (PSIUdrivers.zip). USB driver software is used by the Power Supply interface and needs to be downloaded only once. It synthesizes a data link between the computer program and the PSIU/activity monitors. For a PC use a COM port and for a Macintosh use a simple serial port.
6. Download the computer program for Macintosh OSX (Intel) or for Windows PC (XP/Vista/7) programs by following instructions provided by manufacturer Notes 308.pdf.
7. Start the computer program and set up the program by clicking on the Preferences, Lights or Monitors. The program will run until the user selects “quit” to stop the program. If the computer program or the computer is shut down the monitors will continue to count beam interruptions, but the counts will not be recorded until the program is re-launched. In that case the first reading will include all the counts since the last time the PSIU sent the data to computer.
8. Select the Preferences tab and choose the Serial Port, PSIU for Macintosh and COM for the PC.
9. Select the reading interval that ranges from seconds, minutes, or an hour.
10. Select the monitors: Each monitor has its unique number that is given by the manufacturer. Select the Monitor Range that corresponds to the numbers given to the monitors by the manufacturer.
11. The Lights box: Make sure that all the monitors are properly connected, which is marked by a green light next to the monitor number on the software. A red light indicates that the connection is lost, and a black box indicates that the system is off or improperly set up.

6. Setting Up the Experiment

1. Remove glass vials containing food from 4 °C and let them warm to room temperature.
2. Separate male and female flies of the same age on CO₂ pad. For aging studies it is possible to start mobility studies as early as 3 days of age.
3. Put 10 male or 10 female flies into each glass vial containing food. Use at least three vials for each experimental and control line of flies and for each gender.
4. Keep the vials on their side until the flies recover from CO₂ to ensure the flies do not get stuck in the food. Separate flies at about 8:00 AM and leave them for about 2 hr at room temperature to recover from CO₂.
5. Place the vials inside the population monitors housed in the incubators.
6. Discard the data collected within the first 24 hr after the flies are put into the incubator to let them adjust to the novel environment.
7. Pass the flies after 3 or 4 days to new vials to avoid drying of the food. If flies are prone to death or are age 40 days or older, pass the flies after 2 days and use data collected for day 2. Also, use more than three vials per group to ensure adequate replicates. Data from vials with dead flies should be disregarded and not included in analysis.

7. Running the Activity Monitors and Calculating the Total Spontaneous Activity

1. Select preferences - the interval for data collection.
   Note: The computer program allows collection of the data at intervals ranging from 1 second to 60 minutes. 10 and 30 minute periods have been found to provide adequate information about mobility without having an overwhelming number of time points. At the selected time period, the program will send the current total count for each monitor to the computer and start counting again from zero. The computer program stores the data in a new folder created by the computer data system. The data collected in each monitor are stored separately, and individual text documents are created for each vial. The data are continuously collected as long as the program operates.
2. At the end of the experiment, scan the data using the FileScan110X for Macintosh OSX (Intel) or SystemMB108 for Windows PC (XP/Vista/7) program.
   Note: The Scan program eliminates duplicate readings and makes sure that the recordings are complete.
3. Save the data collected within a specific time and period of days. Choose an experimental name and copy the files from the computer data folder for analysis.
   Note: At this time, activity intervals can be changed and converted to different ones. The original data will stay stored in the computer data folder and can be retrieved as long as they are not deleted.

8. Data Analysis

1. Copy the data collected in the text files into columns of Excel spreadsheets for data analysis. Data collected by this software are in columns, which contain numbers representing total activity in a single monitor over a period of time selected by the investigator.
   Note: Data collected for each monitor are in separate text files. There are 32 columns for each monitor. The first six columns are empty and contain only 0; next three contain the data collected at the bottom ring, in the middle, and at the top ring. The rest of the channels can be deleted since they do not contain any data. Each ring outputs a single value per time. See screen shot of the raw data in Figure 2.
2. Calculate the total activity within a desired period of time for each monitor that represents the sum of activity collected at three different heights of infrared beams.
   Note: The time period can range from several hours, 24 hours or several days.
3. Determine the average locomotor activity and the standard deviation between the 3 monitors that represent 3 biological replicates.
   Note: The data can be analyzed for statistical significance by using a number of tests. A two-tailed Students’s t-test, a one-way analysis of variance (ANOVA) and a Tukey HSD post-hoc test could be used to determine the effects of several environmental or genetic manipulations on 24 hours of spontaneous locomotor activity¹⁶. There are a number of other programs that can be used and have been previously published¹⁷.

Results

The spontaneous locomotor activity in Drosophila depends on fly gender (Figure 3A), calorie content of the food (Figure 3B) and the light/dark cycle. Once the light is switched off fly activity dramatically decreases. Figure 3A illustrates 24 hours of locomotor activity recordings of male and female flies. An asterisk on the x-axis marks the time when the light was switched off and the transition to dark cycle. Figure 3B illustrates the standard...

Discussion

Spontaneous locomotor activity of flies is influenced by many factors such as age, genetic background, and gender^2,13,18,19. In addition, environmental factors such as caloric content of the food, temperature of the environment, addition of different drugs, and day/night light cycle can affect fly activity. For instance, male flies of the same age have a higher spontaneous physical activity compared to females (Figure 1). Therefore, flies of the same age and gender should be compared to each o...

Materials

Name	Company	Catalog Number	Comments
Sucrose FCC Food Grade 100 LB,	Fisher Scientific MP Biomedicals	ICN90471380
Brewer’s Yeast	Fisher Scientific MP Biomedicals	ICN90331280
Drosophila Agar Fine	SciMart	DR-820-25F
Cornmeal	Fisher Scientific MP Biomedicals	ICN90141125
Methyl4-hydroxybenzoate, tegosept	Sigma	H5501-5KG
EtOH	Pharmco-AAPER	111000200
Active Dry Yeast	Fisher Scientific	ICN10140001
Fly CO2 pad	LabScientific	BGSU-7
Stereo Microscope	Olympus	SZ40
Drosophila carbon dioxide (CO2) tank	Airgas	UN1013
Small paint brush for pushing the flies
Shell vial wide	Fischer Scientific	AS519
Buzzplugs for wide plastic vials	Fischer Scientific	AS275
Glass vials (25 x 95 mm)	Fischer Scientific Kimble 60931-8	AS-574
Sponge plugs for glass vials	SciMart	DR-750
Drosophila Food Dispenser	Applied Scientific (Fischer Scientific)	AS780Q
DPM Drosophila Population Monitor	Trikinetics Inc.
DC Power Supply with line cord	Trikinetics Inc.
PSIU9 The Power Supply Interface Unit	Trikinetics Inc.
Telephone cables and 5 way splitters	Trikinetics Inc.
Universal Serial Bus (USB) hardware	Trikinetics Inc.
Macintosh or Windows PC with UCB port
DAMSystem308X Data Acquisition Software for Macintoch OSX (Intel)	www.trikinetics.com
DAMSystem308 Data Acquisition Software for Windows PC (XP/Vista/7)	www.trikinetics.com
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DAMFileScan108X software for Macintosh	www.trikinetics.com
DAMFileScan108X software for Windows PC (XP/Vista/7)	www.trikinetics.com
USB software (PSIUdrivers.zip)	www.trikinetics.com
DAMSystem Notes 308	(http://www.trikinetics.com/Downloads/DAMSystem%20Notes%20308.pdf