A model system using insects to vector Fusarium tumidum for biological control of gorse (Ulex europaeus)

Yamoah, Emmanuel

January 2007

The overall objective of this study was to test the hypothesis that insects can vector F. tumidum conidia to infect gorse plants with the aim of developing an alternative approach to mycoherbicide delivery to control weeds. Four potential insect species (Apion ulicis, Cydia ulicetana, Epiphyas postvittana and Sericothrips staphylinus) were assessed for their ability to vector F. tumidum conidia. To achieve this, the external microflora (bacteria and fungi) and the size and location of fungal spores on the cuticle of these insect species were determined. In addition, the ability of the insects to pick up and deposit F. tumidum conidia on agar was studied. Based on the results from these experiments, E. postvittana was selected for more detailed experiments to determine transmission of F. tumidum to infect potted gorse plants. The factors promoting pathogenicity of F. tumidum against gorse and the pathogen loading required to infect and kill the weed were also determined. The external microflora of the four insect species were recovered by washing and plating techniques and identified by morphology and polymerase chain reaction restriction fragment length polymorphism (PCR-RFLP) and sequencing of internally transcribed spacer (ITS) and 16S rDNA. A culture-independent technique (direct PCR) was also used to assess fungal diversity by direct amplification of ITS sequences from the washings of the insects. All insect species carried Alternaria, Cladosporium, Nectria, Penicillium, Phoma, Pseudozyma spp. and entomopathogens. Ninety four per cent of the 178 cloned amplicons had ITS sequences similarity to Nectria mauritiicola. E. postvittana carried the largest fungal spores (mean surface area of 125.9 ìm2) and the most fungal CFU/insect. About 70% of the fungi isolated from the insects were also present on the host plant (gorse) and the understorey grass. The mean size of fungal spores recovered from the insect species correlated strongly with their body length (R² = 85%). Methylobacterium aquaticum and Pseudomonas lutea were common on all four insect species. Pseudomonas fluorescens was the most abundant bacterial species. In the pathogenicity trials, the effectiveness of F. tumidum in reducing root and shoot biomass of 16 and 8 wk old gorse plants was significantly increased with wounding of the plants. Older plants (32 wk old) which were wounded and inoculated were significantly shorter, more infected and developed more tip dieback (80%) than plants which were not wounded (32%). This indicates that damage caused by phytophagous insect species present on gorse through feeding and oviposition may enhance infection by F. tumidum. Wounding may release nutrients (e.g. Mg and Zn) essential for conidia germination and germ tube elongation and also provide easier access for germ tube penetration. Conidial germination and germ tube length were increased by 50 and 877%, respectively when incubated in 0.2% of gorse extract solution for 24 h compared with incubation in water. Inoculum suspensions amended with 0.2% of gorse extract caused more infection and significantly reduced biomass production of 24 wk old gorse plants than suspensions without gorse extract. A minimum number of about 900 viable conidia/infection site of F. tumidum were required to infect gorse leaves. However, incorporation of amendments (which can injure the leaf cuticle) or provision of nutrients (i.e. gorse extract or glucose) in the formulation might decrease the number of conidia required for lesion formation. Scanning electron micrographs showed that germ tube penetration of gorse tissue was limited to open stomata which partly explain the large number of conidia required for infection. The flowers and leaves were more susceptible to F. tumidum infection than the spines, stems and pods. An experiment to determine the number of infection sites required to cause plant mortality showed that the entire plant needs to be inoculated in order for the pathogen to kill 10 wk old plants as F. tumidum is a non systemic pathogen. The number of infection sites correlated strongly with disease severity (R² = 99.3%). At least 50% of the plant was required to be inoculated to cause a significant reduction in shoot dry weight. F. tumidum, applied as soil inoculant using inoculated wheat grains in three separate experiments, significantly suppressed gorse seedling emergence and biomass production. In experiments to determine the loading capacity of the insect species, E. postvittana, the largest insect species studied, carried significantly more (68) and deposited significantly more (29) F. tumidum conidia than the other species. Each E. postvittana, loaded with 5,000 conidia of F. tumidum, transmitted approximately 310 conidia onto gorse plants but this did not cause any infection or affect plant growth as determined by shoot fresh weight and shoot height. E. postvittana on its own did not cause any significant damage to gorse and did not enhance F. tumidum infection. It also failed to spread the pathogen from infected plants to the healthy ones. There was no evidence of synergism between the two agents and damage caused by the combination of both E. postvittana and F. tumidum was equivalent to that caused by F. tumidum alone. This study has shown that E. postvittana has the greatest capacity to vector F. tumidum since it naturally carried the largest and the most fungal spores (429 CFU/insect). Moreover, it naturally carried Fusarium spp. such as F. lateritium, F. tricinctum and Gibberella pulicaris (anamorph Fusarium sambucinum) and was capable of carrying and depositing most F. tumidum conidia on agar. Coupled with the availability of pheromone for attracting the male insects, E. postvittana may be a suitable insect vector for delivering F. tumidum conidia on gorse using this novel biocontrol strategy. Although it is a polyphagous insect, and may visit non-target plants, F. tumidum is a very specific pathogen of gorse, broom and a few closely related plant species. Hence, using this insect species to vector F. tumidum in a biological control programme, should not pose a significant threat to plants of economic importance. However, successful control of gorse using this "lure-load-infect" concept would depend, to a large extent on the virulence of the pathogen as insects, due to the large size of F. tumidum macroconidia, can carry only a small number of it.

Fusarium tumidum

insect microflora

PCR-RFLP

ITS

16S rDNA

mycoherbicide

gorse

biological control

wounding

insect vectors

lure-load-infect

Caractérisation microbiologique de l'argile à Opalinus du Mont Terri et de l'argilite du Callovo-Oxfordien de Meuse/Haute-Marne

Poulain, Sebastien

12 December 2006

Cette thèse entre dans le cadre des recherches de l'axe II de la loi Bataille (30/12/1991) sur l'éventualité d'un stockage des déchets nucléaires de haute activité à vie longue en couches géologiques profondes. A son voisinage, la présence de microorganismes pourrait influencer la mobilité de radionucléides issus des colis de déchets. Ce travail a consisté à rechercher la présence de microorganismes autochtones dans l'argile à Opalinus du Mont Terri (Suisse) et dans l'argilite du Callovo-Oxfordien de Meuse/Haute-Marne (France). L'exploration de ces environnements jusqu'à présent peu étudiés du point de vue microbiologique indique une très faible densité cellulaire dans ces sédiments argileux, mais a néanmoins conduit à l'isolement d'espèces bactériennes nouvelles. De plus, des analyses microbiologiques ont permis la caractérisation d'une partie de la population microbienne introduite dans le laboratoire souterrain de Meuse/Haute-Marne par la ventilation du site et l'activité humaine.

[CHIM] Chemical Sciences

[SDV] Life Sciences

argile

cultures d'enrichissement microbien

rDNA-PCR

séquençage

Mapping the Distribution of the EPS Matrix Within Mixed Microbial Flocs

Khezry, Mojtaba

22 May 2012

The efficacy Biological wastewater treatment process is largely dependent on the formation of microbial flocs and settleability before the water is released into the environment. Settleability and flocculation are reliant upon stable physicochemical parameters. Extracellular polymeric substance constituents dictate physicochemical parameters of flocs. The fluctuation of these constituents within mixed microbial flocs is poorly studied. A novel aspect of this research was the use of CLSM data to get a semi- quantitative assessment of the constituents within mixed microbial flocs. Wastewater treatment flocs were characterized for eubacterial ecology, physicochemical properties, and they were visualized through correlative microscopy. It was observed that the microbial communities from the three sampling sites exhibited significant variability in numerous physicochemical properties. Overall, these results provide a first step to examine micro-localization of physicochemical properties, architecture and processes within flocs that may help better understand the causes of floc- related inefficiencies in biological wastewater treatment. / Canadian Hemophilia Society

Wastewater treatment

EPSprotein:EPScarbohydrate

CLSM

COM

SAXS

TEM

Mapping Distribution

EPS

Correlative Microscopy

DGGE

physicochemical

bacterial 16S rDNA

Anàlisi polifàsica de soques de "Pseudomonas fluorescens" potencials agents de biocontrol de malalties de fruiters

Badosa Romañó, Esther

21 December 2001

Molts bacteris del grup fluorescent del gènere Pseudomonas són capaços de controlar malalties de les plantes causades per fongs i bacteris fitopatògens (ACBs) o mostren activitat com a bacteris promotors del creixement de les plantes (BPCPs). S'han descrit diversos metabòlits que intervenen de manera important en la seva activitat com a ACBs i BPCPs entre els quals en destaquen el 2,4-diacetilfloroglucinol (Phl), àcid fenazin-1-carboxílic (PCA), Pirrolnitrina (Prn), àcid cianhídric (HCN), àcid 3-indolacètic (IAA), sideròfors i quitinases.L'objectiu principal del nostre treball ha estat la comparació de les característiques d'un grup de Pseudomonas del grup fluorescent utilitzant una aproximació polifàsica amb la finalitat d'establir possibles relacions entre algunes de les característiques i la capacitat d'actuar com a ACB o BPCP.Atesa la importància en el biocontrol de la producció de metabòlits com Phl, PCA i Prn, l'objectiu preliminar ha estat la recerca i obtenció de soques productores d'aquests metabòlits. Per assolir aquest objectiu s'ha emprat una aproximació molecular basada en la detecció dels gens biosintètics implicats en la seva producció en lloc de la detecció directa dels metabòlits per evitar els efectes que poden tenir les condicions de cultiu en la inducció o repressió de la seva síntesi. S'han realitzat diferents protocols basats (i) en la cerca assistida de productors mitjançant l'ús de marcadors fenotípics i posterior confirmació per PCR i, (ii) en l'ús de la PCR per a la detecció dels gens directament dels extractes bacterians, d'enriquiments d'aquests extractes i la realització de la hibridació en colònies per al posterior aïllament. La cerca assistida de productors de Phl mitjançant marcadors fenotípics i posteriorment la utilització de tècniques moleculars (amplificació per PCR del gen phlD), ha estat el millor mètode en el tipus de mostres processades en el nostre treball, on la proporció de productors és relativament baixa. En total s'han aïllat a partir de diversos ambients 4 soques portadores dels gens de la síntesi de PCA, 15 de Phl i 1 de Prn.S'ha constituït una col·lecció de 72 soques de Pseudomonas del grup fluorescent que inclou 18 aïllats propis portadors dels gens biosintètics necessaris per la producció de Phl PCA i Prn; 6 soques de referència procedents de col·leccions de cultius tipus, 14 soques productores dels diferents antibiòtics cedides per altres investigadors i una selecció de 34 soques procedents d'un treball previ realitzat en el nostre grup de recerca. A la col·lecció s'hi troben soques candidates a ACB i BPCP de diverses malalties i plantes.Les 72 soques s'han caracteritzat fenotípica i genotípicament. La caracterització fenotípica s'ha portat a terme mitjançant la identificació a nivell d'espècie amb galeries API 20NE i proves bioquímiques específiques; la producció de metabòlits com PCA, Phl, Prn, IAA, HCN, quitinases i sideròfors mitjançant l'ús de diferents tècniques; antagonisme in vitro en diversos medis enfront dos fongs (Stemphylium vesicarium i Penicillium expansum) i tres bacteris fitopatògens (Erwinia amylovora, Pseudomonas syringae pv. syringae i Xanthomonas arboricola pv. juglandis); l'eficàcia de la inhibició de la infecció en bioassaigs in vivo sobre material vegetal enfront els fongs P. expansum en poma i S. vesicarium en fulles de perera i enfront el bacteri E. amylovora en fruits immadurs de perera i, finalment, en assaigs de promoció de creixement en dos portaempelts comercials de Prunus. Cal destacar que P. expansum causa la podridura blava en pomes i peres en postcollita, S. vesicarium la taca bruna de la perera i E. amylovora el foc bacterià de les rosàcies.El nombre de soques de Pseudomonas, sobre el total de les 72 estudiades, productores d'IAA (4) i quitinases (6) és baix, mentre que és elevat en el cas del HCN (32), que a més està associat a la producció de Phl. Els resultats obtinguts en l'antagonisme in vitro han mostrat en el cas dels bacteris que és dependent del patogen indicador i del medi de cultiu. La presència o absència de ferro no sembla ser un factor que potencií l'antagonisme. En el cas dels fongs no s'ha observat però, influència del medi de cultiu emprat. En el total de 72 soques s'ha observat un percentatge baix de soques que manifesten antagonisme en tots els medis assajats vers 3 o 4 dels patògens (7). Solament 2 d'aquestes 7 soques han mostrat ser també efectives en bioassaigs d'inhibició de les infeccions causades per 2 dels 3 patògens assajats. Algunes de les soques efectives en els bioassaigs no són antagonistes in vitro en cap dels medis assajats enfront el mateix patogen. En el cas de la promoció del creixement, s'han observat més soques promotores del creixement del portaempelts de prunera Marianna 2624 que no en l'híbrid de presseguer-ametller GF677 i les eficàcies assolides són també majors en el cas de Marianna 2624, detectant una elevada especificitat soca/portaempeltsLa caracterització genotípica s'ha realitzat mitjançant l'anàlisi dels polimorfismes en la longitud dels fragments de restricció de DNA ribosomal (RFLP-rDNA) i l'anàlisi dels polimorfismes en la longitud dels fragments de macrorestricció genòmica de DNA cromosòmic separats per electroforesi en camp polsant (MRFLP-PFGE). Ambdues anàlisis van mostrar una gran heterogeneïtat genètica entre les soques caracteritzades i no s'ha pogut relacionar les agrupacions obtingudes amb les característiques fenotípiques o capacitat d'actuar com a ACB o BPCP. Els patrons de macrorestricció genòmica (MRFLP-PFGE) del bacteri model P. fluorescens EPS288 són estables en el temps i independents de les condicions de cultiu assajades al laboratori o en mostres naturals, mostrant ser una tècnica eficaç en la identificació de reaïllats de mostres naturals inoculades prèviament amb el bacteri.Una selecció de soques que comparteixen el fet de produir floroglucinol s'han caracteritzat mitjançant RFLP i seqüenciació del gen phlD. S'ha establert una relació entre les agrupacions obtingudes en les anàlisis RFLP-rDNA, RFLP-phlD i les seqüències del gen. En l'anàlisi filogenètica de les seqüències del gen phlD s'ha observat un elevat grau de polimorfisme obtenint-se 3 agrupacions principals. Les agrupacions semblen relacionar-se amb els patrons de producció de metabòlits (Phl, HCN i Prn en una primera agrupació; Phl i HCN en la segona i solament Phl en la tercera), però aquestes no s'han pogut relacionar amb l'origen geogràfic de les soques o la seva activitat com a ACBs i/o BPCP.Amb les dades obtingudes de la caracterització fenotípica i genotípica s'ha realitzat una anàlisi multivariant (correspondències, correlacions d'Spearman i de freqüències amb variables categòriques). S'ha demostrat la importància de disposar d'una tècnica que permeti depurar una col·lecció de soques descartant les soques genèticament idèntiques, ja que influeixen en els resultats de les anàlisis. Pels tres patògens assajats com a indicadors i els dos portaempelts emprats, no s'ha observat cap correlació entre la inhibició de la infecció o la promoció del creixement amb les característiques fenotípiques i genotípiques de les soques que fos significatiu i consistent en les tres tècniques emprades. / Many bacteria pertaining to the fluorescent Pseudomonas group are able to control plant diseases caused by bacterial and fungal plant pathogens (BCAs). Also, some of them exhibit activity as plant growth promoting bacteria (PGPBs). Several metabolites like 2,4-diacetylphloroglucinol (PHL), phenazin-1-carboxilic acid (PCA), pyrrolnitrin (Prn), hydrogen cyanide (HCN), indol-3-acetic acid, siderophores and chitinases has been described accounting for their ability of being BCAs or PBPBs.The aim of the present work was to compare the phenotypic and genotypic characteristics of a selected group of fluorescent Pseudomonas by means of a polyphasic approach in order to establish relationships with the ability of being BCA and PGPB.Due to the importance of production of metabolites like Phl, PCA and Prn in biocontrol, the preliminary objective of this work was to search and isolate of metabolite producing strains. To achieve this objective a molecular approach was used based on the detection of biosynthetic genes, which are implicated in the metabolite production, instead of direct detection of the metabolites. The procedure was performed to avoid the effect of culture conditions on induction or repression of metabolite synthesis. Two procedures were used (i) assisted search of metabolite producing strains by means of phenotypic markers and subsequent confirmation by PCR analysis, (2) direct use of PCR for gene detection in direct extracts or enrichments from samples and subsequent colony-hybridization for assistance in strain isolation. The best method for isolation of Phl producers in the type of samples processed in the present work, where the frequency of Phl producers is very low, was the assisted search by means of phenotypic markers followed of a confirmation by PCR amplification of phlD gene. Four strains harboring the PCA genes, 15 strains with Phl genes, and one with Prn genes were isolated.A collection of 72 strains of Pseudomonas pertaining to the fluorescent group was made including 18 isolates derived from the present work which harbor the biosynthetic genes for PhL, PCA and Prn production; 6 strains from reference collections; 14 strains producing several antibiotics which were supplied by other colleagues; and a selection of 34 strains from a previous work performed by our research group. Within the collection there are many strains with promising potential as BCAs and PGPBs of several diseases and plant hosts.The collection was characterized phenotypically and genotypically. The phenotypic characterization included identification at the species level with the aid of API20NE kit and several specific biochemical tests; the production of metabolites such as PCA, Phl, Prn, IAA, HCN, chitinases and siderophores; in vitro antagonism in several culture media against two fungi (Stemphylium vesicarium and Penicillium expansum) and three bacterial pathogens (Erwinia amylovora, Pseudomonas syringae pv. syringae and Xanthomonas arboricola pv. juglandis); efficacy in biossays of inhibition of infection of plant material by P. expansum on apple fruit tissue and S. vesicarium on pear leaves, E. amylovora on immature pear fruit, and of growth promotion in two commercial Prunus rootstocks. P. expansum causes blue mold rot of apple and pear in postharvest, S. vesicarium cause brown spot of pear and E. amylovora is the causal agent of fire blight of rosaceous plants.The number of strains, over a total of 72 studied, producing IAA and chitinases was very low (4 producing IAA and 6 producing chitinases), whereas a high number of HCN producing strains (32) was detected which was associated to Phl production. In vitro antagonism against bacteria was highly dependent on indicator pathogen and growth medium, but the presence or absence of iron did not seem to affect. However, in the case of antagonism against fungi, no influence of the medium composition was observed. Among the collection a low frequency of strains exhibiting antagonism against 3 or 4 pathogens a total of 7 strains was observed in all tested media. Only two out of the seven strains were effective in infection inhibition bioassays caused by two of the three pathogens tested. Some of the effective strains in the in vivo assays were not antagonist for the indicator pathogen in any of the media tested. In the case of plant growth promoting strains, the growth in rootstock Marianna 2624 was more stimulated than in GF677, and there was a strain-host specificity. Genotypic characterization of strains was performed by means of restriction fragment length polymorphism analysis of the ribosomal DNA (RFLP-rDNA) and macrorestriction fragment length polymorphism analysis of chromosomal DNA separated by pulsed field gel electrophoresis (MRFLP-PFGE). Both techniques showed a high level of genotypic diversity within the collection of strains, and no relationships were observed between clusters and phenotypic characteristics or ability to be BCA or PGPB. Patterns of MRFLP-PFGE for the model bacterium P. fluorescens EPS288 were found stable within time and independent of cultivation conditions in the laboratory or under natural conditions. Therefore the method is highly suitable for identification of strains reisolated from natural samples previously inoculated with the bacterium.A further selection of strains which produce phloroglucinol were characterized by RFLP analysis and phlD sequencing. The groups observed were consistent among the RFLP-rDNA, RFLP-phlD and gene sequence data. Phylogenetic analysis obtained using phlD sequences showed a high level of polymorphism revealing three main clusters. These clusters appear to be related with metabolite production: a first cluster producing Phl, HCN and Prn, a second producing Phl and HCN, and a third producing only Phl. However, this groups were related neither to the geographic origin of strains nor to the activity as BCA or PGPB.A multivariate analysis (correspondence, pairwise Spearman rank correlation, and frequency analysis)was performed using data of phenotypic and genotypic characterization of strains. The results emphasize the importance of discarding from the database those strains being genetically identical because skew the final results. The three types of analysis did not revealed a significant and consistent relationship between the activity of infection inhibition or growth promotion of the strains and their characteristics.

16-23s rDNA(ITS)

Metabòlits secundaris

Metabolitos secundarios

Secondary metabolites

Pseudomonas fluorescens

Antibióticos

Antibiotics

Phytopathologia

PCR

Fitopatologia

PFGE

577

632

Arquitetura da cromatina na região organizadora do nucléolo e o seu papel no controle da expressão dos genes ribossomais / Nucleolus Organizer Regions chromatin architecture and its role in ribosomal genes expression

Larissa Mara de Andrade

30 September 2011

O nucléolo é uma organela nuclear responsável pela produção dos ribossomos, através das Regiões Organizadoras do Nucléolo (NORs). Espécies que possuem mais de um par de cromossomos contendo NORs terão, obrigatoriamente, pelo menos um par ativo, sendo as demais NORs funcionais de acordo com a demanda celular. O mecanismo de compensação de dose é visualizado e bem estabelecido em híbridos interespecíficos, conhecido como dominância nucleolar, com a inativação de NORs de um dos parentais por outras homeólogas ativas que as dominam. A arquitetura da cromatina nas NORs e o controle da sua expressão foram estudados com o objetivo de se entender os mecanismos envolvidos no fenômeno da dominância nucleolar em espécies diplóides que possuem múltiplas NORs. A espécie modelo utilizada neste estudo foi Crotalaria juncea (Leguminosae-Papilionoideae), caracterizada por conter 2n=2x=16, e NORs no braço curto do cromossomo 1, sendo este o principal organizador do nucléolo, e no braço longo do cromossomo 4 adjacente à heterocromatina centromérica, sendo este um sítio adicional (sítio menor) e de expressão facultativa, previamente determinada. Nas raízes de C. juncea sincronizadas, observou-se que a nucleologênese tem seu início durante o final da telófase, em que os 4 sítios de genes ribossomais podem ter atividade e formar até 4 nucléolos, os quais tendem a se fundir durante a interfase. A Hibridação in situ fluorescente (FISH) permitiu estudos da arquitetura da cromatina, com a visualização dos territórios cromossômicos, onde a cromatina não está organizada de forma aleatória dentro do núcleo, e consequentemente o rDNA 45S dentro do nucléolo. Observou-se também que todos os sítios de rDNA 45S possuem diferença no tamanho do arranjo repetitivo. Assim sendo, a hierarquia de dominância está de acordo com o tamanho de cada arranjo (sítio), e estes são ativados de acordo com a demanda celular. As análises das modificações nas histonas mostraram que a H3K9Met1 apresentou marcas fracas no nucléolo, enquanto no restante da cromatina nuclear sua marcação foi intensa. Já a H3K9Met2 apresentou marcação fortemente associada à cromatina presente no nucléolo, com alguns pequenos pontos heterocromáticos dispersos no núcleo. Pela observação entende-se que ambas metilações controlam diferentes tipos de heterocromatinas, ou seja, a H3K9Met2 controla principalmente heterocromatinas associadas aos genes ribossomais, e a H3K9Met controla heterocromatinas não associadas ao rDNA. O rDNA é hiperacetilado dentro do nucléolo para a H3K14. Não foi observada marcação nucleolar para H4K8ac, mas pôde ser observadas regiões hiperacetiladas em outras regiões da cromatina. A metilação do DNA esteve diretamente associada à diferentes níveis de organização da cromatina das NORs. As heterocromatinas adjacentes ao nucléolo apareceram fortemente metiladas, enquanto a cromatina distendida dentro do nucléolo apresentou marcação dispersa, com algumas regiões mais fortemente marcadas, onde a cromatina apresentava-se mais condensada e provavelmente não associados com a cromatina ativa. As fibras estendidas permitiram uma análise de alta resolução, onde foi possível observar que regiões não metiladas apareciam intercaladas entre grandes regiões fortemente metiladas, sugerindo que estas regiões hipometiladas estão, possivelmente, associadas com as alças de transcrição dentro do nucléolo. 12 Esses resultados contribuem para o entendimento sobre o controle genético e epigenético na arquitetura da cromatina ribossomal, bem como seu controle na expressão dos genes ribossomais no genoma das plantas. / The nucleolus is a nuclear organelle responsible for the ribosomes production, by Nucleolus Organizer Regions (NORs). Species presenting more than one chromosome pair with NORs should present, one pair expressing the genes, at least; while the other pairs expressing their genes accordingly to cellular demand. Dosage compensation mechanism is visualized and well established of interspecific hybrids as a well-described phenomena named nucleolar dominance, where a NOR from one parental could lead to inactivation of a NOR from the other parental which is dominated. The chromatin architecture and expression of the NORs were studied to address the mechanism involved in the nucleolar dominance of diploid species containing multiple sites of 45S rDNA. The model species used in the present study was the crop Crotalaria juncea (Leguminosae-Papilionoideae) characterized by 2n=2x=16 chromosomes, being the main NOR mapped into chromosome 1 short arm and presenting an additional site (minor site) in the chromosome 4 long arm adjacent to a centromeric heterochromatin and facultatively expressed. Synchronized meristematic root tip cells determined to nucleologenesis starts during the late-telophase, often expressing every ribosomal gene sites, when up to four nucleoli could be observed and these become merged during interphases. FISH allowed nucleolar chromatin architecture be accessed revealing distinct chromosomal domains (territories), suggesting a non-random distribution of the 45S rDNA, even between homologous chromosomes, into the nucleolus. The 45S rDNA sites from both chromosome pairs 1 and 4 of C. juncea showed differences in their array sizes. The differences in the 45S rDNA array sizes and the order of loci expression suggest a hierarchy of dominance, a feature of nucleolar dominance; being the small RONs activated only on demand. Immunodetection of histone modifications showed different patterns to methylation distribution across the chromatin as a whole; where H3K9Met1 was found mainly distributed along the nuclear chromatin without an evident signal into nucleolus, while H3K9Met2 was detected as conspicuous dots in the nuclear chromatin and highly accumulated into the nucleolus. The results indicate different control on heterochromatin establishment and maintenance, being the modifications specific to certain chromosomal regions. Indeed, H3K9Met is a key component in the nucleolus chromatin architecture and expression. The chromatin inside the nucleolus showed a high accumulation of H3K14ac, with a weak fluorescent signal along the nucleus; on the other hand H4K8ac showed a strong signal homogenously distributed across the nuclear chromatin, but without evident signals inside the nucleolus. DNA methylation was directly associated with different levels of chromatin organization of the NORs. The heterochromatic regions associated to RON are highly methylated, while the chromatin inside the nucleolus showed weaker signals, with some bright spots probably in condensed regions and related to chromatin inactivity. Extended DNA fiber allowed a higher resolution mapping that revealed long methylated regions intermingled by nomethylated ones, being the last probably associated to transcriptional loops of rRNA genes into the nucleolus. The results presented herein contributes to a better understand about the nucleolar chromatin architecture and the genetic and epigenetic control of the ribosomal genes expression on plant genomes.

Citogenética

Cromatina

Cromossomos

DNA

Expressão gênica

Genes

Genomas

Nucléolo.

45S rDNA

Additional loci

DNA methylation

Epigenetics.

FISH

Histones modifications

Nucleolus

Interação entre bactérias endofíticas e do rizoplano com Eucalyptus / Interaction between endophytic and rhizoplane bacteria with Eucalyptus

Anderson Ferreira

15 February 2008

Os microrganismos endofíticos são aqueles, cultiváveis ou não, que habitam o interior da planta hospedeira sem causar danos aparentes ou estruturas externas visíveis. Essa interação microrganismos-planta é intrínseca a determinadas espécies de plantas e/ou bactérias. Nas últimas décadas os estudos de microrganismos endofíticos têm sido realizados em diversas plantas hospedeiras, sendo esses estudos direcionados principalmente para a diversidade e características benéficas induzidas, inclusive o controle biológico de doenças. A doença causada pelo fungo Ceratocystis fimbriata é considerada emergente no setor florestal. O Brasil está entre os maiores produtores mundiais de eucalipto e a expansão do setor juntamente com o cultivo clonal tem acarretado o aumento da incidência de patógenos. O surgimento de novas doenças exige estudos relacionados tanto a interação do agente patogênico com hospedeiro quanto de todos os componentes do patossistema. Neste contexto, os microrganismos endofíticos têm sido descritos como potenciais controladores biológicos de doenças. Dessa forma, o presente trabalho teve por objetivos avaliar a interação de C. fimbriata com a comunidade bacteriana associada à Eucalyptus sp. Adicionalmente, foi estudada a possível transferência desses endófitos via sementes e o padrão de colonização de Pantoea agglomerans em plântulas. Foi observado que plantas não infestadas por C. fimbriata apresentaram maior densidade bacteriana no rizoplano (20,66 x 104 UFC.cm2 -1 de raiz), enquanto que para a comunidade endofítica, a maior densidade foi observada em plantas infectadas pelo fungo (25,13 x 104 UFC.g-1 de raiz). As análises por ARDRA possibilitaram a obtenção de 8 e 13 ribotipos nas comunidades endofítica de raiz e do rizoplano, respectivamente. Os ribotipos mais freqüentes foram identificados como Bacillus cereus. As análises de diversidade por meio de DGGE das comunidades do rizoplano e endofítica de raiz mostraram que a infestação pelo fungo interfere na colonização de Eucalyptus. Foi observado também que bactérias endofíticas estão presentes no interior de sementes de Eucalyptus spp. em uma densidade de 0,33 a 1,83 X 102 UFC.g-1, para as espécies E. camandulensis e E. urophylla, respectivamente. A densidade bacteriana endofítica de plântulas obtidas de sementes desinfectadas superficialmente variaram entre 0,27 X 102 a 0,87 X 102 UFC.g-1, para E. citriodora e o híbrido E. robusta x E. grandis, respectivamente. Em algumas espécies de Eucalyptus não foram isoladas bactérias endofíticas das sementes e plântulas. Os resultados mostraram que algumas espécies de bactérias endofíticas podem ser transmitidas verticalmente por sementes. P. agglomerans inoculada nas sementes foi capaz de colonizar as plântulas após a germinação da semente, indicando que esta pode ser uma das formas utilizadas pelos microrganismos para colonizar e se estabelecer na planta hospedeira. Assim, os resultados obtidos neste trabalho mostram ainda que possa existir interação entre a presença de C. fimbriata e a comunidade bacteriana endofítica e do rizoplano de Eucalyptus. Foi possível observar também que estas bactérias endofíticas que são transmitidas por meio de sementes, permitindo que plântulas previamente inoculadas com bactérias benéficas possam ser produzidas antes de serem levadas a campo. / The endophytic microorganisms are those, cultivated or not, that inhabit the interior of the plant host without causing apparent damages or visible external structures. This interaction microorganisms-plant is specific to certain species of plants and/or bacteria. In the last few years studies of endophytic microorganisms have been carried out in several plant hosts, being these studies focused mainly to diversity and biotechnological potential, such as biological control of disease. The disease caused by the phytopathogenic fungi Ceratocystis fimbriata is considered emerging by the reforestation companies. Brazil is one of the largest world eucalyptus producers and the increasing of the eucalyptus production associated to clonal reproduction has allowed the increase in pathogen incidence. Studies that evaluate the interaction between pathogens and the microbial community associated to the host plant may allow understanding how disease symptoms come up. Endophytic microorganisms have been described as potential biological control of diseases and therefore, the aims of the present work were to i) study the interaction between C. fimbriata and the bacterial community associated to the Eucalyptus sp.; ii) evaluate the bacterial dissemination by seeds; iii) evaluate the colonization profile of Pantoea agglomerans in seedlings after seed inoculation. It was observed that the highest bacterial density on the rhizoplane (20.66 x 104 CFU.cm2 -1 of root) was observed in C. fimbriata uninfectedplants, while for endophytic community the highest density was observed in C. fimbriata infected plants (25.13 x 104 CFU.g-1 of root). The ARDRA analyses showed that the bacterial community of eucalyptus is composed by 8 and 13 ribotypes on rhizoplane and inside the roots (endophytic), respectively. The most frequent ribotypes were identified as Bacillus cereus. The DGGE analyses of diversity of endophytic and rhizoplane community showed that fungi infection shift the colonization of Eucalyptus associated bacteria. The bacterial community inside Eucalyptus spp. seeds ranged from 0.33 to 1.83 X 102 CFU.g-1, for E. camandulensis and E. urophylla, respectively. After seed germination the endophytic bacterial density in seedlings ranged from 0,27 X 102 to 0,87 X 102 CFU.g-1, for E. citriodora and the hybrid E. robusta x E. grandis, respectively. Although, endophytic bacteria have been isolated from seeds, for some plant species, bacteria were not isolated from seedlings. Also, some bacteria may be vertically transmitted from seed to seedlings, but some is specific for seeds. Seed inoculation of P. agglomerans resulted in seedlings colonized by these bacteria, suggesting that these bacteria could be seed transmitted. The results obtained in the present study show that the fungi C. fimbriata inside the Eucalyptus host can shift the endophytic and rhizoplane bacterial diversity. Also, these endophytic bacteria could be transmitted vertically by seeds, allowing that seeds previously inoculated with beneficial bacteria may result in protected plants before planting in the field.

Bactérias

Ecologia microbiana

Eucalipto

Fungos fitopatogênicos

Microrganismos endofíticos.

16S rDNA

DGGE

Fluorescence microscopy.

Microbial ecology

Plant microbe interctions

Diversidade genética de enterobactérias endofíticas de diferentes hospedeiros e colonização de Catharantus roseus por endófitos expressando o gene gfp. / Genetic diversity of endophytic enterobacteria from different hosts and colonization of Catharantus roseus by endophytes expressing gfp gene.

Adalgisa Ribeiro Torres

02 May 2005

Bactérias endofíticas são aquelas que habitam o interior de tecidos vegetais, sem causar dano aparente aos mesmos, além de desempenhar funções importantes no processo de adaptação das plantas. Especial interesse tem sido dado a tais bactérias devido ao seu potencial no controle biológico. Por isso, é muito importante estudar a diversidade genética de endófitos, além de avaliar o impacto da introdução de endófitos geneticamente modificados no ambiente. Estudos vêm sendo feitos nesse sentido, mas não com bactérias endofíticas da família Enterobacteriaceae. Desta forma, o presente trabalho teve como objetivos estudar a diversidade genética de bactérias endofíticas da família Enterobacteriaceae isoladas de plantas de cacau, cana-de-açúcar, citros, eucalipto e soja, utilizando diferentes técnicas moleculares. Análises por ARDRA e seqüenciamento do rDNA 16S identificaram 20 haplótipos e revelaram que os isolados pertenceram aos gêneros Enterobacter, Erwinia e Pantoea, sendo este último o mais freqüente. Tais estudos revelaram ainda que a diversidade dos isolados variou de acordo com a planta hospedeira. A técnica de BOX-PCR foi também utilizada para avaliar a diversidade dos isolados. Um total de 23 diferentes OTUs (operational taxonimic units) obtidas indicaram que o total de isolados avaliados compreenderam pelo menos 23 espécies diferentes. Dois isolados foram transformados com pPAgfp, um plasmídio contendo os genes de resistência ao antibiótico ampicilina e o gene gfp, que codifica a proteína verde fluorescente. Tais isolados foram inoculados em plântulas de Catharantus roseus (vinca) e foi feito reisolamento de bactérias endofíticas em dois períodos diferentes após a inoculação. O impacto desta inoculação na diversidade da comunidade microbiana natural de vinca foi avaliado utilizando-se a técnica de ARDRA, a qual mostrou que os endófitos expressando gfp colonizaram as raízes e caules das plantas inoculadas, sem causar qualquer sintoma de doença. Além disso, os colonizadores endofíticos não levaram à diminuição da diversidade da população microbiana natural de vinca. Os resultados obtidos poderão contribuir para a compreensão sobre a interação entre Enterobacteriaceae endofítica e planta hospedeira, além de ajudar a responder questões sobre o papel ecológico dos endofíticos e seu potencial biotecnológico. / Endophytic bacteria have been defined as those that reside within living plant tissues, or extracted from inner plant parts without causing apparent damage to them. They also are able to play an important role in the process of plant adaptation. There is an increasing interest to endophytic bacteria and its potential in the biological control and many studies has been done in order to evaluate the diversity and the impact of endophytes and genetically modified endophytes (GME) released into environment. In this way, information about the diversity of endophytic bacteria has been obtained, except for bacteria exclusively from Enterobacteriaceae family belonged to different host plants. Thus, the aim of the present work was study the diversity of Enterobacteriaceae bacteria isolated from citrus, cocoa, eucalypti, soybean and sugar cane by different molecular approaches. The 16S rDNA of each isolate was amplified by PCR and the isolates were grouped into 20 clusters by analysis of restriction patterns of the PCR-amplified 16S rDNA (ARDRA). These analysis showed a variety of organisms, with 5 different genera encountered: Pantoea was most frequently encountered followed by Enterobacter and Erwinia, which isolates presented the great bacterial diversity according to host plants. Through cluster analysis of the BOX-PCR technique profiles, 23 different OTUs (Operational Taxonomic Units) were distinguished, the presence of 23 OTUs could indicate that isolates comprised at least 23 different species. Two isolates were transformed with pPAgfp, a plasmid harboring the ampicillim resistance gene and the gfp gene, which encodes for the green fluorescent protein. These two isolates were inoculated in seedlings of Catharantus roseus (vinca) and re-isolation of endophytic was performed in two times after inoculation. The impact of endophytes inoculation was evaluated by using the ARDRA technique. It showed that endophytes expressing gfp colonized roots and shoots of inoculated plants without causing any symptom of disease. Besides, the endophytes colonizers do not decreased the diversity of the vinca’s natural microbiota. The results obtained here provided important insights into the endophytic Enterobacteriaceae-host relationship that will be useful for further answer basic questions about the ecological role of the endophytes and its biotechnological potential.

bactéria endofítica

diversidade genética

enterobactéria

marcador molecular

vinca

16S rDNA sequencing

box - pcr

enterobacteria - endophytes

genetic diversity

gfp

Controle genético e epigenético da expressão heteromórfica de regiões organizadoras do nucléolo em Crotalaria retusa L. (Leguminosae-Papilionoideae) / Genetic and epigenetic control of the heteromorphic expression of nucleolus organizer regions in Crotalaria retusa L. (Leguminosae-Papilionoideae)

Maria Cecília Perantoni Fuchs

16 September 2009

O presente trabalho teve por objetivo compreender e analisar os mecanismos genéticos e epigenéticos da expressão diferencial de regiões organizadoras do nucléolo - RONs através do estudo de dois acessos (CRT-1 e CRT-2) de Crotalaria retusa. O acesso CRT-1 é uma cultivar, enquanto que o acesso CRT-2 é proveniente de uma população periférica da orla marítima de Ilhéus BA. Por serem temporalmente e espacialmente separados, acredita-se que os acessos foram submetidos a pressões seletivas diferentes, resultando em alterações dos padrões epigenéticos, principalmente nas RONs. Para o desenvolvimento deste trabalho foram realizadas medidas cromossômicas e nucleolares a partir de células coradas pelo método de Feulgen e por nitrato de prata, coloração com fluorocromos específicos às regiões cromossômicas ricas em nucleotídeos GC e AT, mapeamento físico dos locos de DNA ribossômico 45S por hibridação in situ fluorescente, análise qualitativa e quantitativa de modificações pós-traducionais de histonas por Western blot e eletroforese bidimensional de extrato protéico radicular com enfoque em proteínas envolvidas nos mecanismos epigenéticos. As análises citológicas demonstraram uma grande semelhança nos cariótipos dos dois acessos, diferindo apenas no tamanho do segmento proximal do braço curto do cromossomo 1. Em ambos os acessos foi observada uma expressão nucleolar diferencial em, aproximadamente, 50% das células; contudo, a expressão diferencial em CRT-2 apresentou-se consideravelmente maior. Além disso, os dois acessos demonstraram diferenças quantitativas nas modificações pós-traducionais de histonas e em proteínas possivelmente envolvidas em mecanismos epigenéticos. Uma vez que as variações epigenéticas podem ser modificadas por fatores ambientais, sugere-se que as diferenças nos padrões de modificações de histonas e nos perfis protéicos encontradas entre os acessos, como também a expressão diferencial mais expressiva em CRT-2, sejam devidas às diferentes pressões seletivas as quais as populações originais foram submetidas. O estudo dos mecanismos genéticos e epigenéticos na dominância nucleolar possibilita uma maior compreensão da ação do remodelamento da cromatina no controle da expressão gênica do rDNA, como também da expressão gênica em geral. / The aim of this present work was to understand and analyze the genetic and epigenetic mechanisms of differential expression of the nucleolus organizer regions - NORs through the study of two accesses (CRT-1 and CRT-2) of Crotalaria retusa. Access CRT-1 is a cultivar, while access CRT-2 is from a peripheral population of the shoreline of Ilhéus BA. Because they are temporally and spatially separated, it is believed that the accesses were submitted to different selective pressures, resulting in changes in epigenetic patterns, primarily in NORs. To develop this work, it was carried out chromosomal and nucleolar measurements from cell stained by Feulgen method and silver nitrate, staining with specific fluorochromes to chromosomal regions rich in GC and AT nucleotides, physical mapping of 45S ribosomal DNA loci by fluorescent in situ hybridization, qualitative and quantitative analysis of post-translational histone modifications by western blot, and two-dimensional electrophoresis of root extract protein focusing on proteins involved in epigenetic mechanisms. The cytological analysis showed a great similarity in karyotypes of two accessions, differing only in size of the proximal segment of the sort arm of chromosome 1. In both accesses, it was observed a differential nucleolar expression in approximately 50% of the cells; however, the differential expression in CRT-2 showed considerably larger. Furthermore, the two accesses showed quantitative differences in the posttranslational histone modifications, and in a protein possibly involved in epigenetic mechanisms. Since epigenetic variations can be modified by environmental factors, it is suggested that differences in patterns of histone modifications and protein profiles found between the accesses, but also the most significant differential expression in CRT-2, are due to different selective pressures to which the original populations were submitted. Studies of the epigenetic mechanisms in nucleolar dominance allows a better understanding of the action of the remodeling of chromatin in controlling the dosage of rRNA genes, but also in the control of gene expression in general.

Citogenética vegetal

Controle genético

Crotalária

DNA

Expressão gênica

NucIeólo.

differential expression

Epigenetic

Nucleolar dominance

Nucleolar organizer region.

rDNA 45S

Damping-off and stem rot of cowpea in Benin caused by Sclerotium Rolfsii

Adandonon, Appolinaire

14 January 2005

The damping-off and stem rot disease syndrome is harmful to many cultivated crops. Damping-off and stem rot caused by Sclerotium rolfsii Sacc. on cowpea results in yield losses with serious socio-economic implications. The objectives of the present study were to investigate the occurrence of the diseases in Benin, study etiology and factors influencing the diseases, and develop strategies for the control of the diseases in the field. Results showed that the diseases are distributed countrywide. Sclerotium rolfsii was the main causal agent but minor pathogens, namely Pythium sp., Rhizoctonia solani Kühn and Phoma pomorum Thüm were also recorded. In the Ouémé valley, the diseases were favoured by soil moisture and S. rolfsii initial inoculum that were higher closer to the river. Sclerotium rolfsii isolates collected in the valley showed genetic diversity in terms of pathogenicity, mycelial compatibility groups and ITS rDNA sequences. A paper-based screening method was found to be a rapid laboratory method for screening for resistance in cowpea cultivars. Furtheremore, Moringa oleifera L. leaf extracts, Trichoderma Kd 63 and Trichoderma IITA 508 significantly reduced the disease incidence. The best disease control was recorded in the field when M. oleifera seed treatment was integrated with a soil sprinkle of Trichoderma. The present work provides information on damping-off and stem rot of cowpea in Benin and control strategies for ecologically sustainable cowpea production. / Thesis (DPhil (Microbiology and Plant Pathology))--University of Pretoria, 2006. / Microbiology and Plant Pathology / unrestricted

Cowpea

Damping-off and stem rot

Trichoderma

sclerotium rolfsii

Screening

Polyphenols

Moringa oleifera

Its rdna

Integrated control

Genetic diversity

Biocontrol

UCTD

Filogenia de Porphyra spp. (Rhodophyta): sequenciamento do gene nuclear para o RNA da subunidade pequena do ribossomo (rDNA 18S) e estudos morfológicos da fase Conchocelis / Phylogene of Porphyra spp (Rhodophyta): sequencing of the nuclear gene coding for the RNA from the small subunity of the ribosome (18S rDNA) and morphological studies of the Conchocelis phase

Mariana Cabral de Oliveira

15 December 1993

O gênero Porphyra (Rhodophyta) apresenta uma considerável importância econômica, sendo extensivamente cultivado e consumido como alimento. O gênero é representado por mais de 70 espécies e apresenta ampla distribuição geográfica, desde regiões tropicais até polares. Sua taxonomia, baseada em poucos caracteres da fase macroscópica do seu ciclo de vida, é ainda bastante problemática. Para tentar entender melhor a taxonomia e a história evolutiva de Porphyra foram utilizadas metodologias de biologia molecular e características da fase conchocelis do ciclo de vida. Verificou-se que caracteres da fase microscópica podem ser utilizados para complementar os conhecimentos taxonômicos tradicionais. Para tentar elucidar a posição filogenética do gênero Porphyra na divisão Rhodophyta e, dentro do gênero, entre espécies do Atlântico, o gene nuclear que codifica para o RNA ribossomal da subunidade pequena do ribossomo (rDNA 18S) foi amplificado através de PCR, clonado e completamente sequenciado. Foram utilizadas três espécies de Porphyra da Nova Escócia (Canadá) e duas de São Paulo (Brasil). As sequências obtidas foram alinhadas com as de alguns eucariontes e de outras algas vermelhas, incluindo uma sequência publicada de \"Porphyra umbilicalis\" da França. As árvores filogenéticas foram construídas através dos métodos de parcimônia, distancia e máxima verossimilhança. As analises mostraram que o gênero Porphyra é monofilético para as cinco espécies estudadas e constitui um dos ramos mais antigos dentro das algas vermelhas já analisados. O gênero Porphyra, subclasse Bangiophycidae, apresentou uma diferença substancial em relação aos gêneros da subclasse Florrideophycidae, sustentando assim, a divisão de Rhodophyta em duas subclasses pela taxonomia tradicional. Entre os eucariontes, Porphyra divergiu ao mesmo tempo que o nuclemorfo de Cryptomonas. O alto grau de divergência genética encontrada entre espécies de Porphyra, além de indicações do registo fóssil, na literatura, sugerem que o gênero é bastante primitivo dentro das algas vermelhas. Surpreendentemente, a sequência publicada para \"Porphyra umbilicalis\" apresentou mais de 99% de identidade com uma espécie de Palmaria que pertence à subclasse Florideophycidae; neste caso, a biologia molecular serviu para comprovar a identificação errônea do exemplar cuja sequência foi publicada. Durante a análise filogenética, verificou-se a ocorrência de um intron do grupo ICI nos genes rDNA 18S de Porphyra spiralis var. amplifolia. Esse intron ocorre na mesma posição que os introns do grupo IC1 nos rDNA 18S dos fungos Pneumocystis carinii, Protomyces inouyei e da alga verde Chlorella ellipsoidea, e apresenta identidade de sequências nos domínios P1 e P2, fora da região conservada, com o intron de Pn. Carinii. Três variantes, diferindo do tamanho da seqüencia do domínio P1, foram observados em três populações com distribuição geográfica diferente. O variante maior pode se auto-processar (\"self-splice\") in vitro. Quadros abertos de leitura estão presentes nos introns, mas não correspondem a nenhum gene conhecido. Introns estão presentes no rDNA 18S de outras espécies de Porphyra, que também podem apresentar variantes do rDNA 18S sem introns / The red algas genus Porphyra has considerable economic importance, and some species are extensively cultivated for human food. The genus is represented by more than 70 species, and occurs worldwide. Its taxonomy, based mainly on morphological characters of the macroscopic phase of its life-cycle is still unsettled. Alternatives to try to understand better the taxonomy and evolutive history of the genus were ascertained. It was verified that characters of the microscopic, filamentous phase, of the life-cycle of Porphyra may be used to complement the traditional taxonomic studies. To try to elucidate the phylogenetic position of Porphyra relative to the other red algae, and within the genus, among isolates from different locations, nuclear-encoded small-subunit ribosomal RNA genes (18S rDNAs) were PCR-amplified, cloned and completely sequenced. Three species of Porphyra from Nova Scotia and two species from Brasil were aligned with 18S sequences of other eukaryotes, including one published sequence of \"Porphyra umbilicalis\" from France. Phylogenetic trees were constructed by parsimony, distance and maximum-likelihood procedures. Analysis of our data revealed that these Porphyra species represented one of the deepest branches so far discovered within red algae. There was a great degree of primary sequence difference between Porphyra (subclass Bangiophycidae), and the other red algae belonging to the subclasses Florideophycidae. These results support the division of red algae into two subclasses by traditional taxonomy. Among eukaryotes Porphyra diverges at the same point as the Cryptomonas nucleomorph. The great among of sequence divergence, and the fossil record suggest that Porphyra, my indeed, be a very primitive red alga. Surprisingly, the 18S RNA sequence of the French \"Porphyra umbilicalis\" does not fit in our Porphyra category; instead, it has more than 99% identity with a species of Palmaria belonging to the subclass Florideophycidae. Therefore it was concluded that \"P. umbilicalis\" with the published sequence was actually a Palmaria palmate that was misidentified. During the phylogenetic analysis it was found that a group IC1 intron occurs in nuclear 18S rRNA genes of Porphyra spiralis var. amplifolia. This intron occurs at the same position of the group IC1 introns in 18S rDNAs of the fungus Pneumocystis carinii, Protomyces inouyei and the green alga Chlorella ellipsoidea, and shares primary-structural identity with the Pn. Carinii intron in domains P1 and P2, outside the conserved core. Three size-variants, differing in amount of optimal sequence in P1, exist and are differentially distributed in geographically distinct populations. The largest variant can self-splice in vitro. Open reading frames are present, but do correspond to known genes. Introns are present in the 18S rDNAs of several other Porphyra species, that may also have intronless rDNA copies

Algas vermelhas

Bangiales

Conchocelis

Filogenia molecular

Porphyra

Pyropia

SSUrDNA

Bangiales

Conchocelis

Molecular phylogeny

Porphyra

Pyropia

Red seaweed

SSU rDNA