Neelam Dabas

• The yeast Candida albicans is a member of the normal microflora on the mucosal surfaces of the gastrointestinal and urogenital tract in healthy persons. However, it is an opportunistic pathogen that can cause a range of infections from superficial to disseminated, in response to perturbation of the normal microflora or alterations in the host immunity. C. albicans exhibits a variety of characteristics such as adhesion, morphogenetic switching and secreted aspartic protease production that contribute to its virulence. Expression of many of theseThe yeast Candida albicans is a member of the normal microflora on the mucosal surfaces of the gastrointestinal and urogenital tract in healthy persons. However, it is an opportunistic pathogen that can cause a range of infections from superficial to disseminated, in response to perturbation of the normal microflora or alterations in the host immunity. C. albicans exhibits a variety of characteristics such as adhesion, morphogenetic switching and secreted aspartic protease production that contribute to its virulence. Expression of many of these virulence factors is controlled by the availability of essential element, nitrogen. C. albicans undergoes morphogenetic transition to form filaments under nitrogen starvation conditions and this switch is controlled by the ammonium permease Mep2p. However, little is known about how this signaling function of Mep2p is regulated. Mutational analysis of Mep2p was carried out to identify the residues that confer signaling activity to this permease. The C-terminal cytoplasmic tail of Mep2p contains a signaling domain that is dispensable for ammonium transport but essential for the signaling activity of Mep2p. In this work, progressive C-terminal truncations analysis demonstrated that a MEP2DC433 allele was still able to induce filamentation while nitrogen starvation-induced filamentous growth was abolished in cells expressing a MEP2DC432 allele. Therefore, tyrosine at position 433 (Y433) is the last amino acid in Mep2p that is essential for signaling. To gain insights into how the signaling activity of Mep2p is regulated by ammonium availability and transport, conserved residues that have been implicated in ammonium binding or uptake were mutated. Mutation of D180, which has been proposed to mediate initial contact with extracellular ammonium, or the pore-lining residues H188 and H342 abolished Mep2p expression, indicating that these residues are important for protein stability. Mutation of F239, which together with F126 is predicted to form an extracytosolic gate to the conductance channel, abolished both ammonium uptake and Mep2p-dependent filamentation, despite proper localization of the protein. On the other hand, mutation of W167, which is assumed to participate along with Y122, F126, and S243 in the recruitment and coordination of the ammonium ion at the extracytosolic side of the cell membrane, also abolished filamentation without having a strong impact on ammonium transport, demonstrating that extracellular alterations in Mep2p can affect intracellular signaling. Mutation of Y122 reduced ammonium uptake much more strongly than mutation of W167 but still allowed efficient filamentation, indicating that the signaling activity of Mep2p is not directly correlated with its transport activity. An important aspect in the ability of Mep2p to stimulate filamentation in response to nitrogen limitation is its high expression levels. The cis-acting sequences and trans-acting regulators that mediate MEP2 induction in response to nitrogen limitation were identified. Promoter analysis revealed that two putative binding sites for GATA transcription factors have a central role in MEP2 expression, as deletion of the region containing these sites or mutation of the GATAA sequences in the full-length MEP2 promoter strongly reduced MEP2 expression. To elucidate the roles of the GATA transcription factors GLN3 and GAT1 in regulating MEP2 expression, mutants lacking one or both of these transcription factors were constructed. Mep2p expression was strongly reduced in gln3D and gat1D single mutants and virtually abolished in gln3D gat1D double mutants. Deletion of GLN3 strongly inhibited filamentous growth under limiting nitrogen conditions, which could be rescued by constitutive expression of MEP2 from the ADH1 promoter. In contrast, inactivation of GAT1 had no effect on filamentation. Surprisingly, filamentation became partially independent of the presence of a functional MEP2 gene in the gat1D mutants, indicating that the loss of GAT1 function results in the activation of other pathways that induce filamentous growth. These findings demonstrated that the GATA transcription factors Gln3p and Gat1p control expression of the MEP2 ammonium permease and that GLN3 is also an important regulator of nitrogen starvation-induced filamentous growth in C. albicans. C. albicans mutants lacking both the GATA transcription factors Gln3p and Gat1p were unable to grow in a medium containing an alternative nitrogen source, bovine serum albumin (BSA) as the sole nitrogen source. The ability to utilize proteins as sole source of nitrogen for growth of C. albicans is conferred by the secreted aspartic protease Sap2p, which degrades the proteins, and oligopeptide transporters that mediate uptake of the proteolytic products into cell. The growth defect of gln3D gat1D mutants was mainly caused by their inability to express the SAP2 gene, as SAP2 expression from the constitutive ADH1 promoter restored the ability of the mutants to grow on BSA. Expression of STP1, which encodes a transcription factor that is required for SAP2 induction in the presence of proteins, was regulated by Gln3p and Gat1p. Forced expression of STP1 from a tetracycline-inducible promoter bypassed the requirement of the GATA transcription factors for growth of C. albicans on proteins. When preferred nitrogen sources are available, SAP2 is repressed and this nitrogen catabolite repression of SAP2 was correlated with downregulation of STP1 under these conditions. Tetracycline-induced STP1 expression abolished nitrogen catabolite repression of SAP2, demonstrating that regulation of STP1 expression levels by the GATA transcription factors is a key aspect of both positive and negative regulation of SAP2 expression. Therefore, by using a regulatory cascade in which expression of the specific transcription factor Stp1p is controlled by the general regulators Gln3p and Gat1p, C. albicans places SAP2 expression under nitrogen control and ensures proper expression of this virulence determinant. In summary, the present study illustrated how GATA factors, Gln3p and Gat1p, play partially overlapping, but distinct roles, in mediating the appropriate responses of C. albicans to the availability of different nitrogen sources. These responses are also determinants of pathogenicity of the fungus. The relative contributions of Gln3p and Gat1p vary with their target genes and the availability of nitrogen source. Overall, these findings provide us with a better understanding of the molecular basis of some of the important processes that help in adaptation of C. albicans to various environmental conditions. The yeast Candida albicans is a member of the normal microflora on the mucosal surfaces of the gastrointestinal and urogenital tract in healthy persons. However, it is an opportunistic pathogen that can cause a range of infections from superficial to disseminated, in response to perturbation of the normal microflora or alterations in the host immunity. C. albicans exhibits a variety of characteristics such as adhesion, morphogenetic switching and secreted aspartic protease production that contribute to its virulence. Expression of many of these virulence factors is controlled by the availability of essential element, nitrogen. C. albicans undergoes morphogenetic transition to form filaments under nitrogen starvation conditions and this switch is controlled by the ammonium permease Mep2p. However, little is known about how this signaling function of Mep2p is regulated. Mutational analysis of Mep2p was carried out to identify the residues that confer signaling activity to this permease. The C-terminal cytoplasmic tail of Mep2p contains a signaling domain that is dispensable for ammonium transport but essential for the signaling activity of Mep2p. In this work, progressive C-terminal truncations analysis demonstrated that a MEP2DC433 allele was still able to induce filamentation while nitrogen starvation-induced filamentous growth was abolished in cells expressing a MEP2DC432 allele. Therefore, tyrosine at position 433 (Y433) is the last amino acid in Mep2p that is essential for signaling. To gain insights into how the signaling activity of Mep2p is regulated by ammonium availability and transport, conserved residues that have been implicated in ammonium binding or uptake were mutated. Mutation of D180, which has been proposed to mediate initial contact with extracellular ammonium, or the pore-lining residues H188 and H342 abolished Mep2p expression, indicating that these residues are important for protein stability. Mutation of F239, which together with F126 is predicted to form an extracytosolic gate to the conductance channel, abolished both ammonium uptake and Mep2p-dependent filamentation, despite proper localization of the protein. On the other hand, mutation of W167, which is assumed to participate along with Y122, F126, and S243 in the recruitment and coordination of the ammonium ion at the extracytosolic side of the cell membrane, also abolished filamentation without having a strong impact on ammonium transport, demonstrating that extracellular alterations in Mep2p can affect intracellular signaling. Mutation of Y122 reduced ammonium uptake much more strongly than mutation of W167 but still allowed efficient filamentation, indicating that the signaling activity of Mep2p is not directly correlated with its transport activity. An important aspect in the ability of Mep2p to stimulate filamentation in response to nitrogen limitation is its high expression levels. The cis-acting sequences and trans-acting regulators that mediate MEP2 induction in response to nitrogen limitation were identified. Promoter analysis revealed that two putative binding sites for GATA transcription factors have a central role in MEP2 expression, as deletion of the region containing these sites or mutation of the GATAA sequences in the full-length MEP2 promoter strongly reduced MEP2 expression. To elucidate the roles of the GATA transcription factors GLN3 and GAT1 in regulating MEP2 expression, mutants lacking one or both of these transcription factors were constructed. Mep2p expression was strongly reduced in gln3D and gat1D single mutants and virtually abolished in gln3D gat1D double mutants. Deletion of GLN3 strongly inhibited filamentous growth under limiting nitrogen conditions, which could be rescued by constitutive expression of MEP2 from the ADH1 promoter. In contrast, inactivation of GAT1 had no effect on filamentation. Surprisingly, filamentation became partially independent of the presence of a functional MEP2 gene in the gat1D mutants, indicating that the loss of GAT1 function results in the activation of other pathways that induce filamentous growth. These findings demonstrated that the GATA transcription factors Gln3p and Gat1p control expression of the MEP2 ammonium permease and that GLN3 is also an important regulator of nitrogen starvation-induced filamentous growth in C. albicans. C. albicans mutants lacking both the GATA transcription factors Gln3p and Gat1p were unable to grow in a medium containing an alternative nitrogen source, bovine serum albumin (BSA) as the sole nitrogen source. The ability to utilize proteins as sole source of nitrogen for growth of C. albicans is conferred by the secreted aspartic protease Sap2p, which degrades the proteins, and oligopeptide transporters that mediate uptake of the proteolytic products into cell. The growth defect of gln3D gat1D mutants was mainly caused by their inability to express the SAP2 gene, as SAP2 expression from the constitutive ADH1 promoter restored the ability of the mutants to grow on BSA. Expression of STP1, which encodes a transcription factor that is required for SAP2 induction in the presence of proteins, was regulated by Gln3p and Gat1p. Forced expression of STP1 from a tetracycline-inducible promoter bypassed the requirement of the GATA transcription factors for growth of C. albicans on proteins. When preferred nitrogen sources are available, SAP2 is repressed and this nitrogen catabolite repression of SAP2 was correlated with downregulation of STP1 under these conditions. Tetracycline-induced STP1 expression abolished nitrogen catabolite repression of SAP2, demonstrating that regulation of STP1 expression levels by the GATA transcription factors is a key aspect of both positive and negative regulation of SAP2 expression. Therefore, by using a regulatory cascade in which expression of the specific transcription factor Stp1p is controlled by the general regulators Gln3p and Gat1p, C. albicans places SAP2 expression under nitrogen control and ensures proper expression of this virulence determinant. In summary, the present study illustrated how GATA factors, Gln3p and Gat1p, play partially overlapping, but distinct roles, in mediating the appropriate responses of C. albicans to the availability of different nitrogen sources. These responses are also determinants of pathogenicity of the fungus. The relative contributions of Gln3p and Gat1p vary with their target genes and the availability of nitrogen source. Overall, these findings provide us with a better understanding of the molecular basis of some of the important processes that help in adaptation of C. albicans to various environmental conditions.…
• Der Hefepilz Candida albicans ist ein harmloser Kommensale auf den Schleimhäuten des Gastrointestinal- und Urogenitaltrakts der meisten gesunden Menschen. Bei einer Störung der natürlichen Mikroflora oder des Wirtsimmunsystems kann der Pilz jedoch auch oberflächliche und sogar systemische Infektionen verursachen. C. albicans weist eine Reihe von Eigenschaften auf, die zur Virulenz des Erregers beitragen. Dazu gehören die Adhärenz an unterschiedliche Wirtsoberflächen, die morphologische Variabilität des Pilzes und die Sekretion vonDer Hefepilz Candida albicans ist ein harmloser Kommensale auf den Schleimhäuten des Gastrointestinal- und Urogenitaltrakts der meisten gesunden Menschen. Bei einer Störung der natürlichen Mikroflora oder des Wirtsimmunsystems kann der Pilz jedoch auch oberflächliche und sogar systemische Infektionen verursachen. C. albicans weist eine Reihe von Eigenschaften auf, die zur Virulenz des Erregers beitragen. Dazu gehören die Adhärenz an unterschiedliche Wirtsoberflächen, die morphologische Variabilität des Pilzes und die Sekretion von Aspartatproteasen. Die Expression vieler dieser Virulenzfaktoren wird unter anderem durch die Verfügbarkeit von Stickstoff reguliert. Unter Stickstoffmangelbedingungen wechselt C. albicans vom Wachstum als sprossende Hefe zum filamentösen Wachstum, und dieser Wechsel wird durch die Ammoniumpermease Mep2p reguliert. Wie die Induktion des filamentösen Wachstums durch Mep2p kontrolliert wird, ist jedoch weitgehend unbekannt. In der vorliegenden Arbeit wurde eine Mutationsanalyse von Mep2p durchgeführt, um Aminosäuren zu identifizieren, die an der Signalfunktion dieser Permease beteiligt sind. Die C-terminale cytoplasmatische Domäne von Mep2p wird für den Ammoniumtransport nicht benötigt, ist jedoch essentiell für die Signaltransduktion. Progressive C-terminale Verkürzungen von Mep2p zeigten, dass ein MEP2DC433-Allel immer noch in der Lage war, das filamentöse Wachstum zu induzieren, wohingegen die Deletion einer weiteren Aminosäure die Morphogenese blockierte. Das Tyrosin an Position 433 (Y433) ist deshalb die letzte Aminosäure, die für die Signalfunktion von Mep2p essentiell ist. Um besser zu verstehen, wie die Signalaktivität von Mep2p durch die Verfügbarkeit und den Transport von Ammonium reguliert wird, wurden verschiedene hochkonservierte Aminosäuren mutiert, die vermutlich an der Bindung oder dem Transport von Ammonium in die Zelle beteiligt sind. Die Mutation von D180, von dem postuliert wurde, dass es den initialen Kontakt mit extrazellulärem Ammonium ermöglicht, oder der im Transportkanal lokalisierten Histidine H188 und H342 hatte zur Folge, dass Mep2p nicht mehr exprimiert wurde, so dass diese Aminosäuren vermutlich für die Proteinstabilität wichtig sind. Die Mutation von F239, das zusammen mit F126 eine extracytosolische Pforte zur Transportpore bildet, verhinderte trotz korrekter Membranlokalisation sowohl den Ammoniumtransport als auch das filamentöse Wachstum. Allerdings führte auch die Mutation von W167, das vermutlich zusammen mit Y122, F126 und S243 an der Rekrutierung des Ammoniumions an der extrazellulären Seite der Membran beteiligt ist, zur Blockierung des filamentösen Wachstums, obwohl der Ammoniumtransport kaum beeinflusst war. Dies zeigte, dass die intrazelluäre Signaltransduktion durch extrazelluläre Veränderungen in Mep2p beeinflusst werden kann. Die Mutation von Y122 reduzierte die Ammoniumaufnahme weitaus starker als die Mutation von W167, erlaubte jedoch immer noch ein effizientes filamentöses Wachstum. Die Signalaktivität von Mep2p ist deshalb offensichtlich nicht direkt mit der Transportaktivität des Proteins korreliert. Ein wichtiger Aspekt in der Fähigkeit von Mep2p, die Morphogenese zu stimulieren, ist die vergleichsweise starke Expression des Proteins. Um die Regulation der MEP2-Expression aufzuklären, wurden die cis-regulatorischen Sequenzen und die trans-aktivierenden Faktoren, die die MEP2-Induktion unter Stickstoffmangel vermitteln, identifiziert. Eine Promotoranalyse zeigte, dass zwei mutmaßliche Bindungsstellen für GATA-Transkriptionsfaktoren eine zentrale Rolle in der MEP2-Expression haben, da die Deletion oder Mutation dieser GATAA-Sequenzen die Expression von MEP2 stark reduzierte. Um die Rolle der GATA-Transkriptionsfaktoren Gln3p und Gat1p bei der Regulation der MEP2-Expression zu untersuchen, wurden Mutanten hergestellt, in denen die entsprechenden Gene deletiert waren. Die Expression von Mep2p war in gln3D und gat1D Einzelmutanten stark verringert und in gln3D gat1D Doppelmutanten nicht mehr nachweisbar. Die Deletion von GLN3 hatte auch eine starke Reduktion des filamentösen Wachstums zur Folge, die durch die konstitutive Expression von MEP2 unter Kontrolle des ADH1-Promotors aufgehoben wurde. Dagegen hatte die Deletion von GAT1 keinen Einfluss auf das filamentöse Wachstum. Überraschenderweise war das filamentöse Wachstum in den gat1D Mutanten teilweise unabhängig von Mep2p, was darauf hinwies, dass in Abwesenheit von GAT1 andere Signalwege aktiviert werden, die die Morphogenese stimulieren. Diese Ergebnisse zeigten, dass die GATA-Transkriptionsfaktoren Gln3p und Gat1p die Expression der Ammoniumpermease MEP2 kontrollieren und dass Gln3p auch ein wichtiger Regulator des durch Stickstoffmangel induzierten filamentösen Wachstums von C. albicans ist. Mutanten, in denen die beiden GATA-Transkriptionsfaktoren Gln3p und Gat1p fehlten, waren nicht mehr in der Lage, in einem Medium zu wachsen, das bovines Serumalbumin (BSA) als einzige Stickstoffquelle enthält. Die Fähigkeit von C. albicans, Proteine als einzige Stickstoffquelle zum Wachstum zu verwenden, wird durch die sekretierte Aspartatprotease Sap2p, die die Proteine zu Peptiden abbaut, und durch Oligopeptidtransporter, die diese Peptide in die Zelle aufnehmen, vermittelt. Der Wachstumsdefekt der gln3D gat1D Doppelmutanten war hauptsächlich durch einen Defekt in der SAP2-Expression verursacht, da die Expression von SAP2 unter Kontrolle des konstitutiven ADH1-Promotors die Fähigkeit zum Wachstum auf BSA wieder herstellte. Es zeigte sich, dass Gln3p und Gat1p die Expression des Transkriptionsfaktors STP1, der für die Induktion von SAP2 in Gegenwart von Proteinen notwendig ist, regulieren. Bei einer Expression von STP1 unter Kontrolle des induzierbaren Tet-Promotors waren Gln3p und Gat1p nicht mehr notwendig für das Wachstum auf Proteinen. Wenn bevorzugte Stickstoffquellen verfügbar sind, wird SAP2 auch in Gegenwart von Proteinen reprimiert, und diese Stickstoff-Katabolitrepression korrelierte mit einer reduzierten STP1-Expression. Die Expression von STP1 unter Kontrolle des Tet-Promotors hob diese Repression auf, was zeigte, dass die Regulation der STP1-Expression durch die GATA-Transkriptionsfaktoren eine Schlüsselrolle sowohl bei der positiven als auch bei der negativen Kontrolle der SAP2-Expression spielt. Eine regulatorische Kaskade, in der die Expression des spezifischen Transkriptionsfaktors Stp1p durch die allgemeinen Regulatoren Gln3p und Gat1p kontrolliert wird, stellt die Expression von SAP2 in C. albicans deshalb unter Stickstoffkontrolle und gewährleistet eine angepasste Expression dieses Virulenzfaktors. Die Ergebnisse dieser Arbeit illustrieren, dass die GATA-Faktoren Gln3p und Gat1p zum Teil überlappende aber auch spezifische Funktionen in der Anpassung von C. albicans an die Verfügbarkeit verschiedener Stickstoffquellen haben. Diese Anpassungsmechanismen spielen auch eine Rolle in der Pathogenität des Pilzes, wobei die relative Bedeutung von Gln3p und Gat1p vom Zielgen und der Stickstoffquelle abhängt. Diese Erkenntnisse geben einen vertieften Eiblick in die molekularen Grundlagen der Anpassung von C. albicans an unterschiedliche Umweltbedingungen.…