Introduction
One of the earliest observations in the study of circadian rhythms was that continuous light (LL) lengthens circadian period in most nocturnal animal species
The first question to be raised is whether a dim red LED can affect the circadian system of mice. The circadian rhythm of locomotor activity in rats is entrained by red light
The second question is whether light presented only in response to activity can lengthen period in mice. Pittendrigh and Daan suggested that light pulses during the photosensitive portion of an animal's circadian cycle mimic the effect of LL on period
In earlier studies we showed that C57BL/6 and DBA/2 mice differed in their Aschoff affect comparing constant dark to constant full-spectrum LL. At 10 lux, the C57BL/6 mice had an increase in period of 1.20 hours but the period of the DBA/2 mice increased only 0.20 hours
This study tests the hypotheses that a dim red LED provided as feedback to activity elicits an increase in circadian period of locomotor activity and that C57BL/6 and DBA/2 mice have a differential response to the red light stimulus.
Methods
General housing and care
Mice were housed singly in optically clear polycarbonate cages (L × H × W: 11 × 8 × 7 in) with approximately 250 ml of Sani-chip® (Harlan Teklad) bedding. They were acclimated under alternating 200 lux light and dark of 12 hours each (LD 12:12) for at least two weeks prior to the start of the study. Food (Teklad 7001 Mouse & Rat Diet 4%) and water were continuously available throughout the study. All animals were maintained in facilities fully accredited by the Association for the Assessment and Accreditation of Laboratory Animal Care. All research protocols and animal care were approved by the Institutional Animal Care and Use Committee in accordance with the guidelines of the
Experimental housing and care
For measurement of circadian period, all test mice were kept in a sound attenuating, ventilated room at a constant temperature (23°C) and under continuous darkness (DD). Sound attenuating, opaque dividers were placed between the test cages. Caretakers wore a Pelican Versabrite headlamp fitted with a red safelight beam diffuser. The diffuser/filter transmitted light greater than 600 nm only. Care in the darkroom consisted of ten min per day and each mouse was inspected for less than a minute. Daily visits occurred at random times between 8 am and 5 pm.
Locomotor activity assessment
Daily locomotor activity of the mice was monitored with passive infrared detectors (Ademco, Syosset, NY) mounted over each cage. The passive infrared (ir) proximity sensor works by emitting pulses of ir light, and then measuring the distance to objects from the flight time of the reflected signal. Whenever the distance changes, the detector opens or closes a switch. All detectors were tested to ensure response uniformity. Each detector had a red LED that switched on when motion was detected, then switched off 3 to 5 seconds after movement was no longer sensed. The LED could be disabled with a switch mounted on the motion sensor circuit board.
Spectral analysis
The irradiance spectra of the LEDs were determined using an S.I. Photonics fiber optic spectrophotometer (Tucson, AZ). The distance between the fiber optic input probe and the LED was 18 cm (the depth of the mouse cage). A random sample of eight of the 16 motion sensors used in the study was assessed. A hand-held light meter (UDT Instruments, Baltimore, MD) was used to measure illuminance produced by the LED at about 5 cm from the bottom of the cage and 13 cm from the LED. The test was repeated with the LEDs covered with black electrician's tape.
Assessment of circadian period of locomotor activity
Activity events were grouped into 5-minute bins by the Stanford Chronobiology Systems' (Stanford, CA) data processing and automatic storage system integrated into a Dell computer. Clocklab, the biological rhythm analysis software (Actimetrics, Evansville, IL), was used to calculate the period of locomotor activity of each mouse using linear regression through activity onsets of the last 8 to 10 days of each treatment.
Experiment 1: Hypothesis – LEDfb changes circadian period compared to DD
Mouse husbandry
C57BL/6 mice were bred in our facility from mice purchased from Jackson Laboratory (Bar Harbor, ME). Two male and six female C57BL/6 mice between the ages of 185 to 295 d were studied.
Experimental protocol
Four mice were put under motion sensors with the LED enabled (LEDfb), and four were put under sensors with the LED disabled (DD). The locomotor activity of the mice was monitored for two weeks (Stage 1). Then treatment was switched, and activity of the mice was monitored for another two weeks (Stage 2). The circadian period for each stage was calculated from the last 8 to 10 days under a given condition.
Statistical analysis
A factorial ANOVA (SAS ver. 9.1) tested for effect of sex, age, lighting condition (LEDfb compared to DD) and sequence of light treatment (LEDfb first compared to DD first). A post-hoc Tukey's Studentized Range test compared periods under different lighting protocols.
Experiment 2: Hypothesis – The effect of LEDfb on circadian period can be eliminated by blocking the light source
Mouse husbandry
Twelve male C57BL/6 mice aged 30 d were purchased from Jackson Laboratory and housed singly.
Experimental protocol
Following acclimation to our facility in LD 12:12 for two weeks, they were moved into DD. All mice were put under motion sensors with the LED enabled (LEDfb), but black electrician's tape covered the LEDs of six motion sensors (taped LED) for two weeks. For Stage 2, all the LEDs were turned off for two weeks of DD. For Stage 3, the treatment condition of Stage 1 was switched, i.e. all LEDs were enabled but the LEDs previously covered by tape were uncovered and the previously uncovered LEDs were covered. Mouse activity was monitored continuously throughout the experiment.
Statistical analysis
A one-way ANOVA tested for effect of lighting condition (DD compared to LEDfb and taped LED), with a post-hoc Tukey's Studentized Range test.
Experiment 3: Hypothesis – C57BL/6 and DBA/2 mice have different response to LEDfb
Mouse husbandry
Eight male C57BL/6 mice and eight male DBA/2 mice were purchased from Jackson Laboratory, age 4 weeks.
Experimental protocol
Following acclimation to our facility in LD 12:12 for two weeks, mice were moved into DD. Four mice of each strain (DBA/2 and C57BL/6) were put under motion sensors with the LED enabled (LEDfb), and four of each strain were put under sensors with the light disabled (DD). At the end of Stage 1, they were moved to LD 12:12 for one week. When mice returned to the assessment room under DD, the treatment condition was switched. Activities of all mice were monitored for another two weeks.
Statistical analysis
A two-factor ANOVA tested for effect of strain and lighting condition (LEDfb compared to DD) with a post-hoc Tukey's Studentized Range test. The change in period from LEDfb compared to DD (Δτ) was calculated for each mouse and compared by a
Results
Light measurements
The irradiance spectrum of the LED for a sample of 8 proximity sensors was a narrow band centered on 652 nm. Figure
The irradiance spectrum of a red LED integrated into the passive-infrared motion sensor circuitry
The irradiance spectrum of a red LED integrated into the passive-infrared motion sensor circuitry.
Experiment 1: LEDfb changes circadian period compared to DD
Representative actograms of C57BL/6 mice under DD and dim red LEDfb are shown in Figure
Double-plotted actograms of C57BL/6 mice under DD and dim red LEDfb
Double-plotted actograms of C57BL/6 mice under DD and dim red LEDfb. Lighting conditions are shown to the right of each actogram.
The circadian period of C57BL/6 mice is longer under dim red LEDfb than DD conditions (p = 0.0095)
The circadian period of C57BL/6 mice is longer under dim red LEDfb than DD conditions (p = 0.0095). Lines show the mean period for each group.
Experiment 2: The effect of LEDfb on circadian period can be eliminated by blocking the light source
Representative actograms of C57BL/6 mice under DD, dim red LEDfb, and LEDs coved with black tape are shown in Figure
Double-plotted actograms of C57BL/6 mice under DD, dim red LEDfb, and LEDs covered with black tape
Double-plotted actograms of C57BL/6 mice under DD, dim red LEDfb, and LEDs covered with black tape. Lighting conditions are shown to the right of each actogram. Arrows show onset of new lighting conditions.
Circadian period of C57BL/6 mice is longer under dim red LEDfb than when the light source is covered by black tape (p < 0.01) or DD (p < 0.025)
Circadian period of C57BL/6 mice is longer under dim red LEDfb than when the light source is covered by black tape (p < 0.01) or DD (p < 0.025). Lines show the mean period for each group.
Experiment 3: C57BL/6 and DBA/2 mice do not have different responses to LEDfb
Representative actograms of DBA/2 and C57BL/6 mice under DD and dim red LEDfb are shown in Figure
Double plotted actograms of DBA/2 and C57BL/6 mice under DD (top) and dim red LEDfb (bottom)
Double plotted actograms of DBA/2 and C57BL/6 mice under DD (top) and dim red LEDfb (bottom). The actograms at top and bottom are from one DBA/2 mouse (left) and one C57BL/6 mouse (right). Lighting conditions were separated by two weeks of LD 12:12.
The circadian period of both DBA/2 and C57BL/6 mice under DD (filled symbols) and dim red LEDfb (open symbols)
The circadian period of both DBA/2 and C57BL/6 mice under DD (filled symbols) and dim red LEDfb (open symbols). Lines show the mean period for each group. Overall, mice had longer period under LEDfb than DD (p < 0.025), and C57BL/6 mice had longer periods than DBA/2 mice (p < 0.01).
The mean increase in period with LEDfb (period under LEDfb minus period under DD, Δτ) for C57BL/6 mice was 0.15 ± 0.05 h. For DBA/2 mice, Δτ was 0.32 ± 0.13 h. The increase in period with LEDfb did not differ between strains by
In summary, circadian period was significantly longer under LEDfb (a small, red LED whose intensity was about 1 lux which came on only when a mouse was active) than that under DD in both C57BL/6 and DBA/2 strains of mice. The LEDs gave off red light in a narrow band centered on 652 nm. Covering the LED with black tape blocked the effect of the dim red light. Furthermore, there was no difference in this effect between the two strains.
Discussion
This study suggests that the circadian system in mice is responsive to long wavelength red light. The result is surprising because recent studies suggest that melanopsin, in combination with the classical rod and cone photoreceptors, account for the transduction of photic information to the circadian system. There are no studies of spectral sensitivity of the Aschoff effect in mice. However, the spectral sensitivity of photoreceptors mediating circadian phase-shifts in mice is vanishingly small at wavelengths above 600 nm
One possible explanation is that there is another photopigment present in mammals that is sensitive to far-red light and affects period rather than phase. It cannot be excluded that period and phase are affected by different light receptors or light receptive pathways. It seems more likely that low sensitivity to red light via the known circadian photopigments has a cumulative period-lengthening effect on the pacemaker. The timing of light exposure could have amplified this effect. Under LEDfb mice received light between circadian time (CT 12) and CT 24, during their active phase. The period-response curves (τRC) of mice have period-shortening between CT 4 and CT 16 and period-lengthening between CT 16 and CT 4
This study has several limitations. Only the Aschoff effect was investigated, and this was not under the usual protocol of constant light. Nevertheless, the increase in circadian period of mice under LEDfb was consistent with a prior activity feedback study in rats, where wheel-running triggered full-spectrum illumination resulting in lengthened circadian period
Covering the LED with black tape blocked the effect of the dim red light. We conclude that ultrasound from the LEDs or the electronics associated with their illumination did not produce the effect. Mice emit ultrasonic cries and this is important in maternal behavior
The C57BL/6 and DBA/2 mice did not differ in the amount period increased with 1 lux red light LEDfb. This is in contrast to an earlier study where C57BL/6 mice had a greater increase in period with 10 lux full-spectrum LL vs DD than DBA/2 mice
The results of this study suggest that investigators cannot use continuous dim red light to simulate DD, and must be judicious in using red "safe" lights for animal care in DD. Further studies are needed to determine whether constant red light of this output spectra and intensity lengthens period more than LEDfb, and whether it can phase-shift the circadian rhythms in mice.
Conclusion
Mice under a dim, long-wavelength red light that came on intermittently when the animals were active had a circadian period that was long compared to their free-running period under DD. Covering the light with black tape blocked the response. Furthermore, under the conditions described, the magnitude of the mean circadian period increase in DBA/2 and C57BL/6 strains of mice was indistinguishable.
Competing interests
The author(s) declare that they have no competing interests.
Authors' contributions
JRH conceived of the study, participated in its design and statistical analysis and drafted the manuscript.
ARH carried out experiment 1, designed and carried out experiment 3, and wrote the Methods section.
AMH participated in the statistical analysis and designed and set up experiment 2.
ARM carried out experiment 2, participated in the statistical analysis and assisted in drafting the manuscript.
All authors read and approved the final manuscript.