113 research outputs found
Septum formation is regulated by the RHO4-specific exchange factors BUD3 and RGF3 and by the landmark protein BUD4 in Neurospora crassa
P>Rho GTPases have multiple, yet poorly defined functions during cytokinesis. By screening a Neurospora crassa knock-out collection for Rho guanine nucleotide exchange factor (GEF) mutants that phenocopy rho-4 defects (i.e. lack of septa, slow growth, abnormal branching and cytoplasmic leakage), we identified two strains defective in homologues of Bud3p and Rgf3 of budding and fission yeast respectively. The function of these proteins as RHO4-specific GEFs was determined by in vitro assays. In vivo microscopy suggested that the two GEFs and their target GTPase act as two independent modules during the selection of the septation site and the actual septation process. Furthermore, we determined that the N. crassa homologue of the anillinrelated protein BUD4 is required for septum initiation and that its deficiency leads to typical rho4 defects. Localization of BUD4 as a cortical ring prior to septation initiation was independent of functional BUD3 or RGF3. These data position BUD4 upstream of both RHO4 functions in the septation process and make BUD4 a prime candidate for a cortical marker protein involved in the selection of future septation sites. The persistence of both BUD proteins and of RHO4 at the septal pore suggests additional functions of these proteins at mature septa.DFG [SPP1111
Phospho-regulation of the Neurospora crassa septation initiation network.
Proper cell division is essential for growth and development of uni- and multicellular organisms. The fungal septation initiation network (SIN) functions as kinase cascade that connects cell cycle progression with the initiation of cytokinesis. Miss-regulation of the homologous Hippo pathway in animals results in excessive cell proliferation and formation of tumors, underscoring the conservation of both pathways. How SIN proteins interact and transmit signals through the cascade is only beginning to be understood. Moreover, our understanding of septum formation and its regulation in filamentous fungi, which represent the vast majority of the fungal kingdom, is highly fragmentary. We determined that a tripartite kinase cascade, consisting of CDC-7, SID-1 and DBF-2, together with their regulatory subunits CDC-14 and MOB-1, is important for septum formation in the model mold Neurospora crassa. DBF-2 activity and septum formation requires auto-phosphorylation at Ser499 within the activation segment and phosphorylation of Thr671 in the hydrophobic motif by SID-1. Moreover, SID-1-stimulated DBF-2 activity is further enhanced by CDC-7, supporting a stepwise activation mechanism of the tripartite SIN kinase cascade in fungi. However, in contrast to the situation described for unicellular yeasts, the localization of the entire SIN cascade to spindle pole bodies is constitutive and cell cycle independent. Moreover, all SIN proteins except CDC-7 form cortical rings prior to septum initiation and localize to constricting septa. Thus, SIN localization and activity regulation significantly differs in unicellular versus syncytial ascomycete fungi
Fungal communication requires the MAK-2 pathway elements STE-20 and RAS-2, the NRC-1 adapter STE-50 and the MAP kinase scaffold HAM-5.
Intercellular communication is critical for the survival of unicellular organisms as well as for the development and function of multicellular tissues. Cell-to-cell signaling is also required to develop the interconnected mycelial network characteristic of filamentous fungi and is a prerequisite for symbiotic and pathogenic host colonization achieved by molds. Somatic cell-cell communication and subsequent cell fusion is governed by the MAK-2 mitogen activated protein kinase (MAPK) cascade in the filamentous ascomycete model Neurospora crassa, yet the composition and mode of regulation of the MAK-2 pathway are currently unclear. In order to identify additional components involved in MAK-2 signaling we performed affinity purification experiments coupled to mass spectrometry with strains expressing functional GFP-fusion proteins of the MAPK cascade. This approach identified STE-50 as a regulatory subunit of the Ste11p homolog NRC-1 and HAM-5 as cell-communication-specific scaffold protein of the MAPK cascade. Moreover, we defined a network of proteins consisting of two Ste20-related kinases, the small GTPase RAS-2 and the adenylate cyclase capping protein CAP-1 that function upstream of the MAK-2 pathway and whose signals converge on the NRC-1/STE-50 MAP3K complex and the HAM-5 scaffold. Finally, our data suggest an involvement of the striatin interacting phosphatase and kinase (STRIPAK) complex, the casein kinase 2 heterodimer, the phospholipid flippase modulators YPK-1 and NRC-2 and motor protein-dependent vesicle trafficking in the regulation of MAK-2 pathway activity and function. Taken together, these data will have significant implications for our mechanistic understanding of MAPK signaling and for homotypic cell-cell communication in fungi and higher eukaryotes
Proper actin ring formation and septum constriction requires coordinated regulation of SIN and MOR pathways through the germinal centre kinase MST-1.
Nuclear DBF2p-related (NDR) kinases constitute a functionally conserved protein family of eukaryotic regulators that control cell division and polarity. In fungi, they function as effector kinases of the morphogenesis (MOR) and septation initiation (SIN) networks and are activated by pathway-specific germinal centre (GC) kinases. We characterized a third GC kinase, MST-1, that connects both kinase cascades. Genetic and biochemical interactions with SIN components and life cell imaging identify MST-1 as SIN-associated kinase that functions in parallel with the GC kinase SID-1 to activate the SIN-effector kinase DBF-2. SID-1 and MST-1 are both regulated by the upstream SIN kinase CDC-7, yet in an opposite manner. Aberrant cortical actomyosin rings are formed in Δmst-1, which resulted in mis-positioned septa and irregular spirals, indicating that MST-1-dependent regulation of the SIN is required for proper formation and constriction of the septal actomyosin ring. However, MST-1 also interacts with several components of the MOR network and modulates MOR activity at multiple levels. MST-1 functions as promiscuous enzyme and also activates the MOR effector kinase COT-1 through hydrophobic motif phosphorylation. In addition, MST-1 physically interacts with the MOR kinase POD-6, and dimerization of both proteins inactivates the GC kinase hetero-complex. These data specify an antagonistic relationship between the SIN and MOR during septum formation in the filamentous ascomycete model Neurospora crassa that is, at least in part, coordinated through the GC kinase MST-1. The similarity of the SIN and MOR pathways to the animal Hippo and Ndr pathways, respectively, suggests that intensive cross-communication between distinct NDR kinase modules may also be relevant for the homologous NDR kinases of higher eukaryotes
RHO1 and RHO2 share partially overlapping functions in the regulation of cell wall integrity and hyphal polarity in Neurospora crassa
Rho proteins are key regulators of cellular morphogenesis, but their function in filamentous fungi is poorly understood. By generating conditional rho-1 mutants, we dissected the function of the essential GTPase RHO1 in cell polarization and maintenance of cell wall integrity in Neurospora crassa. We identified NCU00668/RGF1 as RHO1-specific exchange factor, which controls actin organization and the cell wall integrity MAK1 MAP kinase pathway through the direct interaction of active RHO1 with the formin BNI1 and PKC1 respectively. The activity of RGF1 is controlled by an intramolecular interaction of its DEP and GEF domains that blocks the activation of the GTPase. Moreover, the N-terminal region including the DEP domain of RGF1 interacts with the plasma membrane sensor NCU06910/WSC1, potentially to activate the cell wall integrity pathway. RHO1 also functions as regulatory subunit of the glucan synthase. N. crassa possesses a second GTPase, RHO2, that is highly homologous to RHO1. RHO2 is of minor importance for growth and does not interact with BNI1. Conditional rho-1;rho-2 double mutants display strong synthetic growth and cell polarity defects. We show that RHO2 does not regulate glucan synthase activity and the actin cytoskeleton, but physically interacts with PKC1 to regulate the cell wall integrity pathway
HAM-2 and HAM-3 are central for the assembly of the Neurospora STRIPAK complex at the nuclear envelope and regulate nuclear accumulation of the MAP kinase MAK-1 in a MAK-2-dependent manner
Intercellular communication and somatic cell fusion are important for fungal colony establishment, multicellular differentiation and have been associated with host colonization and virulence of pathogenic species. By a combination of genetic, biochemical and live cell imaging techniques, we characterized the Neurospora crassaSTRIPAK complex that is essential for self-signalling and consists of the six proteins HAM-2/STRIP, HAM-3/striatin, HAM-4/SLMAP, MOB-3/phocein, PPG-1/PP2A-C and PP2A-A. We describe that the core STRIPAK components HAM-2 and HAM-3 are central for the assembly of the complex at the nuclear envelope, while the phosphatase PPG-1 only transiently associates with this central subcomplex. Our data connect the STRIPAK complex with two MAP kinase pathways: (i) nuclear accumulation of the cell wall integrity MAP kinase MAK-1 depends on the functional integrity of the STRIPAK complex at the nuclear envelope, and (ii) phosphorylation of MOB-3 by the MAP kinase MAK-2 impacts the nuclear accumulation of MAK-1. In summary, these data support a model, in which MAK-2-dependent phosphorylation of MOB-3 is part of a MAK-1 import mechanism. Although self-communication remained intact in the absence of nuclear MAK-1 accumulation, supporting the presence of multiple mechanisms that co-ordinate robust intercellular communication, proper fruiting body morphology was dependent on the MAK-2-phosphorylated N-terminus of MOB-3
The essential phosphoinositide kinase MSS-4 is required for polar hyphal morphogenesis, localizing to sites of growth and cell fusion in Neurospora crassa.
Fungal hyphae and plant pollen tubes are among the most highly polarized cells known and pose extraordinary requirements on their cell polarity machinery. Cellular morphogenesis is driven through the phospholipid-dependent organization at the apical plasma membrane. We characterized the contribution of phosphoinositides (PIs) in hyphal growth of the filamentous ascomycete Neurospora crassa. MSS-4 is an essential gene and its deletion resulted in spherically growing cells that ultimately lyse. Two conditional mss-4-mutants exhibited altered hyphal morphology and aberrant branching at restrictive conditions that were complemented by expression of wild type MSS-4. Recombinant MSS-4 was characterized as a phosphatidylinositolmonophosphate-kinase phosphorylating phosphatidylinositol 4-phosphate (PtdIns4P) to phosphatidylinositol 4,5-bisphosphate (PtdIns(4,5)P(2)). PtdIns3P was also used as a substrate. Sequencing of two conditional mss-4 alleles identified a single substitution of a highly conserved Y750 to N. The biochemical characterization of recombinant protein variants revealed Y750 as critical for PI4P 5-kinase activity of MSS-4 and of plant PI4P 5-kinases. The conditional growth defects of mss-4 mutants were caused by severely reduced activity of MSS-4(Y750N), enabling the formation of only trace amounts of PtdIns(4,5)P(2). In N. crassa hyphae, PtdIns(4,5)P(2) localized predominantly in the plasma membrane of hyphae and along septa. Fluorescence-tagged MSS-4 formed a subapical collar at hyphal tips, localized to constricting septa and accumulated at contact points of fusing N. crassa germlings, indicating MSS-4 is responsible for the formation of relevant pools of PtdIns(4,5)P(2) that control polar and directional growth and septation. N. crassa MSS-4 differs from yeast, plant and mammalian PI4P 5-kinases by containing additional protein domains. The N-terminal domain of N. crassa MSS-4 was required for correct membrane association. The data presented for N. crassa MSS-4 and its roles in hyphal growth are discussed with a comparative perspective on PI-control of polar tip growth in different organismic kingdoms
Sorgerecht und Geschlecht – Eine historische Skizze
Autorin: Dr. Maya Halatcheva-Trapp „Die Macht des Vaters war immer heilig“, denn – so die französische Historikerin Yvonne Knibiehler – sie verband „die väterliche mit der göttlichen Herrschaft“ und beruhte gleichermaßen auf religiöser Mystifizierung und juristischer Privilegierung des Mannes in der Familie. [1] Entlang dieser symbolischen und rechtlich kodifizierten Macht wurden über Jahrhunderte hinweg die Sorge- und Geschlechter-verhältnisse im Abendland kulturell entworfen und legitimie..
Characterization of NDR kinase signalling pathways during septum formation in Neurospora crassa
Die Zellteilung/Zytokinese ist ein grundlegender zellulärer Prozess und essentiell für das Wachstum von einzelligen und mehrzelligen Organismen. Reguliert wird dieser Prozess durch komplexe molekulare Mechanismen sowie einer Vielzahl von interaktiven Netzwerken. In Pilzen koordiniert eine Kinase-Kaskade, das Septierungs-Initiierungs Netzwerk (SIN) das Fortschreiten des Zellzyklus mit dem Beginn der Zellteilung und kontrolliert die Septenbildung. Fehlregulation des homologen Hippo Netzwerks in Tieren führt zu Gewebewucherungen und Tumorbildung, was die konservierte Bedeutung dieser Regulationsnetzwerke in verschiedenen Organismen unterstreicht. Obwohl die Septenbildung essentiell für das Wachstum und die Differenzierung von Schimmelpilzen ist, bleibt die Frage wie die Septierung reguliert wird und aus welchen Komponenten sich das SIN Netzwerk in filamentösen Pilzen zusammensetzt bisher noch unbeantwortet.
Mit Hilfe von in silico Analysen konnten homologe Proteine für fast alle SIN Netzwerk Komponenten im Modellorganismus Neurospora crassa identifiziert werden. Die Analyse dieser vorhergesagten SIN Komponenten ermöglichte die Charakterisierung der SIN-Kinase-Kaskade, bestehend aus CDC-7, SID-1 und DBF-2 sowie den entsprechenden, regulatorischen Untereinheiten CDC-14 und MOB-1. Es konnte gezeigt werden, dass DBF-2 durch SID-1 am hydrophoben Motiv phosphoryliert und aktiviert wird und dass eine SID-1 abhängige Stimulation von DBF-2 durch Zugabe von CDC-7 weiter gesteigert wird. Diese Daten liefern den ersten biochemischen Nachweis für die schrittweise Aktivierung einer dreistufigen SIN-Kinase-Kaskade in Pilzen. Es wurde weiterhin gezeigt, dass die gesamte SIN Kaskade konstitutiv und Zellzyklus unabhängig an den Spindelpolkörpern akkumuliert und dass alle SIN Proteine an kontrahierenden Septen lokalisieren. Demzufolge ist im Gegensatz zu den einzelligen Pilzen die Lokalisation und Aktivität der SIN Komponenten in Synzytium-bildenden Ascomyzeten Zellzyklus unabhängig. Darüber hinaus deutet die Charakterisierung von DBF-2 Mutanten, in denen die beiden regulatorischen Aminosäuren (Ser499 and Thr671) mutiert sind, darauf hin, dass ein dynamischer Phosphorylierungs-/Dephosphorylierungszyklus des Ser499 entscheidend für die Aktivität und Funktion von DBF-2 in N. crassa ist. Diese Daten haben Einfluss auf das allgemeine Verständnis der Aktivierung von NDR Kinasen, denn bisher wurde für NDR Kinasen höherer Eukaryonten eine folgegebundene Phosphorylierung beider regulatorischer Reste angenommen.
Der Ste20-verwandten Kinase MST-1 konnte eine Funktion als SIN-assoziierte Kinase, die parallel zu SID-1 agiert, zugeordnet werden. SID-1 und MST-1 werden auf entgegengesetzte Weise von der oberhalb agierenden SIN Kinase CDC-7 reguliert, was nahelegt, dass MST-1 für die Feinabstimmung des SIN erforderlich ist. Lifeact- und Formin-GFP Reporter Konstrukte zeigten, dass in der Δmst-1 Mutante abnormale, kortikale Actomyosin-Ringe gebildet werden, was eine Fehlpositionierung der Septen und die Bildung von unregelmäßigen Spiralen zur Folge hat. Diese Defekte entsprechen partiell jenen der MOR Mutanten. Diese Mutanten weisen ein defektes NDR Kinase Netzwerk auf, welches für das polare Wachstum verantwortlich ist (MOR). Es stellte sich heraus, dass MST-1 mit den zentralen MOR Kinasen POD-6 und COT-1 interagiert und sowohl die SIN Effektor Kinase DBF-2 als auch die MOR Effektor Kinase COT-1 aktiviert. Somit fungiert MST-1 als dual-spezifisches Enzym. Eine weitere Vernetzung beider Signalwege ist durch die Bildung von Heterodimeren gegeben.
Die in dieser Studie identifizierten verschiedenen Ebenen der Vernetzung des SIN und MOR, sowie entsprechende Daten aus anderen Modellorganismen wie S. pombe und D. melanogaster, lassen vermuten, dass antagonistische Interaktionen zwischen homologen NDR Kinase Netzwerken ein genereller Mechanismus zur Koordination beider Signalwege darstellt und auch in höheren Organismen konserviert ist.
Durch die Annotierung mehrerer Pilzgenome wurden zahlreiche Gene mit einer Homologie zu den S. cerevisiae BUD Genen auch in filamentösen Pilzen identifiziert. Epistatische und biochemische Analysen ergaben, dass das MOR Netzwerk als negativer Regulator der Septenbildung oberhalb des BUD komplex fungiert und dass COT-1 im Gegensatz zu DBF-2, die beiden Septierungsmarkerproteine BUD-3/BUD-4 phosphoryliert. Folglich könnte die Regulation von BUD-3 (und eventuell auch BUD-4) durch COT-1 ein Mechanismus des MOR Netzwerks sein, um die Septenbildung in N. crassa zu inhibieren.Cytokinesis is a fundamental cellular process essential for cell proliferation of unicellular and multicellular organisms. The molecular pathways that regulate cytokinesis are highly complex and involve a large number of components that form elaborate interactive networks. The fungal septation initiation network (SIN) functions as kinase cascade that connects cell cycle progression with the initiation of cytokinesis and control septum formation. Miss-regulation of the homologous Hippo pathway in animals results in excessive proliferation and formation of tumors, underscoring the conservation and importance of these kinase networks. While septum formation is essential for proper growth and differentiation of molds, the regulation of septation and the composition of the SIN in filamentous fungi are only beginning to be unraveled.
The in silico analysis of the genome of the model mold Neurospora crassa identified homologs for most SIN network components. Analysis of these predicted SIN proteins allowed the characterization of the SIN kinase cascade consisting of CDC-7, SID-1 and DBF-2 together with their regulatory subunits CDC-14 and MOB-1, respectively. It was determined that SID-1 activates DBF-2 through hydrophobic motif phosphorylation and that SID-1-stimulated DBF-2 activity is further enhanced by CDC-7, providing the first biochemical evidence for a stepwise activation of the tripartite SIN kinase cascade in fungi. The entire SIN cascade localizes in a constitutive and cell cycle independent manner to spindle pole bodies and all SIN proteins accumulated at forming septa. Thus, in contrast to unicellular fungi the SIN localization and activity regulation is cell-cycle independent in syncytial ascomycetes. Moreover, the characterization of DBF-2 variants harbouring mutations in the two regulatory sites (Ser499 and Thr671) suggest that a dynamic phosphorylation/dephosphorylation cycle of Ser499 may be critical for N. crassa DBF-2 activity and function. These data have implications for NDR kinase activity regulation in general, because the sequential phosphorylation of both regulatory sites has been so far predicted for NDR kinases of higher eukaryotes.
The Ste20-related kinase MST-1 was identified as SIN-associated kinase acting in parallel to SID-1. SID-1 and MST-1 were both regulated by the upstream SIN kinase CDC-7, yet in an opposite manner, suggesting that MST-1 is required for fine-tuning the SIN. Lifeact- and formin-GFP reporter constructs revealed the formation of aberrant cortical actomyosin rings in ∆mst-1, which resulted in miss-positioned septa and irregular spirals. These defects phenocopy those of mutants defective in a NDR kinase pathway required for cell polarization called MOR, and it was determined that MST-1 also interacted with the central MOR kinases POD-6 and COT-1. MST-1 functions as promiscuous enzyme by activating the SIN and MOR effector kinases DBF-2 and COT-1. Moreover, crosstalk of the SIN and MOR pathways is also achieved by heterodimer formation between DBF-2 and COT-1. The multiple levels of cross-communication between the SIN and MOR identified in this study and other model systems such as S. pombe or D. melanogaster, suggest the possibility that the antagonistic interactions between homologous NDR kinase networks may be a general mechanism to coordinate these pathways in higher organisms.
The annotation of multiple fungal genomes revealed the presence of several genes homologous to the bud site selection genes of budding yeast. Epistasis and biochemical analysis revealed that the MOR functions as negative regulator upstream of the BUD complex and COT-1, but not DBF-2 phosphorylates BUD-3/BUD-4 landmark proteins. Thus, regulation of BUD-3 (and possibly also BUD-4) by COT-1 may be one mechanism of the MOR pathway to inhibit septum formation in N. crassa
Self-archiving dermatology articles
Discusses the merits of depositing medical journal articles in open repositories
- …
