Abstract

Circadian rhythms are generated by molecular clocks that are universally used to synchronize behavior and physiology with the 24-hour solar cycle. This proposal seeks to understand the biochemical basis of circadian timing and photoentrainment, the process by which molecular clocks are aligned to the external light/dark cycle. In mammals, circadian rhythms arise from set of interlocked transcription feedback loops involving dedicated clock proteins: at the center of this network, CLOCK:BMAL1 activates transcription of its repressors PERIOD (PER) and CRYPTOCHROME (CRY), which ultimately feed back to complete a ~24-hour long cycle of gene activation and repression. Photoentrainment is important to keep molecular clocks on track with environmental light cycles. Chronic circadian misalignment (i.e. jetlag) leads to increased risk for metabolic disorders, cardiovascular disease and cancer due to disruption of the systemic control of physiology by circadian rhythms. While much of the photoentrainment pathway has been laid out from ocular photoreception to its acute induction of Per mRNA in the master clock of the brain, crucially, the final biochemical steps that execute entrainment on the molecular level remain completely unknown. Exposure to light before dawn leads to phase advances of the molecular clock, while light after dusk delays the clock, both of which keep CLOCK:BMAL1 activity aligned with the day. How does this plasticity in phase shifting arise from the same light-dependent induction of Per mRNA that occurs at dusk and dawn? ChIP-seq studies provide evidence for distinct repressive complexes that assemble in the evening, an `early' complex of PER and CRY proteins that assembles at dusk on CLOCK:BMAL1 and a `late' complex of CRY1 bound alone to CLOCK:BMAL1 at dawn. Our central hypothesis is that differences in the composition of early and late repressive complexes are exploited for entrainment, leading to differential regulation by light-induced PER2 at dusk and dawn. We will test this with three specific aims. First, the molecular basis for differences in regulation of CLOCK:BMAL1 by CRY1, CRY2 and PER2 will be defined with biochemical, biophysical, and cellular studies. Second, structures of early and late repressive complexes will be determined by cryo-electron microscopy to identify overall changes in molecular architecture of the core clock proteins that occur throughout the evening. Third, the development of a new optogenetic model for the study of cellular clocks will allow the identification of biochemical determinants by which clocks are entrained to external stimuli. Collectively, these lines of study will address how core clock proteins interact throughout the evening in distinct regulatory complexes to generate circadian timekeeping and respond to external stimuli.

Public Health Relevance

Circadian rhythms synchronize our behavior and physiology into daily rhythms that align with the light/dark cycle. Our work seeks to understand how circadian timing is generated through the assembly and regulation of clock protein complexes and how this molecular clock adjusts in response to light at dawn and dusk. Understanding how light influences circadian rhythms at the molecular level could identify new strategies to leverage the health- promoting effects of aligning our biological clocks with the light/dark cycle.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM107069-08
Application #
9984400
Study Section
Macromolecular Structure and Function B Study Section (MSFB)
Program Officer
Sesma, Michael A
Project Start
2013-08-15
Project End
2022-07-31
Budget Start
2020-08-01
Budget End
2021-07-31
Support Year
8
Fiscal Year
2020
Total Cost
Indirect Cost

  Institution

Name
University of California Santa Cruz
Department
Chemistry
Type
Schools of Arts and Sciences
DUNS #
125084723
City
Santa Cruz
State
CA
Country
United States
Zip Code
95064

  Publications

Ceh-Pavia, EfraĆ­n; Partch, Carrie L (2018) Regulating behavior with the flip of a translational switch. Proc Natl Acad Sci U S A 115:13151-13153
Narasimamurthy, Rajesh; Hunt, Sabrina R; Lu, Yining et al. (2018) CK1?/? protein kinase primes the PER2 circadian phosphoswitch. Proc Natl Acad Sci U S A 115:5986-5991
Michael, Alicia K; Fribourgh, Jennifer L; Van Gelder, Russell N et al. (2017) Animal Cryptochromes: Divergent Roles in Light Perception, Circadian Timekeeping and Beyond. Photochem Photobiol 93:128-140
Gustafson, Chelsea L; Parsley, Nicole C; Asimgil, Hande et al. (2017) A Slow Conformational Switch in the BMAL1 Transactivation Domain Modulates Circadian Rhythms. Mol Cell 66:447-457.e7
Fong, Jiunn Cn; Rogers, Andrew; Michael, Alicia K et al. (2017) Structural dynamics of RbmA governs plasticity of Vibrio cholerae biofilms. Elife 6:
Michael, Alicia K; Fribourgh, Jennifer L; Chelliah, Yogarany et al. (2017) Formation of a repressive complex in the mammalian circadian clock is mediated by the secondary pocket of CRY1. Proc Natl Acad Sci U S A 114:1560-1565
Tseng, Roger; Goularte, Nicolette F; Chavan, Archana et al. (2017) Structural basis of the day-night transition in a bacterial circadian clock. Science 355:1174-1180
Fribourgh, Jennifer L; Partch, Carrie L (2017) Assembly and function of bHLH-PAS complexes. Proc Natl Acad Sci U S A 114:5330-5332
Militi, Stefania; Maywood, Elizabeth S; Sandate, Colby R et al. (2016) Early doors (Edo) mutant mouse reveals the importance of period 2 (PER2) PAS domain structure for circadian pacemaking. Proc Natl Acad Sci U S A 113:2756-61
Huynh, Kathy; Partch, Carrie L (2015) Analysis of protein stability and ligand interactions by thermal shift assay. Curr Protoc Protein Sci 79:28.9.1-14

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