A PEST-like element in FREQUENCY determines the length of the circadian period in Neurospora crassa
2001; Springer Nature; Volume: 20; Issue: 24 Linguagem: Inglês
10.1093/emboj/20.24.7074
ISSN1460-2075
Autores Tópico(s)Neurobiology and Insect Physiology Research
ResumoArticle17 December 2001free access A PEST-like element in FREQUENCY determines the length of the circadian period in Neurospora crassa Margit Görl Margit Görl Biochemie–Zentrum Heidelberg, Im Neuenheimer Feld 328, D-69120 Heidelberg, Germany Search for more papers by this author Martha Merrow Martha Merrow Institut für Medizinische Psychologie und Immunologie, Universität München, Goethestrasse 33, D-80336 Munich, Germany Search for more papers by this author Benedikt Huttner Benedikt Huttner Biochemie–Zentrum Heidelberg, Im Neuenheimer Feld 328, D-69120 Heidelberg, Germany Search for more papers by this author Judy Johnson Judy Johnson Institut für Medizinische Psychologie und Immunologie, Universität München, Goethestrasse 33, D-80336 Munich, Germany Search for more papers by this author Till Roenneberg Till Roenneberg Institut für Medizinische Psychologie und Immunologie, Universität München, Goethestrasse 33, D-80336 Munich, Germany Search for more papers by this author Michael Brunner Corresponding Author Michael Brunner Biochemie–Zentrum Heidelberg, Im Neuenheimer Feld 328, D-69120 Heidelberg, Germany Search for more papers by this author Margit Görl Margit Görl Biochemie–Zentrum Heidelberg, Im Neuenheimer Feld 328, D-69120 Heidelberg, Germany Search for more papers by this author Martha Merrow Martha Merrow Institut für Medizinische Psychologie und Immunologie, Universität München, Goethestrasse 33, D-80336 Munich, Germany Search for more papers by this author Benedikt Huttner Benedikt Huttner Biochemie–Zentrum Heidelberg, Im Neuenheimer Feld 328, D-69120 Heidelberg, Germany Search for more papers by this author Judy Johnson Judy Johnson Institut für Medizinische Psychologie und Immunologie, Universität München, Goethestrasse 33, D-80336 Munich, Germany Search for more papers by this author Till Roenneberg Till Roenneberg Institut für Medizinische Psychologie und Immunologie, Universität München, Goethestrasse 33, D-80336 Munich, Germany Search for more papers by this author Michael Brunner Corresponding Author Michael Brunner Biochemie–Zentrum Heidelberg, Im Neuenheimer Feld 328, D-69120 Heidelberg, Germany Search for more papers by this author Author Information Margit Görl1, Martha Merrow2, Benedikt Huttner1, Judy Johnson2, Till Roenneberg2 and Michael Brunner 1 1Biochemie–Zentrum Heidelberg, Im Neuenheimer Feld 328, D-69120 Heidelberg, Germany 2Institut für Medizinische Psychologie und Immunologie, Universität München, Goethestrasse 33, D-80336 Munich, Germany *Corresponding author. E-mail: [email protected] The EMBO Journal (2001)20:7074-7084https://doi.org/10.1093/emboj/20.24.7074 PDFDownload PDF of article text and main figures. ToolsAdd to favoritesDownload CitationsTrack CitationsPermissions ShareFacebookTwitterLinked InMendeleyWechatReddit Figures & Info FREQUENCY (FRQ) is a crucial element of the circadian clock in Neurospora crassa. In the course of a circadian day FRQ is successively phosphorylated and degraded. Here we report that two PEST-like elements in FRQ, PEST-1 and PEST-2, are phosphorylated in vitro by recombinant CK-1a and CK-1b, two newly identified Neurospora homologs of casein kinase 1ϵ. CK-1a is localized in the cytosol and the nuclei of Neurospora and it is in a complex with FRQ in vivo. Deletion of PEST-1 results in hypophosphorylation of FRQ and causes significantly increased protein stability. A strain harboring the mutant frqΔPEST-1 gene shows no rhythmic conidiation. Despite the lack of overt rhythmicity, frqΔPEST-1 RNA and FRQΔPEST-1 protein are rhythmically expressed and oscillate in constant darkness with a circadian period of 28 h. Thus, by deletion of PEST-1 the circadian period is lengthened and overt rhythmicity is dissociated from molecular oscillations of clock components. Introduction Most organisms use circadian clocks to regulate physiological and behavioral activities in a time-of-day specific manner. Circadian clocks are cell-autonomous and mediate rhythmic expression of a broad variety of clock-controlled genes with a periodicity of approximately one day even in the absence of environmental cues. Circadian clocks are entrainable by exogenous stimuli (zeitgebers) such as light, temperature and nutrition. Entrainment synchronizes the endogenous oscillations with the exogenous time and allows behavioral flexibility. On the molecular level circadian oscillations are supported by interconnected transcriptional–translational feedback loops of considerable complexity. The interconnected loops seem to function in a similar manner in fungi, flies and mammals (Dunlap et al., 1999; Young, 2000; Albrecht, 2001; Reppert and Weaver, 2001; Williams and Sehgal, 2001). The circadian system of Drosophila melanogaster is well characterized on the molecular level. Drosophila CLOCK (CLK) and CYCLE (CYC) are Per-Arnt-Sim-like (PAS) domain-containing transcription factors that control transcription of period (per) and timeless (tim) RNA (Allada et al., 1998; Darlington et al., 1998; Rutila et al., 1998; McDonald et al., 2001; Wang et al., 2001). When PER and TIM proteins are synthesized they form a complex that enters the nucleus and represses transcription of their own genes by inactivating CLK–CYC (Hardin et al., 1990; Saez and Young, 1996; Lee et al., 1998, 1999). During the course of a day PER and TIM are degraded, which again allows synthesis of per and tim RNA by CLK–CYC (Young, 2000; Williams and Sehgal, 2001). The length of a circadian period is affected by the kinetics of nuclear entry and degradation of PER–TIM. TIM is phosphorylated by SHAGGY, which regulates nuclear translocation of the PER–TIM heterodimer (Martinek et al., 2001). The casein kinase 1ϵ (CK-1ϵ) homolog DOUBLETIME (DBT) triggers degradation of PER via phosphorylation and thereby regulates period length (Price et al., 1998; Rothenfluh et al., 2000; Kloss et al., 2001). PER and TIM not only repress synthesis of their own genes but also support the expression of CLK (Bae et al., 1998; Glossop et al., 1999). Furthermore, TIM increases per RNA levels through a post-transcriptional mechanism (Suri et al., 1999). A central element of the circadian feedback loop of Neurospora crassa is frequency (frq). Expression of frq RNA depends on the oligomeric PAS domain containing transcription factors white collar (WC)-1 and WC-2 (Crosthwaite et al., 1997; Talora et al., 1999). On the other hand, FRQ controls the expression of wc-1 RNA (Merrow et al., 2001) and WC-1 (Lee et al., 2000; Cheng et al., 2001). As a consequence frq RNA and FRQ protein levels oscillate under free-running conditions (constant darkness) with a period of ∼22 h (Aronson et al., 1994; Garceau et al., 1997). frq RNA levels reach a maximum in the subjective late morning followed by a FRQ protein peak ∼4 h later (Garceau et al., 1997; Merrow et al., 1999). FRQ protein enters the nucleus and, when expressed at sufficiently high levels, represses synthesis of its own RNA (Aronson et al., 1994; Merrow et al., 1997; Luo et al., 1998). In the course of the day, FRQ protein is progressively hyperphosphorylated and then degraded. When FRQ protein levels fall below a threshold frq RNA is synthesized again and a new circadian period begins (Garceau et al., 1997). The roles of the multiple phosphorylations of FRQ are not known. However, phosphorylation of FRQ at Ser513 by an unidentified kinase affects protein stability and the length of the circadian period (Liu et al., 2000). FRQ contains two PEST-like sequences, PEST-1 and PEST-2 (Merrow and Dunlap, 1994). PEST sequences are rich in proline (P), aspartic and glutamic acid (E), serine (S), threonine (T) (Rogers et al., 1986). In many cases PEST sequences are implicated in the regulation of protein turnover (Rechsteiner and Rogers, 1996; Marchal et al., 2000; Roth and Davis, 2000). Here we show that PEST-1 and PEST-2 of FRQ are targets for phosphorylation in vitro by CK-1a and CK-1b, two newly identified casein kinases 1 of N.crassa. Deletion of PEST-1 results in loss of the circadian rhythm of conidiation. FRQΔPEST-1 is expressed at high levels; it is hypophosphorylated and significantly more stable than authentic FRQ. Unexpectedly, frqΔPEST-1 RNA and FRQΔPEST-1 protein as well as WC-1 protein oscillate under constant conditions with a period of ∼28 h. The deletion of the PEST-1 sequence in FRQ dissociates the overt conidiation rhythm of Neurospora from molecular oscillations of critical clock components. Results Phosphorylation of PEST sequences in FRQ by casein kinases 1 The length of a circadian period in Drosophila is regulated via phosphorylation of the clock protein PER by DBT, a homolog of human casein kinase 1ϵ (CK-1ϵ) (Kloss et al., 1998). Searching the Neurospora genome we found two CK-1 homologs, CK-1a, which is closely related to DBT, and CK-1b (Figure 1A and B). Attempts to inactivate CK-1a by repeat-induced point mutations (RIPs) (Selker and Garrett, 1988) were unsuccessful (data not shown), suggesting that the gene may be essential for cell viability. To characterize expression of CK-1a Neurospora was grown in the dark. Samples were harvested at 4 h intervals over a time course of 48 h and ck-1a RNA was analyzed by reverse transcription and real time quantitative polymerase chain reaction (RT–PCR) (Figure 1C) and northern blotting (not shown). ck-1a RNA was expressed at constant levels throughout the 48 h period. Figure 1.Identification of N.crassa casein kinases 1, N.c. CK-1a and N.c. CK-1b. (A) Sequence alignment of amino acid residues 1–298 of N.c. CK-1a and residues 1–302 of N.c. CK-1b with the N-terminal kinase domains of selected members of the casein kinase 1 family. The amino acid sequence of N.c. CK-1a is shown in the upper lane. Residues identical to N.c. CK-1a are indicated by a dot. (B) Phylogenetic relationship of members of the casein kinases 1 family. D.m. DBT: D.melanogaster DOUBLETIME; M.a. TAU: M.auratus casein kinase 1 TAU; S.c. HRR25, S.c. CK 1, S.c. CK 2 and S.c. CK 3: S.cerevisiae casein kinases 1; H.s. CK1α, H.s. CK1δ and H.s. CK1ϵ: Homo sapiens casein kinases 1α, 1δ and 1ϵ. (C) ck-1a RNA levels are constant throughout a circadian day. Light-grown Neurospora cultures were transferred to constant darkness (DD) and samples were harvested after the indicated time periods. From each sample total RNA was isolated and cDNA was prepared by using random hexamers for priming. Relative levels of ck-1 RNA and actin RNA were determined by reverse transcription and quantitative RT–PCR using the 5′ nuclease assay detection system (TaqMan™) as described in Materials and methods. For calibration, cDNA was prepared from serial dilutions of RNA from light-grown tissue. The relative ratios of ck-1/actin were plotted versus the corresponding time in DD. Download figure Download PowerPoint CK-1a does not contain a canonical nuclear import signal. Yet, when Neurospora cells were fractionated CK-1a was found in the cytosolic and in the nuclear fraction, similar to DBT in Drosophila (Figure 2A). To investigate whether CK-1a interacts with FRQ in vivo, total protein extracts were prepared from light-grown Neurospora and subjected to immunoprecipitation with affinity-purified antibodies against CK-1a (Figure 2B). CK-1a antibodies coprecipitated specifically FRQ while WC-1 was not precipitated (not shown). Neurospora cells were transferred to darkness and samples were harvested 8, 16 and 36 h after the light–dark (LD) transfer. Total cell lysates were prepared and subjected to immunoprecipitation with affinity-purified antibodies against CK-1a (Figure 2C). FRQ coimmunoprecipitated with CK-1a using extracts prepared at DD8, DD16 and DD36, suggesting that it was in a complex with FRQ throughout a circadian day. However, separation of the immunoprecipitates on long SDS gels revealed that forms of FRQ with low electrophoretic mobility were preferentially coprecipitated with CK-1a, suggesting that CK-1a is in a complex with highly phosphorylated FRQ. Thus, CK-1a either associates specifically with previously phosphorylated forms of FRQ or binds and rapidly phosphorylates FRQ such that complexes between CK-1a and non-phosphorylated FRQ may not accumulate. Figure 2.CK-1a is in a complex with FRQ. (A) Subcellular localization of CK-1a. Light-grown Neurospora cells were fractionated as described (Luo et al., 1998). Cytosolic and nuclear fractions (200 μg each) were analyzed by SDS–PAGE and western blotting with affinity-purified antibodies against CK-1a (αCK-1a) (upper panels) and monoclonal antibodies against Neurospora tubulin (lower panels). (B) Co-immunoprecipitation of FRQ with CK-1a. Total cell extracts from the indicated strains were subjected to immunoprecipitation with affinity-purified CK-1a antibodies. 1 vol. and 2 vol. Ab correspond to the amounts of αCK-1a purified from 0.2 ml and 0.4 ml serum, respectively. Samples (1/3 of total) were analyzed by SDS–PAGE and western blotting with the monoclonal antibody FRQm3G11 (upper panels) and αCK-1a (lower panels). (C) CK-1a is in a complex with hyperphosphorylated FRQ. Total cell extracts were prepared from cells that were grown for the indicated time periods in DD. Samples were subjected to immunoprecipitation with αCK-1a (2 vol. Ab). Total cell extracts (E) and immunoprecipitates (IP) were analyzed by SDS–PAGE and western blotting with FRQm3G11. Right lane: short exposure of the FRQ signal in DD36 extract. Low phosphorylated forms of FRQ are indicated by asterisks. Download figure Download PowerPoint We cloned the cDNAs encoding CK-1a and CK-1b, expressed His-tagged versions of both kinases in Escherichia coli and purified the recombinant proteins by Ni–NTA chromatography (see Materials and methods). The recombinant casein kinases were active in autophosphorylation assays and efficiently phosphorylated β-casein (not shown). In Saccharomyces cerevisiae, casein kinases 1 phosphorylate uracil permease within a PEST sequence and, thereby trigger turnover of the protein (Marchal et al., 2000). FRQ contains two PEST-like elements, PEST-1 and PEST-2 (Figure 3A, upper portion), which are conserved in FRQ proteins from other fungi (Merrow and Dunlap, 1994). The PEST-find scores of 16.4 and 11.3, respectively, are significantly above the threshold level (5.0) (Rogers et al., 1986). PEST-1 is located in the central portion of FRQ and comprises a short confined segment of 17 amino acid residues. PEST-2 is located in the C-terminal portion and is 50 amino acid residues in length. We investigated whether the PEST sequences of FRQ are targets for phosphorylation by CK-1a and CK-1b. Fusion proteins between glutathione S-transferase (GST) and PEST sequences were constructed, expressed and purified. GST–PEST-1 and GST–PEST-2 contain the predicted PEST-like sequences comprising residues 544–560 and 843–893 of FRQ, respectively (Figure 3A, lower portion). Neither CK-1a nor CK-1b phosphorylated GST, which was used as a control (Figure 3B). Similarly, purified maltose-binding protein was not phosphorylated by the recombinant casein kinases (data not shown). GST–PEST-1 was specifically phosphorylated by CK-1a but not by CK-1b (Figure 3B). GST–PEST-2 was efficiently phosphorylated by CK-1a and with lower efficiency by CK-1b. Thus, PEST-2 appears to be a target for both casein kinases 1, while PEST-1 is a candidate sequence for specific phosphorylation of FRQ by CK-1a, the Neurospora homolog of Drosophila DBT. Figure 3.Phosphorylation of PEST-like elements in FRQ by recombinant CK-1a and CK-1b. (A) Construction of GST fusion proteins. FRQ is schematically outlined in the upper portion. Two PEST-like elements were identified with ‘PEST-find’ (http://www.at.embnet.org/embnet/tools/bio/PESTfind). PEST-1 (score 16.4) and PEST-2 (score 11.3) are indicated with black boxes. The gray box corresponds to residues from 478–519 of FRQ. Ser513 is indicated by an asterisk. FRQ-derived sequences that were fused to GST (hatched box) are shown in the lower part. (B) Specific phosphorylation of GST–PEST-1 by CK-1a and of GST–PEST-2 by CK-1a and CK-1b. The indicated GST fusion proteins (500 ng) were incubated with 50 ng recombinant His-tagged CK-1a (upper panel) and CK-1b (lower panel) for 60 min at 37°C in the presence of [32P]γ-ATP (2 Ci/mmol). Samples were analyzed by SDS–PAGE and autoradiography. Download figure Download PowerPoint FRQ is phosphorylated at Thr501, Ser513 and Ser519 (Liu et al., 2000). To test whether these sites are phosphorylated by the Neurospora casein kinases 1, we constructed GST–S513, a fusion protein containing residues 478–519 of FRQ. Recombinant GST–S513 was neither phosphorylated by CK-1a nor by CK-1b (Figure 3B). Based on the evidence from in vitro phosphorylation assays, which must be interpreted with caution, FRQ might be phosphorylated by multiple kinases. However, a bona fide role of different kinases in the circadian system of Neurospora remains to be established. Deletion of PEST-1 in FRQ results in loss of overt rhythmicity Since PEST-1 was specifically phosphorylated by CK-1a, we deleted the region encoding PEST-1 (17 amino acid residues) from frq and expressed the mutant gene under control of its own promoter in a frq-less Neurospora strain (frq10) (Aronson et al., 1994). When the resulting strain, frqΔPEST-1, was grown on race tubes in DD, no rhythmic conidiation (banding) was observed (Figure 4A). However, frqΔPEST-1 was growing with unregulated conidiation, while frq10 did not form conidia under these conditions. A control strain transformed with the wild-type frq gene showed a normal banding pattern with a periodicity of ∼22 h (not shown). Thus, deletion of the PEST-1 region of FRQ results in the loss of overt rhythmicity. Figure 4.frqΔPEST-1 has lost the overt conidiation rhythm. (A) Race tubes were inoculated with frqΔPEST-1, wild type (frq+) and frq null (frq10) and incubated at 25°C in DD. Upper panel: three replicate race tubes from each strain are shown. Lower panel: average conidial densities of triplicate race tubes. (B) frq+ and frqΔPEST-1 show driven conidial banding in 18 h/18 h, 9 h/9 h and 6 h/6 h LD cycles. Race tubes inoculated with the indicated strains were exposed to symmetrical LD cycles. The conidial densities of race tubes were determined and the averages of triplicates were plotted versus the time. The durations of the LD cycles are indicated. The gray background bars correspond to dark periods. Data of frq10 are shown only from the 6 h/6 h LD cycle; frq10 displayed no conidiation rhythm under all tested conditions. Download figure Download PowerPoint Why is conidiation of frqΔPEST-1 arrhythmic in DD? To assess whether frqΔPEST-1 had generally lost the ability to form conidial bands, race tubes were inoculated with frq+, frqΔPEST-1 and frq10 and then exposed to symmetric LD cycles of different length (Figure 4B). frq+ showed banding in LD cycles while frq10 does not band under these conditions (Figure 4B, bottom panel and data not shown), confirming that light-regulated conidial banding requires functional FRQ (Chang and Nakashima, 1997; Merrow et al., 1999; Lakin-Thomas and Brody, 2000). Interestingly, frqΔPEST-1 banded in LD cycles that varied in length between 18 h/18 h and 6 h/6 h. In LD cycles conidiation is driven by light. In 12 h/12 h and longer cycles conidial bands are formed towards the end of the dark phase, while in shorter cycles conidiation, though initiated in the dark, is pushed into the light phase of the following day. This indicates that frqΔPEST-1 has the capacity to form bands when conidiation is driven by light. However, since frqΔPEST-1 does not band in DD it has apparently lost the ability to coordinate conidiation in a temporal fashion under constant conditions. Physical and functional properties of FRQΔPEST-1 To characterize expression of the mutant FRQΔPEST-1 protein, total cell extracts were analyzed from wild-type and mutant strains that were grown in constant light (LL) (Figure 5A, left panel). As estimated by densitometry FRQΔPEST-1 was expressed at ∼3-fold higher levels than FRQ (not shown). Levels of frqΔPEST-1 RNA were slightly lower than levels of frq+ RNA (Figure 5A, right panel), suggesting that the elevated levels of FRQΔPEST-1 were due to an increased stability of the mutant protein (see below). Figure 5.Expression and phosphorylation profile of FRQΔPEST-1. (A) Left panel: protein extracts (200 μg) from light-grown frq+ and frqΔPEST-1 were analyzed by SDS–PAGE and western blotting with the monoclonal anti-FRQm3G11 antibody (αFRQ) (Merrow et al., 2001). Right panel: total RNA was prepared from light-grown strains. frq+ and frqΔPEST-1RNA were quantified by RT–PCR (as described in the legend to Figure 1C). (B) FRQΔPEST-1 is hypophosphorylated. Left panel: total protein extracts from the indicated light-grown strains. Major forms of FRQ that differ in electrophoretic mobility are indicated by asterisks. frq9: frameshift mutant with truncated FRQ; frq10: frq null mutant; frq+: wild-type frq; frq+ (pBM60-wt): frq10 transformed with pBM60 harboring wild-type frq; frqΔPEST-1: frq10 transformed with pBM60 harboring frqΔPEST-1. Central panel: protein extracts were subjected to immunoprecipitation with αFRQ and the precipitates were treated with 1000 U of λ-phosphatase (λ-PPase). Right panel: FRQ and FRQΔPEST-1 were synthesized by coupled in vitro transcription/translation in reticulocyte lysate (Retic. lysate). Samples were analyzed by SDS–PAGE and immunoblotting with αFRQ. Download figure Download PowerPoint The phosphorylation pattern of FRQΔPEST-1 differed, however, significantly from that of FRQ. Light-grown control cells accumulated three major forms of FRQ that differed in electrophoretic mobility (Figure 5B). In contrast, only two major forms of FRQΔPEST-1 were observed. The mobility shifts were due to phosphorylation, since treatment of FRQ with phosphatase prior to SDS–PAGE resulted predominantly in a form of FRQ that co-migrated with in vitro synthesized, non-phosphorylated FRQ. Similarly, phosphatase treatment of FRQΔPEST-1 resulted in a species that co-migrated with in vitro synthesized FRQΔPEST-1 (Figure 5B). Due to the deletion of the PEST-1 region non-phosphorylated FRQΔPEST-1 migrated with a slightly higher mobility than non-phosphorylated FRQ. Thus, the absence of one of the three phosphorylated species in FRQΔPEST-1 indicates that the PEST-1 region is either a direct target for phosphorylation and/or required to direct phosphorylation at other sites. We then analyzed physical properties of FRQΔPEST-1. Deletion of PEST-1 did not alter the subcellular localization of the mutant protein as determined by subcellular fractionation and western blotting (not shown). Sedimentation analysis in sucrose density gradient suggested that the oligomeric state of FRQ (Denault et al., 2001) was not affected by deletion of the PEST-1 sequence (not shown). When Neurospora is transferred from dark to light, synthesis of frq and wc-1 RNA are induced (Crosthwaite et al., 1997; Linden and Macino, 1997). The levels of light-induced RNAs are dependent on FRQ (Heintzen et al., 2001; Merrow et al., 2001). To assess functional properties of FRQΔPEST-1, we measured light inducibility of frq RNA and wc-1 RNA. In frq+ cells both RNAs were rapidly induced by light (Figure 6A, left panels). As expected, RNA levels reached a maximum after ∼10 min and adapted to low levels after longer light exposure of the cells (Arpaia et al., 1999; Heintzen et al., 2001). Similarly, frqΔPEST-1 RNA and wc-1 RNA were rapidly induced by light in frqΔPEST-1 cells and adapted subsequently to lower levels (Figure 6A, right panels). Thus, FRQΔPEST-1 supports inducibility by light as well as adaptation to light of wc-1 and frqΔPEST-1 RNA. Figure 6.Properties of frqΔPEST-1. (A) FRQΔPEST-1 supports light induction of frq and wc-1 RNA. frq+ and frqΔPEST-1 were grown in the dark for 28 h and then exposed to saturating light. Samples were harvested after the indicated time periods and RNA were prepared. frq RNA, frqΔPEST-1 RNA, wc-1 RNA and ribosomal RNA were detected by northern blot analysis and signals were quantified as described (Merrow et al., 2001). The data were normalized to the amount of ribosomal RNA (RNA/rib.RNA). The maximal signal was set to 100. Data are the average of duplicates. (B) Expression levels in LL of FRQΔPEST-1 and WC-1 are elevated in frqΔPEST-1. Protein extracts (200 μg) from frq+ (WT) and frqΔPEST-1 (Δ) were analyzed by SDS–PAGE and immunoblotting with the monoclonal antibodies αFRQ and anti-WC-1m4H4 (αWC-1). (C) FRQΔPEST-1 supports negative feedback after LD transfer. Light-grown frq+ and frqΔPEST-1 cells were transferred to darkness. After the indicated time periods mycelial pads were harvested and RNA was prepared. frq RNA (left panel) and frqΔPEST-1 RNA (right panel) were analyzed by northern blotting and quantified. The maximal signals were set equal to 100. Data are the average of duplicate experiments. (D) Turnover of FRQ and FRQΔPEST-1 after LD transition. Light-grown frq+ and frqΔPEST-1 cells were transferred to the dark and protein extracts were prepared after the indicated time periods. Samples were analyzed by SDS–PAGE and western blotting (upper panels). FRQ was detected by ECL and quantified by densitometry of X-ray films (lower panels). The solid lines represent exponential curve fits (data from t = 0 h were not included). One representative experiment out of three is shown. (E) Stability of FRQΔPEST-1 after the addition of CHX. Cultures were grown in LL for 2 days prior to addition of CHX at time point 0 h. Samples were harvested after the indicated time periods, analyzed by western blotting with αFRQ antibodies and quantified. Download figure Download PowerPoint FRQ facilitates expression of WC-1 in a post-transcriptional manner (Lee et al., 2000; Cheng et al., 2001). Since FRQΔPEST-1 was expressed at high levels, we compared expression levels of WC-1 in light-grown frqΔPEST-1 and frq+. Equal amounts of total cell extracts were analyzed by SDS–PAGE and western blotting (Figure 6B). WC-1 was expressed in frqΔPEST-1 at significantly higher levels than in frq+. wc-1 RNA levels were similar in both strains (not shown), indicating that FRQΔPEST-1 supports the expression of WC-1 in a manner similar to that proposed for FRQ (Lee et al., 2000). Synthesis of frq RNA is repressed when Neurospora cells are transferred from light to darkness. We measured the kinetics of RNA repression in frq+ and frqΔPEST-1 (Figure 6C). In both strains frq RNA levels decreased within 30 min after LD transfer. When frq9 was transferred from light to dark, no significant reduction in the amount of frq9 RNA was observed (not shown and Merrow et al., 1999). This demonstrates that deletion of PEST-1 does not compromise the ability of the cells to negatively feed back on frq transcription. We then measured the kinetics of turnover of FRQ and FRQΔPEST-1 protein. Light-grown cells were transferred to dark to repress new synthesis of frq and frqΔPEST-1 RNA. Subsequently samples were analyzed over a time course of 20 h. Following the LD transfer FRQ and FRQΔPEST-1 were hyperphosphorylated. Due to changes in the phosphorylation pattern it was difficult to compare protein levels between 0 and 2 h (Figure 6D, upper panel). Yet, levels did not appear to change significantly. Subsequently FRQ was rapidly degraded with a half-life of 2.7 ± 0.2 h (Figure 6D, lower panels). In comparison, degradation of FRQΔPEST-1 was slow. The half-life for turnover was 5.6 ± 0.3 h, indicating that the mutant protein was significantly more stable than authentic FRQ. After 16 h in DD hyperphosphorylated FRQ was completely degraded and new synthesis of low phosphorylated forms of FRQ was observed, demonstrating that a new circadian oscillation had commenced. No new synthesis of FRQΔPEST-1 occurred in the observed 20 h time period. To confirm the differences in protein stability, frq and frqΔPEST-1 cells were treated with cycloheximide (CHX) to inhibit protein synthesis, and samples were analyzed over a 16 h period. Again, turnover of FRQ was faster than the turnover of FRQΔPEST-1 (Figure 6E). The overall kinetics of degradation of both proteins were, however, slower in the presence of CHX than in the absence of the drug. FRQ was degraded with a half-life of 3.7 h, while the half-life of degradation of FRQΔPEST-1 was 7.7 h. The slower degradation kinetics may be due to pleiotropic effects of CHX and indicate that ongoing protein synthesis is required for the turnover of FRQ at physiological rates. In summary, the data show that deletion of PEST-1 results in a pronounced stabilization of FRQΔPEST-1 protein. Rhythmicity of frqΔPEST-1 on the molecular level The deletion of PEST-1 does not interfere with crucial FRQ-dependent properties such as regulation of conidiation by light, adaptation of RNA expression levels to light and negative feedback on frq RNA synthesis after LD transfer of cells (see above). We therefore tested whether components of the circadian clock are rhythmically expressed in frqΔPEST-1 cells despite the lack of an overt conidiation rhythm. frqΔPEST-1 cells were grown in liquid culture and harvested at 3 h intervals spanning a time period of 48 h. As a control, frq+ cells were harvested at 4 h intervals over the same period. Total cell lysates of each time point were subjected to western blot analysis. As expected, FRQ was hyperphosphorylated and rapidly turned over (Figure 7A and B, upper panels). New synthesis of unphosphorylated FRQ was observed after 16 h in DD. Surprisingly FRQΔPEST-1 was also rhythmically expressed (Figure 7A and B, central panels). After LD transfer FRQΔP
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