Avaliação de fungos entomopatogênicos visando ao controle da ampola da erva-mate Gyropsylla spegazziniana (Lizer & Trelles) (Hemiptera: Psyllidae) / Activity and characterization of entomopathogenic fungi against paraguay tea ampul (gyropsylla spegazziniana) (lizer & trelles) (hemiptera: psyllidae)

Formentini, Marina Andressa

20 September 2012

Made available in DSpace on 2017-07-10T14:38:34Z (GMT). No. of bitstreams: 1 Marina.pdf: 1184727 bytes, checksum: 464327ef9797c59ec694ee14413ca72c (MD5) Previous issue date: 2012-09-20 / Coordenação de Aperfeiçoamento de Pessoal de Nível Superior / This study aimed to select and characterize strains of entomopathogenic fungi in order to control Gyropsylla spegazziniana. For this, the fifth instar nymphs were transferred to Paraguay tea seedlings, followed by spraying conidial suspensions of 48 strains of Beauveria spp., Metarhizium anisopliae, Isaria spp. and Lecanicillium spp. at a concentration of 1 × 109 conidia/mL. The seedlings were placed in PVC cages kept in a climatized room (26 ± 1°C; 12 h photophase and 60 ± 10% R.H.), and the insect mortality was evaluated daily for 10 days. The most active isolates were compared by means of vegetative growth, conidial production in culture media, insecticidal activity and molecular analyses, by sequencing the region rDNA-ITS and RAPD. The genus 22 Beauveria spp. was more efficient among the entomopathogenic fungi, especially for strain Unioeste 44 that showed the best performance, demonstrating its potential to control the pest. Molecular analysis of rDNA-ITS region allowed the identification of isolates as B. bassiana e B. brongniartii and RAPD markes were associated with virulence / O objetivo desse trabalho foi selecionar e caracterizar isolados de fungos entomopatogênicos, visando o controle dessa praga. Para tal, ninfas de 5o ínstar foram transferidas para mudas de erva-mate, seguido da pulverização de suspensões de conídios (1 × 109 conídios/mL) de 48 isolados de Beauveria spp., Metarhizium anisopliae, Isaria spp. e Lecanicillium spp. As mudas foram acondicionadas em gaiolas de PVC, e mantidas em sala climatizada (26 ± 1°C; 12 h de fotofase e U.R. 60 ± 10%). 21 A mortalidade dos insetos foi avaliada diariamente, por 10 dias e os isolados mais ativos foram comparados entre si por meio do crescimento vegetativo, produção de conídios em meios de cultura, atividade inseticida e análises moleculares, por meio do seqüenciamento da região rDNA-ITS e marcadores RAPD. O gênero Beauveria spp. foi mais eficiente dentre os fungos entomopatogênicos, em especial o isolado Unioeste 44 que apresentou o melhor desempenho, evidenciando seu potencial para o controle da praga. As análises moleculares da região rDNA-ITS possibilitou a identificação dos isolados como B. bassiana e B. brongniartii e os marcadores RAPD foram associados à virulência

controle biológico

Beauveria

Ilex paraguariensis

rDNA-ITS

biological control

Beauveria

Ilex paraguariensis

rDNA-ITS

Genotyp-Identifizierung und Wechselwirkungen an zwei Populus-Chimären

Hansen, Mario Jens

16 September 2005

Zwei Populus-Pfropfchimären (MA und AI), die aus P. x canadensis ‘Marilandica’ (M), P. maximowizcii x P. trichocarpa ‘Androscoggin’ (A) and P. nigra L. ’Italica’ (I) aufgebaut sind, wurden für Untersuchungen zur Laub- und Blütenblattentwicklung genutzt. In MA bildet M die äußere Lage (L1) und ihr Derivat, die Epidermis, während die inneren Lagen (L2, L3 etc.) von A gebildet werden. Bei AI stammt die L1 von A und L2, L3 etc. werden von I gebildet. Die genotypisch andersartige Epidermis bedingt bei Periklinal-Chimären morphologische Effekte wie zum Beispiel einen Fruchtknoten in einigen MA-Blüten. Morphologische Besonderheiten verschiedener Gewebe sowohl von M und A als auch von MA wurden verglichen, um festzustellen, wie sie durch die Gewebetransplantation verändert oder beeinflusst wurden und, um mögliche Genotyp- Interaktionen oder -Wechselwirkungen in einem Gewebe ausfindig zu machen. Für die Genotypidentifizierung in verschiedenen Organen wurde die RAPD-PCR getestet. Einer von 20 getesteten 10mer Zufallsprimern (GGAGTGGACA) ermöglichte bei der Verwendung von DNA aus Blattmaterial die Erzeugung verschiedener Bandenmuster für M und A. Bei der Verwendung von MA-Blattmaterial zeigte sich eine Kombination der Muster von M und A, sodass ein Chimärennachweis für das MA-Blattmaterial erbracht wurde. Für ein übertragbares System wurde die spezifische PCR getestet. Unter Verwendung spezifischer Primer für die 16s-rDNA zeigten die PCR-Produkte einheitliche Banden und nach anschließender Sequenzierung eine weitgehende Übereinstimmung der phylogenetischen Verwandtschaft von I, M und A. Weiterhin wurden die kernkodierten rDNA Bereiche ITS 1 und ITS 2 zwischen 18S und 25S getestet. Für I, M und A konnten jeweils zwei Banden von unterschiedlicher Größe und Sequenz ermittelt werden, die vermutlich auf funktionierende rDNA aber auch auf Pseudogene (beschnitten) in niedriger Kopienzahl hinweisen. Die ITS-Regionen von I, M und A wurden charakterisiert, um einen Einblick in die Struktur und Phylogenie der Salicacaee-Familie zu erhalten. Aus den Sequenzunterschieden konnten für I und A spezifische Primerpaare abgeleitet werden, die für die Identifizierung von I und A in AI und MA verwendet werden können. Mittels A-Marker konnte nachgewiesen werden, dass Fruchtknoten aus MA-Blüten neben M-Gewebe auch den A-Genotyp enthalten. / Two Populus graft chimeras (MA and AI) produced of P. x canadensis ‘Marilandica’ (M), P. maximowizcii x P. trichocarpa ‘Androscoggin’ (A) and P. nigra L. ’Italica’ (I) were used for investigations of leaf and flower development. In MA the exogenous layer (L1) forms the epidermis and is derived from M while inner layers (L2, L3 etc.) descend from A whereas in AI L1 is formed by A while L2, L3 etc. descend from I. The exogenous epidermis of the periclinal chimeras imposes morphological effects such as an extra female sex in some of the MA flowers. The morphological characteristics of different plant tissues of parents and chimera were compared to determine how they were modified or altered by the tissue transplantation and possibly identify co-existing or interacting genotypes in one tissue. RAPD-PCR was tested for its usefulness to amplify polymorphic fingerprints including donor specific DNA fragments. One random 10mer primer (GGAGTGGACA) out of 20 tested revealed the amplification of patterns including donor specific DNA bands using extracts from leaf tissues of the M and A parents that were combined using extract from leaf tissue of the MA chimera. This indicates that the leaves of the MA chimera are formed by tissues of M and A. However, the inherent disadvantage of RAPD-PCR is the reproducibility of PCR product generation. Therefore the discriminative potential of the ITS region located between the rRNA genes was investigated. The application of specific 16S ribosomal DNA (rDNA) primers for amplification and sequencing of PCR products revealed a closely phylogenetic relationship between I, M and A. Consequently the ITS1 and ITS2 of nuclear rDNA between 18S and 25S were used. The amplified fragments were purified, cloned in E. coli and sequenced. Analyses of multiple clones demonstrated extensive paralogy within and between I, M and A ITS operons. For each parent were at least two rDNA operons as well as multiple paralogous sequences within operons identified. The use of PCR and sequence analyses showed that one of the operons encodes a putative expressed (functional) rDNA whereas the second encodes a pseudogen (truncated) in low copy number. We also characterized the ITS regions of I, M and A to gain insights into structure and phylogeny of the Salicacaee family. Based on sequence divergence primers were designed for A and I and used for the identification of A in MA carpels.

Populus-Pfropfchimären

RAPD-PCR

16s-rDNA

kernkodierte rDNA (ITS-Regionen)

Populus graft chimeras

RAPD-PCR

16s-rDNA

nuclear rDNA (ITS regions)

630 Landwirtschaft, Veterinärmedizin

39 Landwirtschaft, Garten

ddc:630

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

Spread of the fascioliasis endemic area assessed by seasonal follow-up of rDNA ITS-2 sequenced lymnaeid populations in Cajamarca, Peru

Bardales-Valdivia, J. N., Bargues, M. D., Hoban-Vergara, C., Bardales-Bardales, C., Goicochea-Portal, C., Bazán-Zurita, H., Del Valle-Mendoza, J., Ortiz, P., Mas-Coma, S.

01 December 2021

Fascioliasis is a worldwide emerging snail-borne zoonotic trematodiasis with a great spreading capacity linked to animal and human movements, climate change, and anthropogenic modifications of freshwater environments. South America is the continent with more human endemic areas caused by Fasciola hepatica, mainly in high altitude areas of Andean regions. The Peruvian Cajamarca area presents the highest human prevalences reported, only lower than those in the Bolivian Altiplano. Sequencing of the complete rDNA ITS-2 allowed for the specific and haplotype classification of lymnaeid snails collected in seasonal field surveys along a transect including 2007–3473 m altitudes. The species Galba truncatula (one haplotype preferentially in higher altitudes) and Pseudosuccinea columella (one haplotype in an isolated population), and the non-transmitting species Lymnaea schirazensis (two haplotypes mainly in lower altitudes) were found. Climatic seasonality proved to influence G. truncatula populations in temporarily dried habitats, whereas L. schirazensis appeared to be more climatologically independent due to its extreme amphibious ecology. Along the southeastern transect from Cajamarca city, G. truncatula and L. schirazensis shared the same site in 7 localities (46.7% of the water collections studied). The detection of G. truncatula in 11 new foci (73.3%), predominantly in northern localities closer to the city, demonstrate that the Cajamarca transmission risk area is markedly wider than previously considered. Lymnaea schirazensis progressively increases its presence when moving away from the city. Results highlight the usefulness of lymnaeid surveys to assess borders of the endemic area and inner distribution of transmission foci. Similar lymnaeid surveys are still in need to be performed in the wide northern and western zones of the Cajamarca city. The coexistence of more than one lymnaeid transmitting species, together with a morphologically indistinguishable non-transmitting species and livestock movements inside the area, conform a complex scenario which poses difficulties for the needed One Health control intervention. / Ministerio de Economía y Competitividad / Revisión por pares

Cajamarca hyperendemic area

Galba truncatula

Human and animal fascioliasis

Lymnaea schirazensis

Peru

Pseudosuccinea columella

rDNA ITS-2 sequencing

Accurate identification and grouping of Rhizoctonia isolates infecting turfgrasses in MD and VA and their sensitivity to selected fungicides in vitro

Amaradasa, Bimal Sajeewa

08 September 2011

Rhizoctonia blight (sensu lato) is a common and serious disease of many turfgrass species. The most widespread causal agent R. solani consists of several genetically different anastomosis groups (AGs) and subgroups. Though anastomosis or hyphal fusion reactions have been used to group Rhizoctonia species, they are time consuming and sometimes difficult to interpret. Anastomosis reactions are incapable of identifying isolates belonging to different AG subgroups within an AG. This study evaluated molecular techniques in comparison with traditional anastomosis grouping (AG) to identify and group isolates of Rhizoctonia. More than 400 Rhizoctonia isolates were collected from diseased turfgrass leaves from eight geographic areas in Virginia and Maryland. A random sample of 86 isolates was selected and initially characterized by colony morphology, nuclei staining and anastomosis grouping. Molecular identification was performed by analysis of rDNA-ITS region and DNA fingerprinting techniques universally primed PCR (UP-PCR) and amplified fragment length polymorphism (AFLP). The cladistic analysis of ITS sequences and UP-PCR fragments supported seven clusters. Isolates of R. solani AG 1-IB (n=18), AG 2-2IIIB (n=30) and AG 5 (n=1) clustered separately. Waitea circinata var. zeae (n=11), and var. circinata (n=4) grouped separately. A cluster of six isolates (UWC) did not fall into any known Waitea group. Most of the binucleate Rhizoctonia-like fungi (BNR) (n=16) grouped separately. AFLP grouping also largely agreed with the above results. However, UWC isolates clustered into two groups. Molecular analyses corresponded well with traditional anastomosis grouping by clustering isolates within an AG or AG subgroup together. UP-PCR cross-hybridization could distinguish closely related Rhizoctonia isolates to their infraspecies level. Genetically related isolates belonging to the same AG subgroups cross-hybridized strongly, while isolates of different AGs did not cross-hybridize or did so weakly. Sequence-characterized amplified region (SCAR) markers were generated from UP-PCR products to identify isolates of major pathogenic groups AG 1-IB and AG 2-2IIIB. Specific primer pairs successfully distinguished isolates of AG 1-IB and AG 2-2IIIB from isolates of other AGs. Sensitivity of Rhizoctonia species and AGs was tested in vitro to commercial formulations of iprodione, triticonazole and pyraclostrobin. W. circinata isolates were moderately sensitive to iprodione while isolates of R. solani and BNR were extremely sensitive. Isolates of AG 2-2IIIB showed less sensitivity to triticonazole than other Rhizoctonia isolates. W. circinata var. zeae isolates were moderately sensitive to pyraclostrobin while most of the other isolates were extremely sensitive. / Ph. D.

EC50

fungicide sensitivity

SCAR markers

cross-hybridization

AFLP

UP-PCR

rDNA-ITS

anastomosis

Waitea circinata

Rhizoctonia solani

brown patch

Diverzitet makrogljiva i njihova uloga u monitoringu stanja šumskih ekosistema Srbije / Diversity of macrofungi and their role in the monitoring of forest ecosystems in Serbia

Rakić Milana

28 September 2019

<p>U&nbsp; okviru&nbsp; ove&nbsp; doktorske&nbsp; disertacije&nbsp; vr&scaron;eno&nbsp; je istraživanje&nbsp; zajednica&nbsp; makrogljiva&nbsp; u&nbsp; okviru&nbsp; 5 &scaron;umskih&nbsp; stani&scaron;ta&nbsp; na&nbsp; Vidliču,&nbsp; Kopaoniku&nbsp; i&nbsp; Tari. Ispitivan&nbsp; je&nbsp; mikodiverzitet&nbsp; sa&nbsp; morfolo&scaron;kog, funkcionalnog i genetskog stanovi&scaron;ta. U istraživanju morolo&scaron;kog&nbsp; i&nbsp; funkcionalnog&nbsp; diverziteta,&nbsp; kori&scaron;ćene su&nbsp; različite&nbsp; klasične&nbsp; metode&nbsp; čiji&nbsp; rezultati&nbsp; su<br />omogućili procenu stanja posmatranih mikocenoza, kao&nbsp; i&nbsp; samih&nbsp; &scaron;umskih&nbsp; stani&scaron;ta.&nbsp; Za&nbsp; analizu&nbsp; sastava vrsta&nbsp; u&nbsp; okviru&nbsp; mikocenoza,&nbsp; kao&nbsp; i&nbsp; procenu&nbsp; uticaja abiotičkih faktora na brojnost i sastav vrsta u okviru različitih funkcionalnih grupa, kori&scaron;ćeno je nekoliko<br />statističkih&nbsp; metoda&nbsp; (PCA,&nbsp; PLS,&nbsp; CA&nbsp; i&nbsp; CCA).&nbsp; Osam vrsta,&nbsp; koje&nbsp; su&nbsp; pripadale&nbsp; najrasprostranjenijim&nbsp; i najzastupljenijim&nbsp; vrstama&nbsp; su&nbsp; odabrane&nbsp; za molekularne&nbsp; analize,&nbsp; koje&nbsp; su&nbsp; podrazumevale sekvenciranje&nbsp; ITS&nbsp; regiona&nbsp; rDNK,&nbsp; analizu&nbsp; njihovih<br />polimorfizama&nbsp; kao&nbsp; i&nbsp; filogenetske&nbsp; analize&nbsp; u&nbsp; okviru vrste/roda.&nbsp; U&nbsp; cilju&nbsp; procene&nbsp; zagađenja&nbsp; stani&scaron;ta,&nbsp; u plodnim telima makrogljiva i njihovom supstratu je određen&nbsp; sadržaj&nbsp; metala&nbsp; (atomskom&nbsp; apsorpcionom spektrofotometrijom)&nbsp; i&nbsp; radionuklida<br />(gamaspektrometrijom).&nbsp; Dobijeni&nbsp; rezultati&nbsp; ukazuju na&nbsp; to&nbsp; da&nbsp; diverzitet&nbsp; makrogljiva&nbsp; oslikava&nbsp; stanje samog&nbsp; stani&scaron;ta&nbsp; i&nbsp; da&nbsp; dugoročnim&nbsp; monitoringom mogu ukazati na promene u njemu.</p> / <p>Within the framework of this doctoral dissertation, monitoring&nbsp; of&nbsp; macrofungal&nbsp; communities,&nbsp; within&nbsp; 5 forest habitats on&nbsp; Vidlič, Kopaonik and Tara, was done. &nbsp; Mycodiversity&nbsp; was&nbsp; investigated&nbsp; from&nbsp; the morphological,&nbsp; functional&nbsp; and&nbsp; genetic&nbsp; point&nbsp; of view. Various classical methods&nbsp; used,&nbsp; enabled the assessment&nbsp; of&nbsp; the&nbsp; condition&nbsp; of&nbsp; macrofungal communities,&nbsp; as&nbsp; well&nbsp; as&nbsp; the&nbsp; observed&nbsp; forest habitats. &nbsp; Several&nbsp; statistical&nbsp; methods&nbsp; (PCA,&nbsp; PLS, CA&nbsp; and&nbsp; CCA)&nbsp; were&nbsp; used&nbsp; to&nbsp; analyze&nbsp; the composition of&nbsp; species within the&nbsp; mycocenosis, as well&nbsp; as&nbsp; the&nbsp; assessment&nbsp; of&nbsp; the&nbsp; effects&nbsp; of&nbsp; abiotic factors&nbsp; on&nbsp; the&nbsp; species&nbsp; richness&nbsp; and&nbsp; species composition&nbsp; within&nbsp; different&nbsp; functional&nbsp; groups.Some&nbsp; of&nbsp; the&nbsp; most&nbsp; represented&nbsp; species&nbsp; have&nbsp; been selected&nbsp; for&nbsp; molecular&nbsp; analyzes,&nbsp; which&nbsp; includedsequencing&nbsp; of&nbsp; the&nbsp; ITS&nbsp; region,&nbsp; the&nbsp; analysis&nbsp; of polymorphisms,&nbsp; as&nbsp; well&nbsp; as&nbsp; phylogenetic&nbsp; analyzes within&nbsp; the&nbsp; species/genus.&nbsp; In&nbsp; order&nbsp; to&nbsp; assess&nbsp; the pollution of habitats, the content of metals (atomic absorption&nbsp; spectrophotometry)&nbsp; and&nbsp; radionuclides (gamma&nbsp; spectrometry)&nbsp; was&nbsp; determined&nbsp; in&nbsp; the sporocarps&nbsp; of&nbsp;&nbsp; macrofungi&nbsp; and&nbsp; their&nbsp; substrate.&nbsp; The obtained&nbsp; results&nbsp; indicate&nbsp; that&nbsp; diversity&nbsp; of macrofungi&nbsp; reflects&nbsp; the&nbsp; state&nbsp; of&nbsp; the&nbsp; habitat&nbsp; itself and that long-term monitoring can indicate changes in it.</p>