Plastid genome rearrangement, gene loss, and sequence divergence in geraniaceae, passifloraceae, and annonaceae.

Blazier, John Christensen

06 February 2014

Plastid genomes of flowering plants are largely identical in gene order and content, but a few lineages have been identified with many gene and intron losses, genomic rearrangements, and accelerated rates of nucleotide substitutions. These aberrant lineages present an opportunity to understand the modes of selection acting on these genomes as well as their long-term stability. My research has focused on two areas within plastid genome evolution in Geraniaceae: first, an investigation of the diversity of unusual plastid genomes in a single genus, Erodium (Geraniaceae) for chapters one and three. Chapter two focuses on the evolution of subunits of the plastid-encoded RNA polymerase (PEP). The first chapter described the loss of plastid-encoded NADPH dehydrogenase (ndh) genes from a clade of 13 Erodium species. Divergence time estimates indicate this clade is less than 5 million years old. This recent loss of ndh genes in Erodium presents an opportunity to investigate changes in photosynthetic function through comparative biochemistry between Erodium species with and without plastid-encoded ndh genes. Second, I examined the evolution of the gene encoding the alpha subunit (rpoA) of PEP in three disparate angiosperm lineages—Pelargonium (Geraniaceae), Passiflora (Passifloraceae), and Annonaceae—in which this gene has diverged so greatly that it is barely recognizable. PEP is conserved in the plastid genomes of all photosynthetic angiosperms. I found multiple lines of evidence indicating that the genes remain functional despite retaining only ~30% sequence identity with rpoA genes from outgroups. The genomes containing these divergent rpoA genes have undergone significant rearrangement due to illegitimate recombination and gene conversion, and I hypothesized that these phenomena have also driven the divergence of rpoA. Third, I conducted a survey of plastid genome evolution in Erodium with the completion of 15 additional whole genomes. Except for Erodium and some legumes, all angiosperm plastid genomes share a quadripartite structure with large and small single copy regions (LSC, SSC) and two inverted repeats (IR). I discovered a species of Erodium that has re-formed a large inverted repeat. Demonstrating a precedent for loss and regain of the IR also impacts models of evolution for other highly rearranged plastid genomes. / text

Erodium

Pelargonium

Geraniaceae

Molecular evolution

Plastid genome

Genomics

RpoA

Ndh genes

Análise da estrutura filogeográfica das espécies do grupo Pilosocereus Aurisetus (Cactaceae) utilizando marcadores moleculares do genoma do cloroplasto (cpDNA)

Bonatelli, Isabel Aparecida da Silva

18 May 2012

Made available in DSpace on 2016-06-02T20:21:30Z (GMT). No. of bitstreams: 1 4533.pdf: 2866936 bytes, checksum: a3b1ef75c45a68a6305453e240c9d466 (MD5) Previous issue date: 2012-05-18 / Universidade Federal de Minas Gerais / PILOSOCEREUS AURISETUS is a taxonomic group composed by eight columnar cacti species occurring on rock outcrops in xeric environments. As other xerophitic species found outside the Caatinga domain, the species populations of P. AURISETUS group exhibit a disjunct distribution pattern within the Cerrado domain in central and eastern Brazil. Such a distribution pattern may have resulted from long-distance dispersal events or fragmentation of a more extensive distribution in the past. The main goal of this work was identify demographic events that possibly shaped the evolutionary history of the group and resulted in the current biogeographic pattern. In the present work, phylogenetic analyses and phylogeographical inferences were implemented using the nucleotide variation of plastid genomic sequences. The phylogenetic analyses showed the absence of reciprocal monophyly for great part of the species and the occurring of quite divergent species from the others of the group: P. jauruensis, P. aureispinus e P. bohlei. In addition, P. machrisii populations formed two distinct clades highly supported by the phylogeny which partly agree with the geographic distribution of the species (north and central-south). Population analyses and phylogeographical inferences allowed the identification of the diversification origin of the group and the possible expansion and fragmentation events which determined the evolutionary pathway of the populations. The genetic variability level and the genetic structure observed alongside the current distribution pattern of the populations and biological information about the species suggest that fragmentation events were the main responsible for the biogeographical pattern of the group, which should be related to the palioclimatic oscillations of the Quaternary. / PILOSOCEREUS AURISETUS é um grupo taxonômico composto por oito espécies de cactos colunares que ocorrem associadas a afloramentos rochosos em ambientes xéricos. Assim como outras espécies xerófitas encontradas fora do domínio da Caatinga, as populações das espécies do grupo P. AURISETUS exibem um padrão de distribuição descontínua dentro do domínio Cerrado no centro e leste do Brasil. Esse padrão de distribuição pode ser resultado de eventos de dispersão a longa distância ou de fragmentação de uma distribuição mais extensa no passado. O objetivo principal desse trabalho foi identificar eventos demográficos que possivelmente moldaram a história evolutiva do grupo e resultaram no padrão biogeográfico atual. No presente trabalho foram realizadas análises filogenéticas e inferências filogeográficas a partir da variação nucleotídica de sequências do genoma plastidial. As análises filogenéticas demonstraram que a maior parte das espécies do grupo não apresenta monofilia recíproca de seus haplótipos e que o grupo abrange três espécies bastante divergentes das demais: P. jauruensis, P. aureispinus e P. bohlei. Adicionalmente, as populações da espécie P. machrisii formaram dois clados distintos e bem suportados na filogenia, os quais concordam parcialmente com a distribuição geográfica da espécie (norte e centro-sul). As análises populacionais e as inferências filogeográficas permitiram inferir a origem da diversificação do grupo e os possíveis eventos de expansão e fragmentação que determinaram o caminho evolutivo das populações. Os níveis de variabilidade genética e estruturação observados, juntamente com o padrão atual de distribuição das populações e informações sobre a biologia das espécies, sugerem que eventos de fragmentação foram os principais responsáveis pelo padrão biogeográfico do grupo, os quais devem estar relacionados às oscilações palioclimáticas do Quaternário.

Filogeografia

Filogenia

Genoma plastidial

Pilosocereus

Cactaceae

Phylogeography

Phylogeny

Plastid genome

Pilosocereus

Cactaceae

CIENCIAS BIOLOGICAS::GENETICA

CaracterizaÃÃo bioquÃmica e molecular da oxidase terminal da plastoquinona (PTOX) em Zea mays / Biochemical and molecular characterization of the terminal oxidase plastoquinone (PTOX) in Zea mays

Francisco Yuri Maia de Sousa

28 October 2008

nÃo hà / O cloroplasto à uma organela caracterÃstica dos organismos fotossintetizantes sendo seu papel primordial na geraÃÃo de energia a partir de gÃs carbÃnico e Ãgua. Essa organela pode ter seu funcionamento comprometido quando submetida a estresses ambientais devido a fragilidade e complexidade do sistema. Para evitar perdas provocadas pelo estresse existem vÃrios mecanismos de adaptaÃÃo e regulaÃÃo das reaÃÃes que ocorrem no cloroplasto. Recentemente caracterizou-se mais um desses provÃveis mecanismos que foi chamado de clororespiraÃÃo. A clororespiraÃÃo foi esclarecida com a descoberta de uma enzima similar a oxidase alternativa da mitocondria que chamou-se de oxidase terminal do plastÃdeo (PTOX). A funÃÃo dessa respiraÃÃo do cloroplasto permanece incerta, mas uma das hipÃteses mais aceitas à que o funcionamento da clororespiraÃÃo poderia prevenir a formaÃÃo de espÃcies reativas de oxigÃnio atravÃs da reciclagem dos intermediÃrios redutores do cloroplasto. No presente trabalho foi caracterizado a presenÃa de dois genes que codificam para a oxidase terminal do plastÃdeo em plantas de Zea mays. Estudou-se tambÃm a expressÃo diferencial de ambos genes da PTOX em resposta ou estresse hÃdrico, alÃm da caracterizaÃÃo da clororespiraÃÃo atravÃs da atividade da NADH desidrogenase plastidial (NDH) em gel de poliacrilamida. A caracterizaÃÃo molecular dos genes da PTOX mostrou homologia de 60% quando comparadas as sequÃncias dos genes e de 79% quando comparadas as prÃ-proteÃnas traduzidas. Os genes dessa proteÃna tÃm estruturas similares, sendo compostos por oito introns e 9 Ãxons. Um estudo das regiÃes dos promotores dos genes mostrou que existiam elementos comuns porÃm a presenÃa de elementos diferentes como, o elementos cis MBS que à responssivo à seca, poderia revelar uma regulaÃÃo diferencial dos genes. A resposta diferencial foi confirmada atravÃs de RT-PCR semiquantitativo. O gene chamado de ptox1 teve sua expressÃo estÃvel, podendo ser considerado um gene constitutivo, enquanto que o gene chamado de ptox2 teve um aumento da expressÃo proporcional ao estresse aplicado tanto em folhas como em raÃzes de plantas de milho. A anÃlise da atividade da NDH em gel (zimograma) revelou a presenÃa dessa enzima em cloroplastos de milho confirmando a presenÃa das enzimas da clororespiraÃÃo. O estudo filogenÃtico de sequencias de cDNA de bancos de dados mostraram que milho e sorgo pertencentes ao grupo das monocotiledÃneas, sÃo espÃcies muito prÃximas e que compartilham dois genes ortÃlogos da PTOX identificados como ptox1 e ptox2. Concluiu-se pela primeira vez a presenÃa de dois genes da PTOX no genoma do milho, uma monocotiledÃena de metabolismo C4. Os genes foram denominados de ptox1 e ptox2. Eles foram encontrados em raÃzes e folhas e apenas o gene da ptox2 pareceu ser induzido em resposta ao estresse osmÃtico. / The chloroplast is an organelle characteristic of photosynthetic organisms and their role in generating energy from carbon dioxide and water. This organelle may be functionally compromised when subjected to environmental stresses due to the fragility and complexity of the system. To avoid losses caused by stress there are several mechanisms of adaptation and adjustment of the reactions that occur in the chloroplast. Recently characterized most likely of these mechanisms has been called clororespiraÃÃo. The clororespiraÃÃo was clarified with the discovery of an enzyme similar to mitochondria that the alternative oxidase is called terminal plastid oxidase (PtOx). The function of chloroplast respiration remains uncertain, but one of the most accepted hypothesis is that the operation of clororespiraÃÃo could prevent the formation of reactive oxygen species by recycling intermediate reducing the chloroplast. Characterized in this study was the presence of two genes coding for the terminal oxidase in plant plastid of Zea mays. Was also studied the differential expression of both genes in response PtOx or water stress, and the characterization of clororespiraÃÃo through the activity of the NADH dehydrogenase plastid (NDH) polyacrylamide gel. The molecular characterization of genes PtOx showed homology of 60% when comparing the sequences of genes and 79% when compared to the pre-translated proteins. Genes of this protein have similar structures are composed of eight introns and exons 9. A study of regions of the promoters of the genes showed that there were common elements but the presence of different elements as the cis elements that MBS is responssivo drought, could reveal a differential regulation of genes. The differential response was confirmed by semiquantitative RT-PCR. The gene was called ptox1 stable expression could be considered a constitutive gene, whereas the gene was called ptox2 increased expression proportional to applied stress in both leaves and roots of corn plants. The analysis of the activity of NDH gel (zymogram) revealed the presence of this enzyme in chloroplasts corn confirming the presence of enzymes clororespiraÃÃo. The phylogenetic analysis of cDNA sequences from databases showed that corn and sorghum in the group of monocots are closely related species which share two of the orthologous genes identified as PtOx ptox1 and ptox2. It appeared that the first time the presence of two genes PtOx into the maize genome, a C4 monocotiledÃena metabolism. Genes were named ptox1 and ptox2. They were found in the roots and leaves and only ptox2 gene appeared to be induced in response to osmotic stress.

Oxidase Terminal do PlastÃdeo

Milho

BioinformÃtica

Plastid terminal oxidase

Corn

Bioinformatics

BIOQUIMICA

Diverzita prasinofytních řas příbuzných plastidu euglen / Diversity of prasinophyte algae related to the euglenid plastid

Lukešová, Soňa

January 2016

Euglenophyceae represent a group of unicellular eukaryotic organisms that have gained during their evolution the ability to photosynthesize. They aquired plastids via secondary endosymbiosis with a green alga as the plastid donor. Phylogenetic studies searching for the origin of this organelle revealed the green alga Pyramimonas parkeae from Prasinophytes as the closest known relative to euglenid plastids. Pyramimonas parkeae and Euglena share several genes clusters with unique order of genes in their plastid genomes, which also point to the Pyramimonadales as the donor of the plastids. However, it is posible, that organisms more closely related to euglenid plastids than P. parkeae, occur in the environment. In my diploma thesis I focused on the exploration of diversity of Pyramimonadales and Euglenophyceae in environmental samples. I used several approaches to perform this task. I amplified parts of the plastid genomes in environmental samples by using specific PCR and determined their position in the phylogenetic tree. I also made large-scale phylogenetic analyses based on 16S rRNA and 18S rRNA sequences from representatives of the groups Euglenophyceae, Prasinophytes and environmental samples. The results revealed the presence of a large number of environmental sequences relative to the...

Evoluce proteomu plastidu euglenidů / Evolution of euglenid plastid proteome

Novák Vanclová, Anna

January 2019

Endosymbiotic gain and transfer of plastids is a widespread evolutionary phenomenon and a major driving force of eukaryotic evolution. The integration of a new organelle is accompanied by changes in its structure, gene content, molecular mechanisms for biogenesis and transport, and re-wiring of the host and organelle metabolic pathways. To understand the course and underlying mechanisms of plastid evolution, it is important to study these processes in variety of secondary algae and notice their differences and similarities. Euglenophytes gained their plastids from green eukaryotic algae after a long history of heterotrophic lifestyle. In my thesis, I participated in analyses of newly generated sequence datasets: transcriptomes of Euglena gracilis and Euglena longa and mass spectrometry-determined proteome of E. gracilis plastid with especial regard to the potential novelties associated with plastid gain and incorporation. In the resulting publications we particularly focus on plastid protein import machinery and targeting signals and report extremely reduced TIC and completely absent TOC in euglenophyte plastid. Using the proteomic dataset, we predict potential novel plastid protein translocases recruited from ER/Golgi and re-analyze plastid signal domains, characterizing previously overlooked...

Organellar DNA Polymerases Gamma I and II in <em>Arabidopsis thaliana</em>

Brammer, Jeffrey M.

17 June 2010

Plants have two organelles outside the nucleus which carry their own DNA, mitochondria and chloroplasts. These organelles are descendants of bacteria that were engulfed by their host according to the endosymbiotic theory. Over time, DNA has been exchanged between these organelles and the nucleus. Two polymerases, DNA Polymerases Gamma I and II, are encoded in the nucleus and remain under nuclear control, but are transported into the mitochondria and chloroplasts. DNA polymerases gamma I and II are two organelle polymerases which have been studied through sequence analysis and shown to localize to both mitochondria and chloroplasts. Little has been done to characterize the activities of these polymerases. Work in tobacco showed the homology of these polymerases to each other and to DNA Polymerase I in bacteria. They have been characterized as being part of the DNA Polymerase A family of polymerases. In my research I have studied the effect of T-DNA insertions within the DNA Polymerase Gamma I and II genes. Since these DNA Polymerases are targeted to the mitochondria and chloroplasts, I studied the effect of knocking out these genes. A plant heterozygous for an insert in DNA Polymerase Gamma I grows slightly slower than wild type plants with an approximately 20% reduction in mitochondrial and chloroplast DNA copy number. A plant homozygous for an insert in this same gene has a drastic phenotype with stunted plants that grow to around 1 inch tall, with floral stems, and have an approximately 50-55% reduction in mitochondrial and chloroplast DNA copy number. Wild type plants can grow to a height of 12-18 inches with floral stems as a comparison. A plant heterozygous for an insert in the DNA Polymerase Gamma II gene grows slightly slower than wild type plants and has an approximately 15% reduction in mitochondrial DNA copy number and a 50% reduction in chloroplast DNA copy number. These plants also produce much less seed than do other mutants and wild type plants.

DNA polymerase

Arabidopsis

Arabidopsis thaliana

gamma polymerase

mitochondrion

mitochondria

chloroplast

plastid

DNA replication

Microbiology

Aspekte der plastidären Transkription

Hertel, Stefanie

13 August 2009

In dieser Arbeit wurde die plastidäre Genexpression hinsichtlich zweier Aspekte untersucht: der Cytokinineinfluss auf die plastidäre Transkription und ihrer Komponenten sowie eine in vivo-Charakterisierung von PrpoB-345, des Promotors des rpoB-Operons im Tabak. Cytokinine beeinflussen die Chloroplastenbiogenese und –funktion. Um den Einfluss von Cytokinin auf die plastidäre Genexpression zu untersuchen, wurden run-on-Transkriptionsassays und quantitative real-time RT-PCR von BA-behandelten seneszenten Tabakblättern und sieben-Tage-alten Arabidopsis- und Tabakpflanzen durchgeführt. Zeitreihenanalysen zeigten eine Aktivierung der plastidären Transkription in jungen Pflanzen und im seneszenten Tabak 2 h bzw. 3 h nach BA-Applikation. Abgeschnittene Blätter von Tabakmutanten mit konstitutiv reduziertem Cytokiningehalt antworteten bereits nach 30 min der Hormonbehandlung. Es gibt jedoch keinen eindeutigen Hinweis für eine direkte Korrelation zwischen der Expression der nukleär kodierten Phagentyp-RNA-Polymerasen und der BA-induzierten transkriptionellen Aktivierung der Plastidengene. Zusammengefasst, scheint die Antwort auf exogenes Cytokinin vom physiologischen Status der Chloroplasten, die von der Pflanzenart sowie vom endogenen Cytokiningehalt beeinflusst werden, abzuhängen. Plastidäre Gene höherer Pflanzen werden von mindestens zwei RNA-Polymerasen transkribiert: die plastidär kodierte RNA-Polymerase vom Bakterientyp (PEP) und die kernkodierte Phagentyp-RNA-Polymerase (NEP). NEP transkribiert das rpoB-Operon, das drei von vier Untereinheiten der PEP kodiert. Transkriptions- und Transkriptanalysen von rpoB-Promotor-Deletionsmutanten ergaben Hinweise auf mögliche Regulationsstellen der Kontrolle der rpoB-Transkription. Neben PrpoB-345 konnten zwei weitere Promotoren kartiert werden. Einer von ihnen ist ein putativer PEP-Promotor, der auf autoregulatorische Rückkopplungsmechanismen bei der PEP-Expression hindeutet. / In this study, plastid gene expression was analyzed focusing on two aspects: the effect of cytokinin on plastid gene transcription and its components, and the in vivo characterization of PrpoB-345, the promoter of the rpoB operon in tobacco. Cytokinins are involved in the control of chloroplast biogenesis and function. To study cytokinin effects on plastid gene expression, chloroplast run-on transcription and quantitative real-time RT-PCR from senescent tobacco leaves as well as Arabidopsis and tobacco seedlings after BA treatment were performed. Analyses of time series revealed that BA-induced changes in plastid gene expression are seemingly under circadian and homeostatic control. After 2 h and 3 h of incubation with cytokinin, a stimulation of chloroplast transcription could be observed in seedlings and senescent leaves, respectively. Detached leaves of tobacco mutants with reduced endogenous cytokinin content responded even faster to BA (30 min). There is no indication of direct correlation of the expression of nuclear-encoded plastid phage-type RNA-polymerases and the BA-induced transcriptional activation of plastid genes. In summary, the responsiveness to exogenous cytokinin depends on the physiological status of chloroplasts influenced by plant species and endogenous cytokinin pool. Plastid genes of higher plants are transcribed by at least two RNA polymerases: the plastid-encoded eubacterial-type RNA polymerase (PEP) and the nucleus-encoded phage-type RNA polymerase (NEP). NEP transcribes the rpoB operon encoding three of four subunits of PEP. Transcription and transcript analyses from rpoB promoter deletion mutants indicated putative regulatory sites of control of rpoB transcription which may also interact with (cytokinin-regulated) specificity factors. Beside PrpoB-345, two additional rpoB promoters could be mapped. One of them is a putative PEP promoter which may imply autoregulatory loops of PEP expression.

Tabak

Arabidopsis

Plastidentranskription

RNA-Stabilität

Phytohormone

Cytokinin

Plastidäre Promotoren

Tabak rpoB-Operon

WG 2300

WE 3250

Tobacco

Arabidopsis

plastid transcription

RNA stability

phytohormones

Cytokinin

Plastid promoters

tobacco rpoB Operon

580 Pflanzen (Botanik)

32 Biologie

ddc:580

Implication des protéines WHIRLY dans la biogénèse du chloroplaste en association avec la protéine SIG6

Truche, Sébastien

12 1900

Le mode vie autotrophique des plantes repose entièrement sur l’intégrité du chloroplaste et notamment l’étape de la biogénèse. La transcription des gènes chloroplastiques, assurée par une PEP (ARN polymérase encodée par le chloroplaste) et deux NEPs (ARN polymérase encodée par le noyau), est l’une des étapes primordiales dans le développement d’un chloroplaste photosynthétique. On distingue trois classes de gènes chloroplastiques : les gènes de classe I, transcrit par la PEP exclusivement; les gènes de classe II, transcrits par la PEP ou les NEPs; et les gènes de classe III, transcrits exclusivement par les NEPs. Pour assurer sa fonction, la PEP doit être associée à des facteurs sigmas. L’un de ceux-ci, la protéine SIG6, est un facteur sigma général et, associé à la PEP, assure la transcription de l’ensemble des gènes de classe I et II lors du développement du chloroplaste photosynthétique. Ainsi, le mutant sig6 présente un phénotype de cotylédons pâles, associé à un retard de biogénèse chloroplastique, ainsi qu’une diminution de la transcription des gènes de classe I, provoquant la diminution de la quantité de protéines de classe I. Dans le laboratoire, nous étudions les deux protéines WHIRLY chloroplastiques (WHY1 et WHY3) pour leur rôle dans le maintien de la stabilité génomique chloroplastique. Toutefois, peu de choses sont encore connues sur leur rôle potentiel dans la transcription ou la biogénèse chloroplastique. Par exemple, lorsque l’on tente de purifier la PEP, on obtient un gros complexe transcriptionnel nommé PTAC (Plastid Transcriptionally Active Chromosome) dans lequel sont retrouvées les deux protéines WHIRLY, suggérant qu’elles pourraient être impliquées dans la transcription chloroplastique. De plus, un possible rôle dans la biogénèse chloroplastique leur a été prêté, notamment chez le maïs. Dans cette étude, nous avons donc cherché à vérifier l’implication des protéines WHIRLY dans la biogénèse chloroplastique par une approche génétique de croisements entre les mutants sig6 et why1why3. Pour cela, nous avons isolé des doubles mutants sig6why1 et sig6why3, ainsi qu’un triple mutant sig6why1why3. À l’aide d’une caractérisation phénotypique et de la quantification de quelques protéines chloroplastiques, nous avons remarqué que la perte d’un des WHIRLY permet de complémenter le phénotype de cotylédons pâles du mutant sig6 et favorise l’expression normale de protéines en principe sous-exprimées dans le mutant sig6. Toutefois, la perte des deux WHIRLY ne permet pas de compenser le phénotype de cotylédons pâles et provoque l’apparition d’un phénotype persistant associé à une expression anormale des protéines chloroplastiques. Ces résultats ne peuvent être expliqués par le rôle des WHIRLY dans le maintien de la stabilité génomique chloroplastique étant donné que le triple mutant sig6why1why3 présente moins de réarrangements que le double mutant why1why3. Finalement, nous montrons que les effets de la perte d’un WHIRLY sur le mutant sig6 peuvent être mimés par l’utilisation de la rifampicine, une drogue inhibant l’ARN polymérase chloroplastique de type bactérienne (PEP). Ensemble, ces résultats démontrent donc l’implication des protéines WHIRLY chloroplastiques dans la biogénèse chloroplastique en association avec la protéine SIG6. Nous proposons un modèle selon lequel les deux protéines WHIRLY permettraient de favoriser l’activité de l’ARN polymérase de type bactérienne, notamment lors du développement du chloroplaste photosynthétique. En cas d’absence d’une des deux protéines, cette diminution partielle d’activité de la PEP favoriserait la mise en place d’un mécanisme de complémentation par le NEPs, permettant finalement de rétablir la biogénèse chloroplastique dans un mutant sig6. En l’absence des deux WHIRLY, le mécanisme de complémentation par les NEPs serait incapable de compenser la forte inhibition de la PEP, se traduisant par une aggravation du retard de développement du chloroplaste dans le mutant sig6. / The autotrophic lifestyle of plants relies entirely on the integrity of chloroplasts and particularly on their biogenesis. Chloroplast gene transcription, performed by a Plastid-Encoded Polymerase (PEP) and two Nuclear-Encoded Polymerases (NEPs), is one of the key steps during the development of photosynthetic chloroplast. There are 3 classes of genes, one transcribed by PEP alone (class I), one by both PEP and NEPs (class II), and the third by NEPs alone (class III). To carry out transcription, PEP associates with plastid sigma factors including the general sigma factor SIG6. sig6 mutants have a pale cotyledon phenotype, a severe decrease in class I gene transcription and a reduction in the level of class I proteins. In our laboratory, we study the role of the two plastid WIHRLY proteins (WHY1 and WHY3) in maintaining plastid genome stability. However, little is known about any role these proteins may play in transcription or chloroplast biogenesis. It seems likely they are involved in plastid gene transcription since they are found in the Plastid Transcriptionally Active Chromosome (PTAC). Moreover, they have been implicated in chloroplast biogenesis in maize. In this study, we verified the implication of these proteins in plastid biogenesis using a genetic approach in which we crossed a sig6 mutant with a why1why3 mutant. We isolated sig6why1 and sig6why3 double mutants and a sig6why1why3 triple mutant. Using a phenotypic characterisation and quantification of some plastid proteins, we show that loss of one of the two Why genes complements the sig6 pale cotyledon phenotype and allows a more normal pattern of expression of plastid proteins that are under-expressed in the sig6 mutant. However, we also show that loss of the two Why genes does not alleviate the sig6 phenotype. Moreover, the triple mutant shows a second pale phenotype on true leaves, and the plastid protein expression pattern is abnormal compared to either sig6 or wild type plants. Those results cannot be explained by the role of WHIRLY proteins in plastid genome stability since the triple mutant shows fewer plastid genome rearrangements than the why1why3 mutant. Finally, we show that inhibition of the PEP polymerase using rifampicin elicits the same complementation of the sig6 phenotype as the loss of one of the two WHIRLY. Together, these results show the implication of WHIRLY proteins in plastid biogenesis in association with SIG6. We propose a model in which WHIRLY act as activators of PEP activity, particularly during the chloroplast biogenesis. Therefore, the absence of one of the WHIRLY would cause a weak inhibition of PEP, facilitating the set-up of a rescue mechanism by NEPs and, consequently, allowing the complementation of plastid biogenesis in the sig6 mutant. However, the absence of the two WHIRLY proteins would cause a strong inhibition of PEP, and the inability of the rescue mechanism by NEPs to compensate for this strong inhibition, resulting in a more severe phenotype in the sig6 mutant.

Sig6

Whirly

Chloroplaste

Transcription

PEP

Rifampicine

Biogénèse chloroplastique

Chloroplast

Plastid biogenesis

Rifampicin

Kleptoplasty in Dinophysis spp : Ecological role and evolutionary implications

Minnhagen, Susanna

January 2010

This thesis deals with the question of whether planktonic protits of the genus Dinophysis have permanent plastids (=chloroplasts) or practice kleptoplasty, i.e. acquire plastids via predation on other microorganisms. Sequencing the plastid 16S rDNA of Dinophysis spp. collected from 4 different geographical regions unveiled two different plastid genotypes within this genera: one that was found at all locations investigated, identical to that of the free-living cryptophyte Teleaulax amphioxeia, and another found only in the Greenland Sea, closely related to that of the cryptophyte Geminigera cryophila. Both types were found within the species D. acuminata. These findings imply that the plastids in Dinophysis spp. were not inherited from a common ancestor, but acquired from feeding. By using flow cytometry in combination with an acidotrophic probe, it was shown that 71 % of the cells in a D. norvegica population in the aphotic zone of the Baltic Sea had food-vacuoles. Dinophysis used to be regarded as a primarily phototrophic organism, and this was a higher proportion of cells with food-vacuoles than reported earlier. To further study if Dinophysis needs constant refill of new plastids from the environment, a new method combining flow-cytometry and quantitative real-time PCR was developed to compare the levels of nuclear and plastid DNA in different phases of the cell-cycle. Results showed that plastid acquisition in Dinophysis was uncoupled with the cell-cycle, which is different than the pattern seen in microalgal species with permanent plastids. Furthermore, when quantitative real-time PCR combined with flow-cytometry was used to follow D. caudata cultures during a 65 days starvation/feeding experiment, the cells first went through a steady decrease in plastid DNA during starvation. In contrast, after feeding on the ciliate Myrionecta rubra, plastid DNA in starved cells increased 7-fold, thereby directly revealing the kleptoplastic behavior. The main conclusion from this thesis is that Dinophysis cells are actively taking up kleptoplastids from the ciliates on which they feed, and that kleptoplasty is an important key to understand Dinophysis ecology. Part of this thesis work has also been dedicated to the application and optimization of new methods, and it shows how quantitative real-time PCR, flow cytometry and molecular methods in different combinations can be used as powerful tools for the study of plankton ecology.

Dinophysis

kleptoplastid

real-time PCR

16S rRNA

plastid evolution

Baltic Sea

Flow cytometry

Marine ecology

Marin ekologi

Implication des protéines WHIRLY dans la biogénèse du chloroplaste en association avec la protéine SIG6

Truche, Sébastien

12 1900

Le mode vie autotrophique des plantes repose entièrement sur l’intégrité du chloroplaste et notamment l’étape de la biogénèse. La transcription des gènes chloroplastiques, assurée par une PEP (ARN polymérase encodée par le chloroplaste) et deux NEPs (ARN polymérase encodée par le noyau), est l’une des étapes primordiales dans le développement d’un chloroplaste photosynthétique. On distingue trois classes de gènes chloroplastiques : les gènes de classe I, transcrit par la PEP exclusivement; les gènes de classe II, transcrits par la PEP ou les NEPs; et les gènes de classe III, transcrits exclusivement par les NEPs. Pour assurer sa fonction, la PEP doit être associée à des facteurs sigmas. L’un de ceux-ci, la protéine SIG6, est un facteur sigma général et, associé à la PEP, assure la transcription de l’ensemble des gènes de classe I et II lors du développement du chloroplaste photosynthétique. Ainsi, le mutant sig6 présente un phénotype de cotylédons pâles, associé à un retard de biogénèse chloroplastique, ainsi qu’une diminution de la transcription des gènes de classe I, provoquant la diminution de la quantité de protéines de classe I. Dans le laboratoire, nous étudions les deux protéines WHIRLY chloroplastiques (WHY1 et WHY3) pour leur rôle dans le maintien de la stabilité génomique chloroplastique. Toutefois, peu de choses sont encore connues sur leur rôle potentiel dans la transcription ou la biogénèse chloroplastique. Par exemple, lorsque l’on tente de purifier la PEP, on obtient un gros complexe transcriptionnel nommé PTAC (Plastid Transcriptionally Active Chromosome) dans lequel sont retrouvées les deux protéines WHIRLY, suggérant qu’elles pourraient être impliquées dans la transcription chloroplastique. De plus, un possible rôle dans la biogénèse chloroplastique leur a été prêté, notamment chez le maïs. Dans cette étude, nous avons donc cherché à vérifier l’implication des protéines WHIRLY dans la biogénèse chloroplastique par une approche génétique de croisements entre les mutants sig6 et why1why3. Pour cela, nous avons isolé des doubles mutants sig6why1 et sig6why3, ainsi qu’un triple mutant sig6why1why3. À l’aide d’une caractérisation phénotypique et de la quantification de quelques protéines chloroplastiques, nous avons remarqué que la perte d’un des WHIRLY permet de complémenter le phénotype de cotylédons pâles du mutant sig6 et favorise l’expression normale de protéines en principe sous-exprimées dans le mutant sig6. Toutefois, la perte des deux WHIRLY ne permet pas de compenser le phénotype de cotylédons pâles et provoque l’apparition d’un phénotype persistant associé à une expression anormale des protéines chloroplastiques. Ces résultats ne peuvent être expliqués par le rôle des WHIRLY dans le maintien de la stabilité génomique chloroplastique étant donné que le triple mutant sig6why1why3 présente moins de réarrangements que le double mutant why1why3. Finalement, nous montrons que les effets de la perte d’un WHIRLY sur le mutant sig6 peuvent être mimés par l’utilisation de la rifampicine, une drogue inhibant l’ARN polymérase chloroplastique de type bactérienne (PEP). Ensemble, ces résultats démontrent donc l’implication des protéines WHIRLY chloroplastiques dans la biogénèse chloroplastique en association avec la protéine SIG6. Nous proposons un modèle selon lequel les deux protéines WHIRLY permettraient de favoriser l’activité de l’ARN polymérase de type bactérienne, notamment lors du développement du chloroplaste photosynthétique. En cas d’absence d’une des deux protéines, cette diminution partielle d’activité de la PEP favoriserait la mise en place d’un mécanisme de complémentation par le NEPs, permettant finalement de rétablir la biogénèse chloroplastique dans un mutant sig6. En l’absence des deux WHIRLY, le mécanisme de complémentation par les NEPs serait incapable de compenser la forte inhibition de la PEP, se traduisant par une aggravation du retard de développement du chloroplaste dans le mutant sig6. / The autotrophic lifestyle of plants relies entirely on the integrity of chloroplasts and particularly on their biogenesis. Chloroplast gene transcription, performed by a Plastid-Encoded Polymerase (PEP) and two Nuclear-Encoded Polymerases (NEPs), is one of the key steps during the development of photosynthetic chloroplast. There are 3 classes of genes, one transcribed by PEP alone (class I), one by both PEP and NEPs (class II), and the third by NEPs alone (class III). To carry out transcription, PEP associates with plastid sigma factors including the general sigma factor SIG6. sig6 mutants have a pale cotyledon phenotype, a severe decrease in class I gene transcription and a reduction in the level of class I proteins. In our laboratory, we study the role of the two plastid WIHRLY proteins (WHY1 and WHY3) in maintaining plastid genome stability. However, little is known about any role these proteins may play in transcription or chloroplast biogenesis. It seems likely they are involved in plastid gene transcription since they are found in the Plastid Transcriptionally Active Chromosome (PTAC). Moreover, they have been implicated in chloroplast biogenesis in maize. In this study, we verified the implication of these proteins in plastid biogenesis using a genetic approach in which we crossed a sig6 mutant with a why1why3 mutant. We isolated sig6why1 and sig6why3 double mutants and a sig6why1why3 triple mutant. Using a phenotypic characterisation and quantification of some plastid proteins, we show that loss of one of the two Why genes complements the sig6 pale cotyledon phenotype and allows a more normal pattern of expression of plastid proteins that are under-expressed in the sig6 mutant. However, we also show that loss of the two Why genes does not alleviate the sig6 phenotype. Moreover, the triple mutant shows a second pale phenotype on true leaves, and the plastid protein expression pattern is abnormal compared to either sig6 or wild type plants. Those results cannot be explained by the role of WHIRLY proteins in plastid genome stability since the triple mutant shows fewer plastid genome rearrangements than the why1why3 mutant. Finally, we show that inhibition of the PEP polymerase using rifampicin elicits the same complementation of the sig6 phenotype as the loss of one of the two WHIRLY. Together, these results show the implication of WHIRLY proteins in plastid biogenesis in association with SIG6. We propose a model in which WHIRLY act as activators of PEP activity, particularly during the chloroplast biogenesis. Therefore, the absence of one of the WHIRLY would cause a weak inhibition of PEP, facilitating the set-up of a rescue mechanism by NEPs and, consequently, allowing the complementation of plastid biogenesis in the sig6 mutant. However, the absence of the two WHIRLY proteins would cause a strong inhibition of PEP, and the inability of the rescue mechanism by NEPs to compensate for this strong inhibition, resulting in a more severe phenotype in the sig6 mutant.

Sig6

Whirly

Chloroplaste

Transcription

PEP

Rifampicine

Biogénèse chloroplastique

Chloroplast

Plastid biogenesis

Rifampicin