CNOT1 regulates circadian behaviour through Per2 mRNA decay in a deadenylation-dependent manner

Circadian clocks are an endogenous internal timekeeping mechanism that drives the rhythmic expression of genes, controlling the 24 h oscillatory pattern in behaviour and physiology. It has been recently shown that post-transcriptional mechanisms are essential for controlling rhythmic gene expression. Controlling the stability of mRNA through poly(A) tail length modulation is one such mechanism. In this study, we show that Cnot1, encoding the scaffold protein of the CCR4-NOT deadenylase complex, is highly expressed in the suprachiasmatic nucleus, the master timekeeper. CNOT1 deficiency in mice results in circadian period lengthening and alterations in the mRNA and protein expression patterns of various clock genes, mainly Per2. Per2 mRNA exhibited a longer poly(A) tail and increased mRNA stability in Cnot1+/− mice. CNOT1 is recruited to Per2 mRNA through BRF1 (ZFP36L1), which itself oscillates in antiphase with Per2 mRNA. Upon Brf1 knockdown, Per2 mRNA is stabilized leading to increased PER2 expression levels. This suggests that CNOT1 plays a role in tuning and regulating the mammalian circadian clock.journal articl

Post-transcriptional Regulation of Circadian Rhythm: Involvement of the CCR4-NOT Complex

Circadian clocks are an endogenous internal timekeeping mechanism that drive the rhythmic expression of genes, controlling the 24 hr oscillatory pattern in behavior and physiology. These cell-autonomous clocks synchronize to external factors primarily light; allowing organisms to anticipate, adapt, and coordinate their biology to the daily light/dark cycle. Post-transcriptional mechanisms have recently been shown to play an essential role in regulating mRNA and protein oscillations in a time-dependent manner. mRNA stability/decay control through poly(A) tail length modulation is one such mechanism. Poly (A) tail shortening results in mRNA destabilization, subsequent decay, and translational repression. The major deadenylase complex in the cytoplasm is the CCR4-NOT complex, which is essential for regulating gene homeostasis by modulating RNA metabolism on multiple fronts primarily mRNA decay. In this thesis, we examine the role of the CCR4-NOT complex in regulating circadian clocks by focusing on CNOT1, the scaffold protein. Cnot1 mRNA exhibits a constantly high expression in the mouse superchiasmatic nucleus (SCN) as well as a rhythmic protein and mRNA pattern in the mouse liver with peak expression at the early morning. Cnot1 deficiency in mice results in elongation of circadian period and alteration in mRNA and protein expression patterns of various clock genes, mainly Per2. The recruitment of CNOT1 to Per2 mRNA is mediated through Zfp36L1 (BRF1), which itself oscillates in antiphase with Per2 mRNA. Upon BRF1 knockdown, Per2 mRNA is stabilized. Taken together, this suggests that CNOT1 plays a role in tuning and regulating the mammalian circadian clock and circadian behavior.Okinawa Institute of Science and Technology Graduate Universit

Quantifying the Life Stages of a Biomolecule: Implications for the Circadian Transcriptome

Viele biologische Prozesse im Verhalten von ganzen Organismen, aber auch in den Prozessen und der biochemischen Zusammensetzung von Zellen zeigen einen zirkadianen Rhythmus, also einen Rhythmus mit einer Periode von etwa 24 Stunden. Diese 24-Stunden-Rhythmen sind in der Genexpression auf allen Ebenen zu finden: von der Tran- skriptionsinitiation bis zur Proteindegradation. Auf Transkriptebene, zirkadiane mRNA-Produktion und mRNA-Abundanz ist umfassend gemessen. Auf der anderen Seite, zirkadiane posttranskriptionelle Regulation ist weit weniger verstanden. In dieser Arbeit untersuche ich, wie bisher ungemessene, posttranskriptionelle Prozesse die rhythmischen Eigenschaften der Genexpression beeinflussen. Dazu beschreibe ich die Lebensstadien eines Bio-Moleküls mit einem Modell-Motiv, einer einfachen Differentialgleichung mit zeitabhängigen, rhythmischen Raten. Als erstes diskutiere ich die Einschränkungen von Phase und Amplitude zirkadianer Transkripte, die nur von konstanter PTR beeinflusst werden. Bei vielen gemessenen Transkripten sind diese Einschränkungen verletzt. In diesen Fällen muss es eine rhythmische PTR geben. Ich untersuche, welche rhythmische PTR diese Fälle erklären können und führe einen statistischen Test ein, der auf unbeobachtete, rhythmische PTR testet. Durch die Analyse zweier Datensätze von Mausleber und -niere finde ich, dass 18% aller zirkadianen Gene in Niere und 34% in Leber rhythmisch posttranskriptionell reguliert sind. Im zweiten Teil analysiere ich weitere Aspekte von PTR in einem Hypothesen-getriebenen Ansatz. Ich zeige, dass Spleißen mit einem Rhythmus von 24 Stunden 12 Stunden-Rhythmen in der Abundanz von mRNA erzeugen kann. Als nächstes schlage ich ein Modell vor, das rhythmische Degradation von Mitgliedern der zirkadianen Uhr beschreibt. Schließlich erweitere ich das Modell-Grundmotiv zu einer partiellen Differentialgleichung (PDG), die das “Altern” von Molekülen beschreibt.In almost all organisms on Earth, many behavioral, physiological, and biochemical activities oscillate with a circadian rhythm, a rhythm with a period of about 24 hours. In gene expression, the 24-hour-rhythm can be found on all stages: from transcription initiation to protein degradation. On the transcript level, circadian mRNA production and mRNA abundance are comprehensively charted through numerous genome-wide high throughput studies. Circadian post-transcriptional regulation, however, is less well understood. In this thesis, I will investigate how unobserved post-transcriptional processes influence rhythmic properties of gene expression. To this end, I quantify the life-stages of biomolecules using one modeling motif, a simple ordinary differential equation describing production and degradation with time-dependent rhythmic rates. This basic modeling motif is systematically varied to examine and discuss various influences of post-transcriptional regulation (PTR) on circadian mRNA expression. I first discuss the restrictions of rhythmic phase and amplitude of circadian transcripts influenced by non-rhythmic PTR. For many genes these restrictions are violated and we have to assume the existence of a rhythmic PTR. I discuss which rhythmic PTR can explain these findings and further introduce a statistical test to quantify the extent of unobserved rhythmic PTR. Analyzing two data sets on mouse liver and kidney, I find that 18% of circadian genes in kidney and 34% in liver are under rhythmic post-transcriptional control. In a second part, I analyze more specific aspects of PTR in a hypothesis-driven approach. Firstly, I find that splicing with a rhythm of 24 hours is able to generate 12-hour rhythms in abundance of mature mRNA. Secondly, I propose and analyze a model to investigate rhythmic degradation of core clock genes. And finally, I extend the core modeling motif to a partial differential equation (PDE) model that accounts for the “aging” process of molecules

The Circadian Deadenylase Nocturnin Is Necessary for Stabilization of the iNOS mRNA in Mice

Nocturnin is a member of the CCR4 deadenylase family, and its expression is under circadian control with peak levels at night. Because it can remove poly(A) tails from mRNAs, it is presumed to play a role in post-transcriptional control of circadian gene expression, but its target mRNAs are not known. Here we demonstrate that Nocturnin expression is acutely induced by the endotoxin lipopolysaccharide (LPS). Mouse embryo fibroblasts (MEFs) lacking Nocturnin exhibit normal patterns of acute induction of TNFα and iNOS mRNAs during the first three hours following LPS treatment, but by 24 hours, while TNFα mRNA levels are indistinguishable from WT cells, iNOS message is significantly reduced 20-fold. Accordingly, analysis of the stability of the mRNAs showed that loss of Nocturnin causes a significant decrease in the half-life of the iNOS mRNA (t1/2 = 3.3 hours in Nocturnin knockout MEFs vs. 12.4 hours in wild type MEFs), while having no effect on the TNFα message. Furthermore, mice lacking Nocturnin lose the normal nighttime peak of hepatic iNOS mRNA, and have improved survival following LPS injection. These data suggest that Nocturnin has a novel stabilizing activity that plays an important role in the circadian response to inflammatory signals

Beyond Transcription: Fine-Tuning of Circadian timekeeping by post-transcriptional regulation

Mateos JL, de Leone MJ, Torchio J, Reichel M, Staiger D. Beyond Transcription: Fine-Tuning of Circadian timekeeping by post-transcriptional regulation. Genes. 2018;9(12): 616.The circadian clock is an important endogenous timekeeper, helping plants to prepare for the periodic changes of light and darkness in their environment. The clockwork of this molecular timer is made up of clock proteins that regulate transcription of their own genes with a 24 h rhythm. Furthermore, the rhythmically expressed clock proteins regulate time-of-day dependent transcription of downstream genes, causing messenger RNA (mRNA) oscillations of a large part of the transcriptome. On top of the transcriptional regulation by the clock, circadian rhythms in mRNAs rely in large parts on post-transcriptional regulation, including alternative pre-mRNA splicing, mRNA degradation, and translational control. Here, we present recent insights into the contribution of post-transcriptional regulation to core clock function and to regulation of circadian gene expression in Arabidopsis thalian

Computational Analyses of mRNA Ribosome Loading in Arabidopsis Thaliana

Translation of mRNA into protein is a critical step in gene expression, but the principles guiding its regulation at the genome level are not completely understood. Translation can be quantified at a genome scale by measuring the ribosome loading of mRNA—the extent to which mRNA is associated with ribosomes. In this dissertation, I present investigations into how genome-wide ribosome loading is controlled in Arabidopsis thaliana. In chapter 1, I give an overview of regulation of ribosome loading and translation. In chapter 2, I present research demonstrating for the first time that genome-wide ribosome loading in plants is partially controlled by the circadian clock. In chapter 3, I present a study of a computational model that describes how various biochemical steps control ribosome loading. And in chapter 4, I conclude by briefly summarizing the dissertation as a whole and discussing future perspectives

Genome-wide analysis of PAPS1-dependent polyadenylation identifies novel roles for functionally specialized poly(A) polymerases in Arabidopsis thaliana

The poly(A) tail at 3’ ends of eukaryotic mRNAs promotes their nuclear export, stability and translational efficiency, and changes in its length can strongly impact gene expression. The Arabidopsis thaliana genome encodes three canonical nuclear poly(A) polymerases,PAPS1, PAPS2 and PAPS4. As shown by their different mutant phenotypes, these three isoforms are functionally specialized, with PAPS1 modifying organ growth and suppressing a constitutive immune response. However, the molecular basis of this specialization is largely unknown. Here, we have estimated poly(A)-tail lengths on a transcriptome-wide scale in wild-type and paps1 mutants. This identified categories of genes as particularly strongly affected in paps1 mutants, including genes encoding ribosomal proteins, cell-division factors and major carbohydrate-metabolic proteins. We experimentally verified two novel functions of PAPS1 in ribosome biogenesis and redox homoeostasis that were predicted based on the analysis of poly(A)-tail length changes in paps1 mutants. When overlaying the PAPS1-dependent effects observed here with coexpression analysis based on independent microarray data, the two clusters of transcripts that are most closely coexpressed with PAPS1 show the strongest change in poly(A)-tail length and transcript abundance in paps1 mutants in our analysis. This suggests that their coexpression reflects at least partly the preferential polyadenylation of these transcripts by PAPS1 versus the other two poly(A)-polymerase isoforms. Thus, transcriptome-wide analysis of poly(A)-tail lengths identifies novel biological functions and likely target transcripts for polyadenylation by PAPS1. Data integration with large-scale co-expression data suggests that changes in the relative activities of the isoforms are used as an endogenous mechanism to co-ordinately modulate plant gene expression