Methods for Detecting PER2:LUCIFERASE Bioluminescence Rhythms in Freely Moving Mice

Author:

Martin-Burgos Blanca1ORCID,Wang Wanqi1ORCID,William Ivana1ORCID,Tir Selma1ORCID,Mohammad Innus2,Javed Reja1,Smith Stormi1,Cui Yilin1ORCID,Arzavala Jessica1,Mora Dalilah1,Smith Ciearra B.34,van der Vinne Vincent45,Molyneux Penny C.1,Miller Stephen C.2,Weaver David R.34ORCID,Leise Tanya L.6ORCID,Harrington Mary E.1ORCID

Affiliation:

1. Neuroscience Program, Smith College, Northampton, Massachusetts

2. Department of Biochemistry and Molecular Pharmacology, University of Massachusetts Chan Medical School, Worcester, Massachusetts

3. Graduate Program in Neuroscience, University of Massachusetts Chan Medical School, Worcester, Massachusetts

4. Department of Neurobiology, University of Massachusetts Chan Medical School, Worcester, Massachusetts

5. Department of Biology, Williams College, Williamstown, Massachusetts

6. Department of Mathematics & Statistics, Amherst College, Amherst, Massachusetts

Abstract

Circadian rhythms are driven by daily oscillations of gene expression. An important tool for studying cellular and tissue circadian rhythms is the use of a gene reporter, such as bioluminescence from the reporter gene luciferase controlled by a rhythmically expressed gene of interest. Here we describe methods that allow measurement of circadian bioluminescence from a freely moving mouse housed in a standard cage. Using a LumiCycle In Vivo (Actimetrics), we determined conditions that allow detection of circadian rhythms of bioluminescence from the PER2 reporter, PER2::LUC, in freely behaving mice. The LumiCycle In Vivo applies a background subtraction that corrects for effects of room temperature on photomultiplier tube (PMT) output. We tested delivery of d-luciferin via a subcutaneous minipump and in the drinking water. We demonstrate spikes in bioluminescence associated with drinking bouts. Further, we demonstrate that a synthetic luciferase substrate, CycLuc1, can support circadian rhythms of bioluminescence, even when delivered at a lower concentration than d-luciferin, and can support longer-term studies. A small difference in phase of the PER2::LUC bioluminescence rhythms, with females phase leading males, can be detected with this technique. We share our analysis scripts and suggestions for further improvements in this method. This approach will be straightforward to apply to mice with tissue-specific reporters, allowing insights into responses of specific peripheral clocks to perturbations such as environmental or pharmacological manipulations.

Funder

National Institutes of Health

Publisher

SAGE Publications

Subject

Physiology (medical),Physiology

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