Structural mimicry confers robustness in the cyanobacterial circadian clock

AbstractThe histidine kinase SasA enhances robustness of circadian rhythms in the cyanobacterium S. elongatus by temporally controlling expression of the core clock components, kaiB and kaiC. Here we show that SasA also engages directly with KaiB and KaiC proteins to regulate the period and enhance robustness of the reconstituted circadian oscillator in vitro, particularly under limiting concentrations of KaiB. In contrast to its role regulating gene expression, oscillator function does not require SasA kinase activity; rather, SasA uses structural mimicry to cooperatively recruit the rare, fold-switched conformation of KaiB to the KaiC hexamer to form the nighttime repressive complex. Cooperativity gives way to competition with increasing concentrations of SasA to define a dynamic window by which SasA directly modulates clock robustness.One Sentence SummarySasA controls the assembly of clock protein complexes through a balance of cooperative and competitive interactions.

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Domains of the rat rDNA promoter must be aligned stereospecifically

Molecular and Cellular Biology ◽

10.1128/mcb.12.3.1266-1275.1992 ◽

1992 ◽

Vol 12 (3) ◽

pp. 1266-1275

Author(s):

W Q Xie ◽

L I Rothblum

Keyword(s):

Protein Complexes ◽

Point Mutations ◽

In Vitro Transcription ◽

Promoter Elements ◽

Repeat Distance ◽

Deletion Mutations ◽

The Core ◽

In Vivo Experiments

Efficient transcription from the rat rDNA promoter results from an undefined interaction between the core (CPE) and upstream (UPE) promoter elements or the protein complexes which form on them. These interactions were demonstrated by the behavior of promoters that contained either linker-scanning or deletion mutations of the UPE in combination with point mutations of the CPE (bidomain mutants). In vivo transcription experiments using point mutations within the CPE (G----A mutation at either -16 or -7) demonstrated that the CPE may in fact consist of two domains. Whereas both of these mutants were rescued by the addition of UBF to in vitro transcription reactions, the CPE mutant -7A/G was inactive in vivo. Experiments with these bidomain mutants demonstrated that the UPE was required for the rescue of the CPE mutants. We also examined the hypothesis that this interaction might require a stereospecific alignment of the promoter elements. Our results indicate that the promoter consists of several domains with differing responses to mutations that alter the distance between, or within, the promoter elements. For example, the insertion or deletion of half-multiples of the helical repeat distance between -167 and -147 had no significant effect on transcription. On the other hand, some sites were sensitive to deletions of any size but not to insertions of up to 20 bp. The analyses of two sites yielded results suggesting that they lay between domains of the promoter that must be on the same side of the DNA helix for promoter activity. The first of these sites mapped between -106 and -95.(ABSTRACT TRUNCATED AT 250 WORDS)

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Evolution Analysis of the Circadian Clock Protein KaiB

Advanced Materials Research ◽

10.4028/www.scientific.net/amr.647.391 ◽

2013 ◽

Vol 647 ◽

pp. 391-395

Author(s):

Liu Sen ◽

Song Liu

Keyword(s):

Circadian Rhythms ◽

Circadian Clock ◽

Feedback Loop ◽

Circadian System ◽

Circadian Rhythmicity ◽

Physiological Functions ◽

Clock System ◽

Evolution Analysis ◽

Clock Protein

Regulation of daily physiological functions with approximate a 24-hour periodicity, or circadian rhythms, is a characteristic of eukaryotes. So far, cyanobacteria are only known prokaryotes reported to possess circadian rhythmicity. The circadian system in cyanobacteria comprises both a post-translational oscillator (PTO) and a transcriptional/translational feedback loop (TTFL). The PTO can be reconstituted in vitro with three purified proteins (KaiA, KaiB, and KaiC) with the existence of ATP. Phase of the nanoclockwork has been associated with the phosphorylation states of KaiC, with KaiA promoting the phosphorylation of KaiC, and KaiB de-phosphorylating KaiC. Here we studied the evolution of the KaiB protein. The result will be helpful in understanding the evolution of the circadian clock system.

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Causal Relationships among Metabolic Circadian Rhythms in Lemna

Zeitschrift für Naturforschung C ◽

10.1515/znc-1984-1-213 ◽

1984 ◽

Vol 39 (1-2) ◽

pp. 73-84 ◽

Cited By ~ 19

Author(s):

Ken Goto

Keyword(s):

Circadian Rhythms ◽

Kinase Activity ◽

Continuous Light ◽

Mirror Image ◽

Nad Kinase ◽

Long Day ◽

Level Of Activity ◽

Night Period

Abstract Biochemical aspects of circadian rhythms were studied using a long-day duckweed, Lemna gibba G3 cultured in short day condition (9 h light at 3800 lux followed by 15 h darkness), which was transferred in continuous light (LL) at the end (LL 0) of the last night period. With such a system I have previously reported a rhythm of affinity for NAD+ of cytoplasmic NAD - dependent glyceraldehyde 3-phosphate dehydrogenase (Cyt-NAD -GPD ) 180° out of phase with that of affinity for NADP+ of chloroplastic NADP-dependent GPD (Chl-NADP-GPD ) and that NADP+ could increase in vitro the affinity for NADP+ of Chl-NADP-GPD . I report here that NADP+ can decrease in vitro the affinity for NAD+ of Cyt-NAD -GPD as well, and furthermore, that the in vivo level of NADP+ oscillates in phase with the rhythm of the affinity for NADP+ of Chl-NADP-GPD. Moreover, I found the existence of mirror-image circadian rhythms, of comparable am plitudes, of in vivo levels of NAD+ + NADH (total NAD) (with peaks, as the ones of Cyt-NAD - GPD. at LL 0 and 24) and of NADP+ + NADPH (total NADP) (with peaks, as the ones of Chl-NADP-GPD, at LL 12 and 36). Consequently, a circadian rhythm in the rate of net in vivo production of total NADP (or NAD) might be expected 90° in advance of that in the level of total NADP (or NAD). Indeed. I found oscillations in the activities of NAD kinase and of NADP phosphatase with peaks occurring, respectively, at LL 6 and at LL 18. Moreover, in vitro treatments with EGTA (a Ca2+-chelator), chlorpromazine and W7 (both inhibitors of calmodulin) were able to both inhibit NAD kinase from its highest level of activity to its minimal one and activate NADP phosphatase from its lowest level of activity to its maximal one. I conclude, therefore, that the in vivo level of Ca2+-calmodulin could oscillate in phase with the rhythm of NAD kinase activity and induce the mirror-image circadian rhythms of activities of NAD kinase and of NADP phosphatase. I propose that the control sequence among the several circadian rhythms I studied could start with changes in Ca2+-calmodulin, then proceed through oscillations in NAD kinase and NADP phosphatase activities, leading to changes in NAD+, NADP+, and NADPH levels, which would themselves induce the Chl-NADP-GPD and Cyt-NAD -GPD rhythms.

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Drosophila Ada2b Is Required for Viability and Normal Histone H3 Acetylation

Molecular and Cellular Biology ◽

10.1128/mcb.24.18.8080-8089.2004 ◽

2004 ◽

Vol 24 (18) ◽

pp. 8080-8089 ◽

Cited By ~ 37

Author(s):

Dai Qi ◽

Jan Larsson ◽

Mattias Mannervik

Keyword(s):

Gene Expression ◽

Transcriptional Activation ◽

Protein Complexes ◽

P53 Protein ◽

Polytene Chromosomes ◽

Histone H3 ◽

Saga Complex ◽

Histone H3 Acetylation ◽

H3 Acetylation

ABSTRACT Regulation of chromatin through histone acetylation is an important step in gene expression. The Gcn5 histone acetyltransferase is part of protein complexes, e.g., the SAGA complex, that interact with transcriptional activators, targeting the enzyme to specific promoters and assisting in recruitment of the basal RNA polymerase transcription machinery. The Ada2 protein directly binds to Gcn5 and stimulates its catalytic activity. Drosophila contains two Ada2 proteins, Drosophila Ada2a (dAda2a) and dAda2b. We have generated flies that lack dAda2b, which is part of a Drosophila SAGA-like complex. dAda2b is required for viability in Drosophila, and its deletion causes a reduction in histone H3 acetylation. A global hypoacetylation of chromatin was detected on polytene chromosomes in dAda2b mutants. This indicates that the dGcn5-dAda2b complex could have functions in addition to assisting in transcriptional activation through gene-specific acetylation. Although the Drosophila p53 protein was previously shown to interact with the SAGA-like complex in vitro, we find that p53 induction of reaper gene expression occurs normally in dAda2b mutants. Moreover, dAda2b mutant animals show excessive p53-dependent apoptosis in response to gamma radiation. Based on this result, we speculate that dAda2b may be necessary for efficient DNA repair or generation of a DNA damage signal. This could be an evolutionarily conserved function, since a yeast ada2 mutant is also sensitive to a genotoxic agent.

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Regulation of SRC-3 (pCIP/ACTR/AIB-1/RAC-3/TRAM-1) Coactivator Activity by IκB Kinase

Molecular and Cellular Biology ◽

10.1128/mcb.22.10.3549-3561.2002 ◽

2002 ◽

Vol 22 (10) ◽

pp. 3549-3561 ◽

Cited By ~ 202

Author(s):

Ray-Chang Wu ◽

Jun Qin ◽

Yoshihiro Hashimoto ◽

Jiemin Wong ◽

Jianming Xu ◽

...

Keyword(s):

Gene Expression ◽

Inflammatory Responses ◽

Protein Complexes ◽

Biochemical Purification ◽

Necrosis Factor Alpha ◽

Iκb Kinase ◽

Ikk Complex ◽

Null Mutant Mice

ABSTRACT In the past few years, many nuclear receptor coactivators have been identified and shown to be an integral part of receptor action. The most frequently studied of these coactivators are members of the steroid receptor coactivator (SRC) family, SRC-1, TIF2/GRIP1/SRC-2, and pCIP/ACTR/AIB-1/RAC-3/TRAM-1/SRC-3. In this report, we describe the biochemical purification of SRC-1 and SRC-3 protein complexes and the subsequent identification of their associated proteins by mass spectrometry. Surprisingly, we found association of SRC-3, but not SRC-1, with the IκB kinase (IKK). IKK is known to be responsible for the degradation of IκB and the subsequent activation of NF-κB. Since NF-κB plays a key role in host immunity and inflammatory responses, we therefore investigated the significance of the SRC-3-IKK complex. We demonstrated that SRC-3 was able to enhance NF-κB-mediated gene expression in concert with IKK. In addition, we showed that SRC-3 was phosphorylated by the IKK complex in vitro. Furthermore, elevated SRC-3 phosphorylation in vivo and translocation of SRC-3 from cytoplasm to nucleus in response to tumor necrosis factor alpha occurred in cells, suggesting control of subcellular localization of SRC-3 by phosphorylation. Finally, the hypothesis that SRC-3 is involved in NF-κB-mediated gene expression is further supported by the reduced expression of interferon regulatory factor 1, a well-known NF-κB target gene, in the spleens of SRC-3 null mutant mice. Taken together, our results not only reveal the IKK-mediated phosphorylation of SRC-3 to be a regulated event that plays an important role but also substantiate the role of SRC-3 in multiple signaling pathways.

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Clock proteins regulate spatiotemporal organization of clock genes to control circadian rhythms

10.1101/2020.10.09.333732 ◽

2020 ◽

Author(s):

Yangbo Xiao ◽

Ye Yuan ◽

Mariana Jimenez ◽

Neeraj Soni ◽

Swathi Yadlapalli

Keyword(s):

Gene Expression ◽

Circadian Rhythms ◽

Nuclear Envelope ◽

Circadian Clock ◽

Clock Genes ◽

Circadian Clocks ◽

Spatiotemporal Organization ◽

Clock Proteins ◽

Expression Behavior ◽

Clock Protein

ABSTRACTCircadian clocks regulate ∼24 hour oscillations in gene expression, behavior, and physiology. While the molecular and neural mechanisms of circadian rhythms are well characterized, how cellular organization of clock components controls circadian clock regulation remains poorly understood. Here, we elucidate how clock proteins regulate circadian rhythms by controlling the spatiotemporal organization of clock genes. Using high-resolution live imaging techniques we demonstrate that Drosophila clock proteins are concentrated in a few discrete foci and are organized at the nuclear envelope; these results are in contrast to longstanding expectations that clock proteins are diffusely distributed in the nucleus. We also show that clock protein foci are highly dynamic and change in number, size, and localization over the circadian cycle. Further, we demonstrate that clock genes are positioned at the nuclear periphery by the clock proteins precisely during the circadian repression phase, suggesting that subnuclear localization of clock genes plays an important role in the control of rhythmic gene expression. Finally, we show that Lamin B receptor, a nuclear envelope protein, is required for peripheral localization of clock protein foci and clock genes and for normal circadian rhythms. These results reveal that clock proteins form dynamic nuclear foci and play a hitherto unexpected role in the subnuclear reorganization of clock genes to control circadian rhythms, identifying a novel mechanism of circadian regulation. Our results further suggest a new role for clock protein foci in the clustering of clock-regulated genes during the repression phase to control gene co-regulation and circadian rhythms.SIGNIFICANCEAlmost all living organisms have evolved circadian clocks to tell time. Circadian clocks regulate ∼24-hour oscillations in gene expression, behavior and physiology. Here, we reveal the surprisingly sophisticated spatiotemporal organization of clock proteins and clock genes and its critical role in circadian clock function. We show, in contrast to current expectations, that clock proteins are concentrated in a few discrete, dynamic nuclear foci at the nuclear envelope during the repression phase. Further, we uncovered several unexpected features of clock protein foci, including their role in positioning the clock genes at the nuclear envelope precisely during the repression phase to enable circadian rhythms. These studies provide fundamental new insights into the cellular mechanisms of circadian rhythms and establish direct links between nuclear organization and circadian clocks.

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TOR signaling modulates Cdk8-dependent GAL gene expression in Saccharomyces cerevisiae

10.1101/2020.05.15.097576 ◽

2020 ◽

Author(s):

Nicole Hawe ◽

Konstantin Mestnikov ◽

Riley Horvath ◽

Mariam Eji-Lasisi ◽

Cindy Lam ◽

...

Keyword(s):

Gene Expression ◽

Rna Polymerase Ii ◽

Nuclear Localization ◽

Kinase Activity ◽

Mediator Complex ◽

Tor Signaling ◽

A Subunit ◽

Insight Into

AbstractCdk8 of the RNA Polymerase II mediator complex regulates genes by phosphorylating sequence specific transcription factors. Despite conserved importance for eukaryotic transcriptional regulation, the signals regulating Cdk8 are unknown. Full induction of the yeast GAL genes requires phosphorylation of Gal4 by Cdk8, and we exploited this requirement for growth of gal3 yeast on galactose to identify mutants affecting Cdk8 activity. Several mutants from the screen produced defects in TOR signaling. A mutant designated gal four throttle (gft) 1, gft1, was identified as an allele of hom3, encoding aspartokinase. Defects in gft1/ hom3 caused hypersensitivity to rapamycin, and constitutive nuclear localization of Gat1. Furthermore, mutations of tor1 or tco89, encoding TORC1 components, also prevented GAL expression in gal3 yeast, and tco89 was determined to be allelic to gft7. Disruption of cdc55, encoding a subunit of PP2A regulated by TOR signaling, suppressed the effect of gft1/ hom3, gft7/ tco89, and tor1 mutations on GAL expression in gal3 yeast, but not of cdk8/ srb10 disruptions or Gal4 S699A mutation. Mutations of gft1/ hom3 and tor1 did not affect kinase activity of Cdk8 in vitro, but caused loss of Gal4 phosphorylation in vivo. These observations demonstrate that TOR signaling regulates GAL induction through the activity of PP2A/ Cdc55, and are consistent with the contention that Cdk8-dependent phosphorylation of Gal4 S699 is opposed by PP2A/ Cdc55 dephosphorylation. These results provide insight into how induction of transcription by a specific inducer can be modulated by global nutritional signals through regulation of Cdk8-dependent phosphorylation.

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Molecular Characterization of a PU.1 Transcription Complex Formed on the IL-1β Proximal Promoter.

Blood ◽

10.1182/blood.v104.11.3547.3547 ◽

2004 ◽

Vol 104 (11) ◽

pp. 3547-3547

Author(s):

Trang Hoang ◽

Benoit Grondin ◽

Martin Lefrancois ◽

Marianne St Denis ◽

Daniel G. Tenen ◽

...

Keyword(s):

Gene Expression ◽

Stress Response ◽

Dna Binding ◽

Leucine Zipper ◽

Protein Complexes ◽

Proximal Promoter ◽

Stress Exposure ◽

Protein Protein Interaction ◽

Nuclear Extracts

Abstract The gene coding for the pro-inflammatory cytokine IL-1β is induced at the transcription level in differentiating macrophages and in stress response. Interestingly, PU.1 and C/EBPβ, two transcription factors implicated in IL-1β gene expression are not induced by stress exposure, while c-Jun is strongly induced. Strikingly, this upregulation of c-Jun is required for IL-1β induction, as cells expressing a c-Jun antisense construct fail to respond to stress exposure. We have mapped the induction of IL-1β gene expression to its proximal promoter and show that it is mediated by the transcriptional synergy between C/EBPβ, c-Jun and PU.1 via specific DNA binding sites for C/EBPβ and PU.1 only. To elucidate how PU.1 and C/EBPβ cooperate with c-Jun at the molecular level, we have optimized a DNA binding assay based on IL-1β promoter fragments immobilized on beads to isolate protein complexes from nuclear extracts, which were subsequently eluted and identified by Western blotting. We show that PU.1 or C/EBPβ alone directly bind this promoter fragment via specific sequences while purified recombinant c-Jun fails to do so. However, the presence of either PU.1 or C/EBPβ on the promoter allows for a recruitment of c-Jun to the DNA template, mediated by direct protein-protein interaction. Interestingly, the leucine zipper domain of c-Jun is essential for its interaction with C/EBPβ while dispensable for PU.1 interaction in vitro whereas its basic domain is required for both interactions. Furthermore, we show that PU.1 and C/EBPβ cooperatively bind the IL-1β promoter, resulting in a synergistic recruitment of c-Jun. Finally, we show that the strength of interaction of c-Jun mutants with PU.1 or C/EBPβ determine the strength of transcription output and c-Jun mutants that fail to associate with either PU.1 or C/EBPβ are transcriptionally inactive. In contrast, c-Jun mutants exhibiting increased homodimerization are more active that the wild type protein. Taken together, our data suggest that c-Jun homodimers can be targeted to the IL-1β promoter in the absence of a specific DNA binding element, and conclude that PU.1 and C/EBPβ are specifically tethered to the IL-1β promoter while c-Jun cooperatively binds these proteins and acts as a transcriptional co-activator. We propose a mechanism based on an initial binding of PU.1 and C/EBPβ to the IL-1β promoter followed by a cooperative recruitment of c-Jun, resulting in transcriptional synergy and IL-1β gene expression in stress response.

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Analysis of the Sequence Conservation of the Circadian Clock Protein KaiC

Advanced Materials Research ◽

10.4028/www.scientific.net/amr.699.184 ◽

2013 ◽

Vol 699 ◽

pp. 184-188

Author(s):

Liu Sen ◽

Song Liu ◽

Fei Yun Chen

Keyword(s):

Circadian Rhythms ◽

Circadian Clock ◽

Feedback Loop ◽

Sequence Variation ◽

Protein Sequences ◽

Circadian System ◽

Site Variation ◽

Key Residues ◽

Clock Protein

Regulation of daily physiological functions with approximate a 24-hour periodicity, or circadian rhythms, is a characteristic of eukaryotes. So far, cyanobacteria are only known prokaryotes reported to possess circadian rhythmicity. The circadian system in cyanobacteria comprises both a post-translational oscillator (PTO) and a transcriptional/translational feedback loop (TTFL). The PTO can be reconstituted in vitro with three purified proteins (KaiA, KaiB, and KaiC) with the existence of ATP. Phase of the nanoclockwork has been associated with the phosphorylation states of KaiC, with KaiA promoting the phosphorylation of KaiC, and KaiB de-phosphorylating KaiC. Here we studied the sequence variation of 65 KaiC proteins in evolution, and determined some key residues in KaiC by analyzing the site variation rates of the protein sequences. These key residues could be used to study the key interactions of KaiC with KaiA and KaiB.

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A microtubule dynamics reconstitutional convention

The Journal of Cell Biology ◽

10.1083/jcb.201610066 ◽

2016 ◽

Vol 215 (3) ◽

pp. 305-307

Author(s):

Kevin C. Slep

Keyword(s):

Kinase Activity ◽

Biological Process ◽

Microtubule Dynamics ◽

The Core ◽

Polo Kinase ◽

Cell Biol ◽

In Vitro Reconstitution ◽

Core Components

In vitro reconstitution is the fundamental test for identification of the core components of a biological process. In this issue, Moriwaki and Goshima (2016. J. Cell Biol. https://doi.org/10.1083/jcb.201604118) reconstitute all phases of microtubule dynamics through the inclusion of five key regulators and demonstrate that Polo kinase activity shifts the system from an interphase mode into an enhanced mitotic mode.

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