Teses / dissertações sobre o tema "Nematode diseases of plants Genetic aspects"
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Williams, Kevin John. "Biological and genetic studies of wheat resistance to Heterodera avenae". Title page, summary and contents only, 1994. http://web4.library.adelaide.edu.au/theses/09PH/09phw7238.pdf.
Texto completo da fonteTaylor, Sharyn Patricia. "The root lesion nematode, Pratylenchus neglectus, in field crops in South Australia". Title page, contents and summary only, 2000. http://web4.library.adelaide.edu.au/theses/09PH/09pht2462.pdf.
Texto completo da fonteVanstone, Vivien Alison. "The role of fungi and the root lesion nematode, Pratylenchus neglectus, in damaging wheat roots in South Australia". Title page, summary and contents only, 1991. http://web4.library.adelaide.edu.au/theses/09PH/09phv281.pdf.
Texto completo da fonteShrestha, Roshi. "A physiological and genetic mapping study of tolerance to root-knot nematode in rice". Thesis, Available from the University of Aberdeen Library and Historic Collections Digital Resources, 2008. http://digitool.abdn.ac.uk:80/webclient/DeliveryManager?application=DIGITOOL-3&owner=resourcediscovery&custom_att_2=simple_viewer&pid=24807.
Texto completo da fonteMaree, H. J. (Hans Jacob). "The expression of Dianthin 30, a ribosome inactivating protein". Thesis, Stellenbosch : Stellenbosch University, 2003. http://hdl.handle.net/10019.1/53633.
Texto completo da fonteENGLISH ABSTRACT: Ribosome inactivating proteins (RIPs) are currently classified as rRNA N-glycosidases, but also have polynucleotide: adenosine glycosidase activity. RIPs are believed to have anti-viral and anti-fungal properties, but the exact mechanism of these proteins still need to be elucidated.The mechanism of resistance however, appears to be independent of the pathogen. For resistance the RIP terminates virus infected plant cells and stops the reproduction and spread of the virus. Transgenic plants containing RIPs should thus be resistant to a wide range of viruses. The ultimate goal of the larger project of which this forms part is the development of virus resistant plants. To monitor the expression of a RIP in a transgenic plant a detection method had to be developed. Antibody detection of the RIP was decided upon as the most cost effective method. The RIP, Dianthin 30 from Dianthus caryophyllus (carnation), was used and expressed in bacterial and insect expression systems. The bacterial expression experiments were done using the pET expression system in BL21(DE3)pLysS cells. The expression in this system yielded recombinant protein at a very low concentration. Expression experiments were also performed in insect tissue culture with the baculovirus vector BAC-TO-BAC™.With this system the expression was also too low to be used for the production of antibodies. A Dianthin 30 specific peptide was then designed and then produced by Bio-Synthesis. This peptide was then used to raise antibodies to detect Dianthin 30. These antibodies were tested on Dianthus caryophyllus proteins. To establish if this detection method was effective to monitor the expression in plants, tobacco plants were transformed with Agrobacterium tumefaciens containing Dianthin 30 in the pART27 plant expression vector. The putative transformed plants were analysed with peR and Southern blots.
AFRIKAANSE OPSOMMING: Tans word Ribosomale-inaktiverende proteïene (RIPs) geklassifiseer as rRNA N-glikosidase wat ook polinukleotied: adenosien glikosidase aktiwiteit bevat. Daar word geglo dat RIPs anti-virale en anti-fungus eienskappe bevat, maar die meganisme van beskerming word nog nie ten volle verstaan nie. Dit is wel bewys dat die meganisme van weerstand onafhanklik is van die patogeen. Virus geinfekteerde plantselle word deur die RIP gedood om die voortplanting en verspreiding te bekamp en sodoende word weerstand bewerkstellig. Transgeniese plante wat dan 'n RIP bevat sal dus weerstandbiedend wees teen 'n wye spektrum virusse. Die hoofdoel van die breër projek, waarvan die projek deel uitmaak: is die ontwikkeling van virusbestande plante. Om die uitdrukking van die RIP in die transgeniese plante te kontroleer, moes 'n deteksie metode ontwikkel word. Die mees koste effektiewe deteksie metode is met teenliggame. Die RIP, Dianthin 30 from Dianthus caryophyllus (angelier) was gebruik vir uitdrukking in bakteriele- en insekweefselkultuur. Die bakteriele uitdrukkingseksperimente was gedoen met die pET uitdrukkings sisteem III BL21(DE3)pLysS selle. Die uitdrukking in die sisteem het slegs rekombinante proteïene gelewer in uiters lae konsentrasies. Uitdrukkingseksperimente was ook gedoen in insekweefselkultuur met die baculovirus vektor BAC-To- BACTM. Met die sisteem was die uitdrukking ook veels te laag om bruikbaar te wees vir die produksie van teenliggame. Daar is toe 'n peptied ontwerp wat Dianthin 30 kan verteenwoordig vir die produksie van teenliggame. Die teenliggame is getoets teen Dianthus caryophyllus proteïene. Om vas te stel of die deteksiemetode wel die uitdrukking van Dianthin 30 sal kan monitor, is tabak ook getransformeer met Dianthin 30. Die transformasies is gedoen met die hulp van Agrobacterium tumefaciens en die pART27 plant uitdrukkings vektor. Die plante is getoets met die polimerase ketting reaksie en Southern klad tegnieke.
Filkowski, Jody, e University of Lethbridge Faculty of Arts and Science. "The effect of pathogens on plant genome stability". Thesis, Lethbridge, Alta. : University of Lethbridge, Dept. of Biological Sciences, 2004, 2004. http://hdl.handle.net/10133/254.
Texto completo da fontexiii, 119 leaves ; 29 cm.
Van, Eeden C. (Christiaan). "The construction of gene silencing transformation vectors for the introduction of multiple-virus resistance in grapevines". Thesis, Stellenbosch : Stellenbosch University, 2004. http://hdl.handle.net/10019.1/53764.
Texto completo da fonteENGLISH ABSTRACT: Viruses are some of the most important pathogens of grapevines. There are no effective chemical treatments, and no grapevine- or other natural resistance genes have been discovered against grapevine infecting viruses. The primary method of grapevine virus control is prevention by biological indexing and molecular- and serological screening of rootstocks and scions before propagation. Due to the spread of grapevine viruses through insect vectors, and in the case of GRSPaV the absence of serological screening, these methods of virus control are not always effective. In the past several methods, from cross-protection to pathogen derived resistance (PDR), have been applied to induce plant virus resistance, but with inconsistent results. In recent years the application of post-transcriptional gene silencing (PTGS), a naturally occurring plant defense mechanism, to induce targeted virus resistance has achieved great success. The Waterhouse research group has designed plant transformation vectors that facilitate specific virus resistance through PTGS. The primary focus of this study was the production of virus specific transformation vectors for the introduction of grapevine virus resistance. The Waterhouse system has been successfully utilised for the construction of three transformation vectors with the pHannibal vector as backbone. Each vector contains homologous virus coat protein (CP) gene segments, cloned in a complementary conformation upstream and downstream of an intron sequence. The primary vector (pHann-SAScon) contains complementary CP gene segments of both GRSPaV and GLRaV-3 and was designed for the introduction of multiple-virus resistance. For the construction of the primary vector the GRSPaV CP gene was isolated from RSP infected grapevines. A clone of the GLRaV-3 CP gene was acquired. The second vector (pHann- LR3CPsas) contains complementary CP gene segments of GLRaV-3. The third vector (pHann-LR2CPsas) contains complementary CP gene segments of GLRaV-2. The cassette containing the complementary CP gene segments of both GRSPaV and GLRaV-3 was cloned into pART27 (pART27-HSAScon), and used to transform N tabacum cv. Petit Havana (SRI), through A. tumefaciens mediated transformation. Unfortunately potential transformants failed to regenerate on rooting media; hence no molecular tests were performed to confirm transformation. Once successful transformants are generated, infection with a recombinant virus vector (consisting of PYX, the GFP gene as screenable marker and the complementary CP gene segments of both GRSPaV and GLRaV-3) will be used to test for the efficacy of the vectors to induce resistance. A secondary aim was added to this project when a need was identified within the South African viticulture industry for GRSPaV specific antibodies to be used in serological screening. To facilitate future serological detection of GRSPaV, the CP gene was isolated and expressed with a bacterial expression system (pETI4b) within the E. coli BL2I(DE3)pLysS cell line. The expressed protein will be used to generate GRSPaV CP specific antibodies.
AFRIKAANSE OPSOMMING: Virusse is van die belangrikste patogene by wingerd. Daar bestaan geen effektiewe chemiese beheer nie, en geen wingerd- of ander natuurlike weerstandsgene teen wingerdvirusse is al ontdek nie. Die primêre metode van beheer t.o.v. wingerdvirusse is voorkoming deur biologiese indeksering, en molekulêre- en serologiese toetsing van onderstokke en entlote voor verspreiding. As gevolg van die verspreiding van wingerdvirusse deur insekvektore, en in die geval van GRSPa V die tekort aan serologiese toetsing, is dié metodes van virusbeheer nie altyd effektief nie. In die verlede is metodes soos kruis-beskerming en patogeen-afgeleide weerstand (PDR) gebruik om virusweerstand te induseer, maar met inkonsekwente resultate. In onlangse jare is post-transkripsionele geenonderdrukking (PTGS), 'n natuurlike plantbeskermingsmeganisme, met groot sukses toegepas om geteikende virusweerstand te induseer. Die Waterhouse-navorsingsgroep het planttransformasievektore ontwerp wat spesifieke virusweerstand induseer d.m.v. PTGS. Die vervaardiging van virus spesifieke tranformasievektore vir die indusering van wingerdvirusweerstand was die primêre doelwit van hierdie studie. Die Waterhouse-sisteem was gebruik vir die konstruksie van drie transformasievektore, met die pHannibal vektor as basis. Elke vektor bevat homoloë virus kapsiedproteïen (CP) geensegmente, gekloneer in 'n komplementêre vorm stroom-op en stroom-af van 'n intronvolgorde. Die primêre vektor (pHann-SAScon) bevat komplementêre CP geensegmente van beide GRSPaV en GLRaV-3, en was ontwerp vir die indusering van veelvoudige-virusweerstand. Die CP-geen van GRSPa V was vanuit RSP-geïnfekteerde wingerd geïsoleer, vir die konstruksie van die primêre vektor. 'n Kloon van die GLRa V-3 CP-geen was verkry. Die tweede vektor (pHann-LR3CPsas) bevat komplementêre CP geensegmente van GLRaV-3. Die derde vektor (pHann-LR2CPsas) bevat komplementêre CP geensegmente van GLRa V-2. Die kasset bestaande uit die komplementêre CP geensegmente van beide GRSPaV en GLRaV-3, was gekloneer in pART27 (pART27-HSAScon), en gebruik om N tabacum cv. Petit Havana (SRI) te transformeer d.m.v. A. tumefaciens bemiddelde transformasie. Ongelukkig het potensiële transformante nie geregenereer op bewortelingsmedia nie; gevolglik was geen molekulêre toetse gedoen om transformasie te bevestig nie. Na suksesvolle transformante gegenereer is, sal infeksie met 'n rekombinante-virusvektor (bestaande uit PYX, die GFP geen as waarneembare merker en die komplementêre CP geensegmente van beide GRSPa V en GLRa V-3) gebruik word om die effektiwiteit van die vektore as weerstandsinduseerders te toets. 'n Sekondêre doelwit is by die projek gevoeg toe 'n behoefte aan GRSPaV spesifieke teenliggame binne die Suid-Afrikaanse wynbedryf geïdentifiseer is, vir gebruik in serologiese toetsing. Om toekomstige serologiese toetsing van GRSPa V te bemiddel, was die CP-geen geïsoleer en in 'n bakteriële uitdrukkingsisteem (PETI4b) uitgedruk, in die E. coli BL21(DE3)pLysS sellyn. Die uitgedrukte proteïne sal gebruik word vir die vervaardiging van GRSPa V CP spesifieke antiliggame.
Ntushelo, Khayalethu. "Comparative studies on genetic variability and fungicide resistance in Tapesia yallundae". Thesis, Stellenbosch : Stellenbosch University, 1998. http://hdl.handle.net/10019.1/55834.
Texto completo da fonteENGLISH ABSTRACT: Eyespot is an important disease of spring wheat (Triticum aestivum L.). Four species of Ramulispora are associated with this disease, of which Tapesia yallundae and T. acuformis. are common. This thesis investigates the broader subjects of genetic variability, reproductive dynamics and fungicide resistance in Tapesia yallundae. Each of the chapters treats specific but related topics. T. yallundae, which is the only species thus far reported from South Africa, has been associated with yield losses of up to 50%. To enable the implementation of more accurate and effective control measures, understanding the dynamics of reproduction and the genetics of the pathogen is of utmost importance. Of the many plant disease control measures such as cultural practices, sanitation, biological control, etc., fungicide application is the most commonly resorted to measure in eyespot control. This thesis investigates the broader subjects of genetic variability, reproductive dynamics and fungicide resistance of Tapesia yallzll7dae. Fungicide application, however, is not without problems. The pathogen can build up resistance to fungicides. The most commonly used fungicides in eyespot control include the benzimidazole carbendazim, triazoles such as flusilazole, tebuconazole, propiconazole, bromuconazole, flutriafol, fenbuconazole, triademinol, and the imidazole, prochloraz. Cases of resistance to the groups listed above have been reported. Frequent monitoring for resistance is thus crucial to prevent wastage of fungicide and unnecessary impregnantation of the environment with potentially ineffective chemicals. In chapter 2 of this thesis 300 isolates of T. yallundae from 15 fields were evaluated for resistance against carbendazim, flusilazole, tebuconazole, propiconazole, bromuconazole, flutriafol and fenbuconazole. These results indicated that to some triazoles, such as fenbuconazole, a high level of resistance was already present in field populations. In a sexually reproducing fungus such as T. yallundae, knowledge pertaining to its ability to pass resistance factors to offspring is equally important. Mating studies were, therefore, also conducted with parental strains that showed signs of triazole resistance. Three generations were subsequently tested for resistance to five triazoles, namely flusilazole, tebuconazole, propiconazole, bromuconazole and flutriafol. Results of this study showed variable sensitivity in progeny, which indicated quantitative inheritance of resistance to triazoles. Although the sexual stage has not yet been observed in the field in South Africa, this knowledge lays the foundation for the long-term understanding of the population dynamics of the fungus. The ability of a heterothallic ascomycete population to reproduce sexually is dependent on the availability of its two mating types, MATI-I and MATI-2, their distribution, and female fertility amongst other factors. In the UK. the teleomorph is commonly observed in the field, which is in contrast to the situation in South Africa, where it has only been induced in the laboratory. A comparative study between the South African and the UK. populations was therefore undertaken. Isolates representative of the two populations were mated with tester strains as both sperm recipients and as sperm donors. This allowed the percentage of hermaphrodites to be determined. No difference in terms of female fertility was observed between the South African and the UK. populations, with both populations showing low effective population numbers. These data suggested, therefore, that the teleomorph would also occur more frequently in South Africa if the climate was more indusive to its development. The overall results of this study indicated that eyes pot could still be controlled by means of fungicide application in South Africa. Although a shift in sensitivity was observed towards fenbuconazole and flusilazole, no resistance was detected towards carbendazim. The latter might be due to the absen<.:eof the sexual stage in the field, coupled by the monocyclic nature of the pathogen and sensible fungicide regimes. The absence of T. acujormis makes the disease situation less complicated in terms of fungicide application and management. Continuous surveys will have to be conducted, however, to monitor this situation in future.
AFRIKAANSE OPSOMMING: Hierdie studie ondersoek die genetiese variasie, reproduksie dinamika en fungisied weerstand in Tapesia yallundae. Elke hoofstuk handel oor spesifieke maar verwante onderwerpe. Oogvlek is 'n belangrike siekte van lentekoring (Triticum aestivum L.). Vier spesies van Ramulispora word geassosieer met die siekte, waarvan Tapesia yallundae en T. acuformis mees algemeen voorkom. T. yallundae, wat tans die enigste spesie is wat in Suid-Afrika aangeteken is, het al verliese van tot 50% veroorsaak. Om meer akkurate en effektiewe beheermaatreels te implementeer, is dit noodsaaklik om die oorlewingsdinamika van die patogeen te verstaan. Van al die siektebeheermaatreels soos kulturele praktyke, sanitasie, biologiese beheer ens., bly fungisiedbehandeling die mees algemene maatreel vir die beheer van oogvlek. Fungisiedtoediening het egter ook verskeie probleme. Die patogeen kan weerstand opbou teen die fungisied. Die mees algemene fungisiedes wat vir oogvlekbeheer aangewend word sluit onder meer die benzimidasool karbendazim in, triasole soos flusilasool, tebukonasool, propikonasool, bromukonasool, flutriafol, fenbukonasool, triadimenol, en die imidasool, prochloraz. Weerstand is egter reeds teen hierdie middels bekend. Gedurige monitering vir weerstand is dus krities om die vermorsing van fungisied en besoedeling van die omgewing met oneffektiewe middels te beperk. In hoofstuk 2 van hierdie manuskrip word 300 isolate van T. yallundae van 15 lande geevalueer vir weerstand teenoor karbendazim, flusilasool, tebukonasool, propikonasool, bromukonasool, flutriafol en fenbukonasool. Resultate dui daarop dat teen sommige van hierdie triasole, soos bv. fenbukonasool, daar reeds 'n hoe vlak van weerstand teenwoordig was in veldpopulasies. In 'n seksueel reproduserende fungus soos T. yalluJ1dae, is dit noodsaaklik om te bepaal wat sy vermoe is om weerstandbiedenheid aan die nageslag oor te dra. Om die rede is paringstudies ook op ouers wat tekens van weerstand teenoor triasole getoon het uitgevoer. Drie generasies was gevolglik getoets vir weerstand teenoor vyf triasole, naamlik flusilasool, tebuconasool, propikonasool, brumukonasool en flutriafol. Resultate van die studie het 'n variasie in sensitiwiteit van die nageslag getoon, wat op 'n kwantitatiewe oorerwing van weerstand teen £riasole dui. Alhoewel die teleomorf nog nie in lande in Suid-Afrika opgemerk is nie, Ie hierdie kennis die fondament vir die langtermyn vertolking van die populasie dinamika van hierdie fungus. Die vermoe van 'n heterotalliese askomiseet populasie om seksueel voort te plant is afhanklik van die beskikbaarheid van sy twee paringstipes, MATI-I en MATl-2, hul verpreiding, vroulike vrugbaarheid en ander faktore. Alhoewel die teleomorf algemeen in lande in die Verenigde Koninkryk opgemerk word, is dit in kontras met die situasie in Suid-Afrika, waar hierdie stadium nog slegs in die laboratorium gelnduseer kon word. 'n Studie is dus onderneem om die Suid-Afrikaanse en V.K. populasies met mekaar te vergelyk. Isolate van die twee populasies is dus gepaar met paringsisolate as beide sperm ontvangers en sperm donors. Hierdie prosedure het dit moontlik gemaak om die persentasie hermafrodiete te bepaal. Geen verskille in vroulike fertiliteit is tussen die Suid-Afrikaanse en V.K. populasies bespeur nie, en beide populasies het ook 'n lae effektiewe populasie getal getoon. Hierdie data het dus voorgestel dat die teleomorf ook meer algemeen in Suid-Afrika sou voorkom as die klimaat meer geskik was vir teleomorf vormmg. Die resultate van hierdie studie het tot die slotsom gelei dat oogvlek steeds deur fungisiedbehandeling in Suid-Afrika beheer kan word. Alhoewel daar 'n merkbare verskuiwing in sensitiwiteit teenoor fenbukonasool en flusilasool was, was geen weerstand teenoor karbendazim waargeneem nie. Laasgenoemde kan dalk toegeskryf word aan die afwesigheid van die teleomorf in die veld, gekombineer met die monosikliese natuur van die patogeen en gebruik van alternerende fungisiedes. Die afwesigheid van T. acuformis maak die plaaslike siektetoestand minder gekompliseerd in terme van fungisied aanwending en bestuur. Voortdurende opnames sal egter uitgevoer moet word om hierdie situasie ook in die toekoms te monitor.
Blignaut, Marguerite. "The molecular and biological characterisation of ORF5 of three South African variants of Grapevine Vitivirus A". Thesis, Stellenbosch : University of Stellenbosch, 2009. http://hdl.handle.net/10019.1/2421.
Texto completo da fonteGrapevine Vitivirus A (GVA), genus Vitivirus, family Flexiviridae is a well characterised single-stranded RNA virus that has been implicated in the grapevine diseases, Kober stem grooving and Shiraz disease. The virus infects both its host, Vitis vinifera and the experimental model plant, Nicotiana spp.. Biological studies performed on the virus in its herbaceous host, Nicotiana benthami- ana, revealed that many divergent variants of the virus exists in South Africa and can induce di erent symptoms in the model plant. Further molecular analysis divided the variants into three molecular groups based on molecular heterogeneity and nucleotide identity. The establishment of an infectious full-length cDNA clone of GVA contributed towards the elucidation of gene functions for 4 of the 5 open reading frames (ORF's), and indicated ORF5 as the pathogenicity determinant within the genome. Further studies also showed that ORF5 encodes for a nucleic acid binding protein that exhibits suppression activity of a plants' natural virus silencing mechanism. Many proteins that have previously been identi ed as the pathogenicity determinant within a viral genome have been found to encode for suppression activity. Although suppression activity has been elucidated within the ORF5 of the Italian cDNA clone of GVA, IS 151, no such study has yet been performed on the divergent South African variants of GVA. Three variants, GTR1-1, GTR1- 2 and GTG11-1, which represent each of the molecular groups (Group III, II and I), were selected for this study. The aim of this study was to visually elucidate suppression activity of RNA transgene silencing by the ORF5's of GTR1-1, GTR1-2 and GTG11-1 in a transient expression assays in transgenic N. benthamiana (line 16c). Pathogenicity studies for these variants were also performed. The ORF5 of the infectious full-length clone, GVA118, which can also serve as an expression vector, was deleted and provided with restriction enzyme sites into which the respective ORF5s and the marker genes, GFP and GUS could be cloned directionally. Infectivity, symptom development and systemic movement were compared between the di erent full length clones after co-in ltration in N. benthamiana. Preliminary results obtained in this study failed to visually indicate any suppression activity encoded by the ORF5 of GTR1-1, GTR1-2 and GTG11-1. The deletion of ORF5 within GVA118 was successful and rendered the infectious full length clone asymptomatic. Directional cloning of the ORF5 of GTR1-1 into the unique restriction enzymes provided previously, resulted in much milder symptoms than those observe for GTR1-2 and GTG11-1. No GFP and GUS accumulation could be detected. This study has established an infectious full-length cDNA clone, pBINSN-e35SGVA118 ORF5-1-1-pA, that can possibly induce much milder symptoms in the herbaceous host, N. benthamiana. This construct can be further characterised as a possible expression vector of foreign proteins in herbaceous hosts and grapevine.
Behjatnia, Seyyed Ali Akbar. "Characterisation of DNA replication of tomato leaf curl geminivirus /". Title page, contents and abstract only, 1997. http://web4.library.adelaide.edu.au/theses/09ACP/09acpb419.pdf.
Texto completo da fonteGalagedara, Nelomie Nayanathara. "Identification of Quantitative Trait Loci for Resistance to Tan Spot in Durum Wheat". Thesis, North Dakota State University, 2018. https://hdl.handle.net/10365/28765.
Texto completo da fontePresello, Daniel A. "Studies on breeding of maize for resistance to ear rots caused by Fusarium spp. and on the occurrence of viruses in maize in eastern Canada". Thesis, McGill University, 2001. http://digitool.Library.McGill.CA:80/R/?func=dbin-jump-full&object_id=38260.
Texto completo da fonteDu, Preez Jacques. "The construction of an infectious clone of grapevine virus A (GV A)". Thesis, Link to the online version, 2005. http://hdl.handle.net/10019/1012.
Texto completo da fonteHuang, Chunyuan. "Mechanisms of Mn efficiency in barley". 1996, 1996. http://web4.library.adelaide.edu.au/theses/09PH/09phh8739.pdf.
Texto completo da fonteMkhize, Thokozani M. "The detection of cherry leaf-roll nepovirus and the use of molecular markers for germplasm identification in walnuts (Juglans regia L.)". Thesis, Stellenbosch : Stellenbosch University, 2003. http://hdl.handle.net/10019.1/53624.
Texto completo da fonteENGLISH ABSTRACT: The aim of this study was to combine two common diagnostic tools: serological kits and genetic fingerprinting to identify cherry leaf-roll nepovirus (CLRV), and to establish a marker system to characterize walnut germplasm. The detection of plant viruses is difficult. Restrictions are imposed for quarantine purposes on the importation of plant material from foreign countries. Modern techniques such as a PCR based screening method for CLRV are required to ensure material do not harbour viruses. A primer pair was designed to amplify a 430 bp non-coding homologous region. For the choice of primers, consensus sequences were considered and areas where the sequence data shared 98.5% homology, were chosen. The sensitivity of this detection method was 100-fold higher when compared to the ELISA. The PCR fragment was verified by nucleotide sequencing. AFLP technology was used to identify polymorphic fragments for 6 walnut cultivars and a rootstock, and SCARs were developed from AFLP specific bands. The AFLP technique distinguished all the walnut cultivars and the rootstock. However, conversion of AFLP fragments to SCAR markers for the development of a simple robust technique for cultivar discrimination, was not successful. Using 27 AFLP primer combinations, polymorphic fragments as high as 47.8% were scored. The reason for the lack of efficient conversion was as the result of the AFLP technique. The SCAR primers were generated from sequences internal to the AFLP primers but the specificity of the markers was in the AFLP primers not the internal sequence. In this study using AFLP, walnut cultivars were found to be closely related. The AFLP primer pairs used, provided polymorphic fragments. From these fragments, 7 SCAR markers were developed. It was expected that these SCARs derived from the AFLP markers would detect slight differences between cultivars. The Paradox SCAR marker was the only one that could divide the cultivars into two groups. When Chandler SCAR products were digested with the restriction enzyme Rsal, the same banding pattern as that of Paradox SCAR products was observed.
AFRIKAANSE OPSOMMING: Die doel van hierdie studie was om twee algemene opsporingstegnieke te kombineer: serologiese toetsstelle en genetiese vingerafdrukke om cherry leaf-roll nepovirus (CLRV) te eien en om In merkersisteem te ontwikkel wat okkerneut kiemplasma kan karakteriseer. Die opsporing van plant virusse is baie moeilik. As gevolg van kwarantyn vereistes, word daar beperkinge geplaas word op die invoer van plant materiaal vanuit die buiteland. Moderne tegnieke soos hierdie een wat op PKR berus, word benodig om te verseker dat CLRV nie in plantmateriaal teenwoordig is nie. In Stel inleiers is ontwerp wat In 430 bp nie-koderende homoloë area amplifiseer. Hiervoor is konsensus volgordes bestudeer en slegs die volgordes wat 98,5% homologie getoon het, is gekies. In vergelyking met ELISA was die sensitiwiteit van hierdie deteksie metode 100 maal beter. DNA volgordebepaling is op die resulterende fragment gedoen om die PKR produk te verifieer. AFLP tegnologie is gebruik om polimorfiese fraqmente vir 6 okkerneut kultivars en 'n onderstok te identifiseer en SCARs is uit hierdie fragmente ontwikkel. Die AFLP tegniek kon tussen al die okkerneut kultivars en die onderstok onderskei. Die omskakeling van die AFLP fragmente in SCAR merkers om sodoende In eenvoudige kragtige tegniek vir kultivar onderskeiding te ontwikkel, was egter nie suksesvol nie. Met die gebruik van 27 AFLP inleier kombinasies, kon polimorfiese fragmente van so hoog as 47.8% verkry word. Die rede hoekom omskakeling onsuksesvol was lê by die aard van die AFLP tegniek. Die SCAR inleiers is ontwikkel uit volyordes intern tot die AFLP inleiers, maar die spesifisiteit van die merkers het juis in die AFLP inleiers gelê en nie in die interne volgordes nie. In hierdie studie, met die gebruik van AFLP, is gevind dat okkerneut kultivars baie naby verwant is. Die AFLP inleierstelle wat gebruik is, het polimorfiese fragmente gelewer. Uit hierdie fragmente is 7 SCAR merkers ontwikkel. Daar is verwag dat die SCARs wat uit die AFLP merkers ontwikkel is, klein verskille tussen kultivars sou opspoor. Dit was egter net die Paradox SCAR merker wat die kultivars in twee groepe kon verdeel. Restriksie ensiem vertering met Rsalop die Chandler SCAR produkte het dieselfde bandpatrone as die van die Paradox SCAR produkte gelewer.
Du, Min. "A greenhouse screening method for resistance to gray leaf spot in maize". Thesis, Virginia Tech, 1993. http://hdl.handle.net/10919/42953.
Texto completo da fonteBecker, John van Wyk. "Plant defence genes expressed in tobacco and yeast". Thesis, Stellenbosch : University of Stellenbosch, 2002. http://hdl.handle.net/10019/2924.
Texto completo da fonteChoe, Y. W. (Young Won). "DNA markers for cereal cyst nematode (Heterodera avenae Woll.) resistance gene in barley". 1995. http://web4.library.adelaide.edu.au/theses/09PH/09phc545.pdf.
Texto completo da fonteChoe, Y. W. (Young Won). "DNA markers for cereal cyst nematode (Heterodera avenae Woll.) resistance gene in barley / Y.W. Choe". Thesis, 1995. http://hdl.handle.net/2440/18680.
Texto completo da fonteVanstone, Vivien Alison. "The role of fungi and the root lesion nematode, Pratylenchus neglectus, in damaging wheat roots in South Australia / Vivien Alison Vanstone". Thesis, 1991. http://hdl.handle.net/2440/19581.
Texto completo da fontevi, 296 leaves, [14] leaves of plates : ill. (some col.), maps ; 30 cm.
Pathogens associated with root damage were investigated in the Murray Mallee region of South Australia over the 1987-1989 growing seasons. Occurence of fungal species and the root lesion nematode (Pratylenchus neglectus) was assessed, and related to the appearance and severity of symptoms on the roots. Field experiments were supplemented with innoculation tests in the glasshouse and laboratory.
Thesis (Ph.D.)--University of Adelaide, Depts. of Plant Science and Crop Protection, 1991
Farsi, Mohammad. "Genetic variation for tolerance and resistance to Pratylenchus neglectus / by Mohammed Farsi". 1995. http://hdl.handle.net/2440/18625.
Texto completo da fonteix, 347 [24] leaves : ill. (some col.) ; 30 cm.
Title page, contents and abstract only. The complete thesis in print form is available from the University Library.
A major problem in the production of agricultural crops including wheat, is the damage caused by destructive plant parasitic nematodes, among these the root lesion nematode (Pratylenchus spp.) The association of P. neglectus with fungi in ceraeal root disease has been reported. Infection is associated with leaf yellowing, which reduces plant photosynthesis and grain yield. In nematode infested soil, well fertilized crops are usually less affected.
Thesis (Ph.D.)--University of Adelaide, Dept. of Plant Science, 1996?
Farsi, Mohammad. "Genetic variation for tolerance and resistance to Pratylenchus neglectus / by Mohammed Farsi". Thesis, 1995. http://hdl.handle.net/2440/18625.
Texto completo da fonteix, 347 [24] leaves : ill. (some col.) ; 30 cm.
A major problem in the production of agricultural crops including wheat, is the damage caused by destructive plant parasitic nematodes, among these the root lesion nematode (Pratylenchus spp.) The association of P. neglectus with fungi in ceraeal root disease has been reported. Infection is associated with leaf yellowing, which reduces plant photosynthesis and grain yield. In nematode infested soil, well fertilized crops are usually less affected.
Thesis (Ph.D.)--University of Adelaide, Dept. of Plant Science, 1996?
Williams, Kevin John. "Biological and genetic studies of wheat resistance to Heterodera avenae / by Kevin Williams". Thesis, 1994. http://hdl.handle.net/2440/21579.
Texto completo da fonteBibliography: leaves 60-75.
viii, 75, [40] leaves, [24] leaves of plates : ill. (some col.) ; 30 cm.
Thesis (Ph.D.)--University of Adelaide, Dept. of Crop Protection, 1995?
Asiedu, Robert. "A study of resistance to cereal cyst nematode (`Heterodera avenae Woll.`) located in the rye genome of triticale / by Robert Asiedu". 1986. http://hdl.handle.net/2440/21224.
Texto completo da fonteiv, 152 leaves, [47] leaves of plates : ill. (1 col.) ; 30 cm.
Title page, contents and abstract only. The complete thesis in print form is available from the University Library.
Thesis (Ph.D.)--University of Adelaide, 1987
Asiedu, Robert. "A study of resistance to cereal cyst nematode (`Heterodera avenae Woll.`) located in the rye genome of triticale / by Robert Asiedu". Thesis, 1986. http://hdl.handle.net/2440/21224.
Texto completo da fonteTaylor, Christopher 1966. "Cytogenetic and molecular genetic markers for chromosome 6R of rye linked to CCN resistance / by Christopher Taylor". 1996. http://hdl.handle.net/2440/18939.
Texto completo da fontexiv, 175, [96] leaves, [17] leaves of plates : ill. (some col.) ; 30 cm.
Title page, contents and abstract only. The complete thesis in print form is available from the University Library.
This thesis reports on the generation of molecular tools for the analysis of chromosome 6R of rye and the application of these tools in structural analysis of 6RL. Results presented include physical and genetic maps of chromosome 6RL incorporating RFLP and PCR markers and CreR, the locus conferring resistance to cereal cyst nematode (CCN). The ability to detect small introgessions of rye chromatin in wheat is demonstrated.
Thesis (Ph.D.)--University of Adelaide, Dept. of Plant Science, 1997
Mitchell, Aaron Thomas. "Genetic and molecular biological studies of annual ryegrass resistance to Anguina funesta / Aaron Thomas Mitchell". 2002. http://hdl.handle.net/2440/21972.
Texto completo da fonteCorrections on back page.
Bibliography: leaves 118-129.
129 leaves : ill. ; 30 cm.
Title page, contents and abstract only. The complete thesis in print form is available from the University Library.
Annual ryegrass toxicity (ARGT) occurs in grazing animals following the ingestion of seedheads of the annual ryegrass Lolium rigidum, infested with the corynetoxin-producing bacteria, Rathayibacter toxicus. Breaking the disease cycle, through the use of lines of L. rigidum resistant to the nematode Anguina funesta can be used to reduce th risk of ARGT outbreaks. In L. rigidum, resistance to A. funesta appears to be under the control of two unknown, but complementary genes. This study explored alternate approaches towards the allocation of genotype for lines of L. rigidum with respect to resistance to A. funesta.
Thesis (Ph.D.)--University of Adelaide, Dept. of Applied and Molecular Ecology, 2003
Hughes, Peter A. "Mode of action and protective effects of small basic protein toxins in transgenic plants". Phd thesis, 1997. http://hdl.handle.net/1885/145680.
Texto completo da fonteRaisheed, Muhammad Saif-ur. "Tissue targeting signals of Tomato leaf curl virus". Thesis, 2007. http://hdl.handle.net/2440/63571.
Texto completo da fonteThesis (Ph.D.) -- University of Adelaide, School of Agriculture, Food and Wine, 2007
Gilbert, Brian M. "Characterization of the response mediated by the plant disease susceptibility gene LOV1". Thesis, 2012. http://hdl.handle.net/1957/34284.
Texto completo da fonteGraduation date: 2013
Access restricted to the OSU Community at author's request from Oct. 9, 2012 - Oct. 9, 2013
"Disease resistance related genes co-regulated in bacterial leaf blight near isogenic lines, Xa2, Xa12 and Xa14". 2004. http://library.cuhk.edu.hk/record=b5891981.
Texto completo da fonteThesis (M.Phil.)--Chinese University of Hong Kong, 2004.
Includes bibliographical references (leaves 171-186).
Abstracts in English and Chinese.
Thesis committee --- p.i
Statement --- p.ii
Abstract --- p.iii
Acknowledgement --- p.viii
General abbreviations --- p.x
Abbreviations of chemicals --- p.xi
List of figures --- p.xii
List of Tables --- p.xiii
Table of contents --- p.xv
Chapter 1. --- Literature review
Chapter 1.1. --- General introduction to rice disease --- p.1
Chapter 1.1.1. --- Pathogenesis of Bacterial Leaf Blight (BLB) --- p.1
Chapter 1.1.2. --- Pathogenesis of rice blast --- p.2
Chapter 1.1.3. --- Control of rice diseases --- p.3
Chapter 1.2. --- Plant defense mechanisms --- p.4
Chapter 1.2.1. --- Basal resistance in plants --- p.4
Chapter 1.2.2. --- Wound induced defense response --- p.5
Chapter 1.2.3. --- Pathogen induced host defense response --- p.6
Chapter 1.3. --- Structure of R gene products --- p.7
Chapter 1.4. --- Recognition between R and Avr proteins in rice --- p.8
Chapter 1.5 --- Current knowledge on Xa resistance and AvrXa avirulence protein --- p.9
Chapter 1.6 --- Current knowledge on Pi resistance and AvrPi avirulence protein --- p.10
Chapter 1.7 --- Pathogen induced signal transduction cascade --- p.12
Chapter 1.7.1. --- R gene mediated signal transduction cascade --- p.12
Chapter 1.7.2. --- Signal events of G-protein activation --- p.12
Chapter 1.7.3. --- Signaling events for the accumulation of Ca2+ in cytosol --- p.13
Chapter 1.7.4. --- Signaling events for oxidative burst --- p.14
Chapter 1.7.5. --- MAPK cascade in defense signaling --- p.15
Chapter 1.7.6. --- Transcriptional regulation of disease resistance related genes --- p.16
Chapter 1.7.7. --- Translational regulation of disease resistance related genes --- p.17
Chapter 1.8. --- Defense responses and defense related genes --- p.19
Chapter 1.8.1. --- Pathogenesis related (PR) proteins --- p.20
Chapter 1.8.2. --- Phytoalexins --- p.21
Chapter 1.9. --- Disease resistance related genes common between rice blast and BLB resistance --- p.22
Chapter 1.10. --- SA induced signal transduction pathway in rice --- p.23
Chapter 1.11. --- Important tools facilitating the identification of disease resistance related genes from BLB resistant rice lines --- p.24
Chapter 1.12. --- Hypothesis --- p.26
Chapter 1.13. --- Project objective --- p.26
Chapter 2. --- Materials and Methods --- p.27
Chapter 2.1. --- Plant Materials --- p.27
Chapter 2.2. --- Pathogen Inoculation --- p.27
Chapter 2.3. --- RNA extraction --- p.29
Chapter 2.4. --- Denaturing gel electrophoresis --- p.29
Chapter 2.5. --- Subtraction libraries construction --- p.30
Chapter 2.5.1. --- Cloning of disease resistance related genes --- p.32
Chapter 2.5.1.1. --- pBluescript II KS (+) T-vector preparation --- p.32
Chapter 2.5.1.2. --- Ligation --- p.32
Chapter 2.5.1.3. --- Transformation --- p.32
Chapter 2.5.1.4. --- Colony picking --- p.33
Chapter 2.5.1.5. --- PCR amplification of DNA inserts --- p.33
Chapter 2.5.1.6. --- Purification of PCR products --- p.34
Chapter 2.6. --- Gene chips printing --- p.34
Chapter 2.7. --- Probes synthesis and gene chips hybridization --- p.35
Chapter 2.8. --- Standard-RNAs synthesis --- p.35
Chapter 2.9. --- Data collection and analysis --- p.36
Chapter 2.10. --- Sequencing --- p.36
Chapter 2.11. --- cDNA synthesis --- p.37
Chapter 2.12. --- RT-PCR --- p.38
Chapter 2.13. --- DNA gel electrophoresis --- p.39
Chapter 3. --- Results --- p.58
Chapter 3.1. --- Construction of BLB gene chips --- p.58
Chapter 3.1.1. --- Preparation of cDNA clones for gene chips construction --- p.58
Chapter 3.1.2. --- Purification of PCR products on microtiter plate --- p.59
Chapter 3.1.3. --- Gene chips construction --- p.59
Chapter 3.1.4. --- DNA immobilization --- p.62
Chapter 3.1.5. --- Probe synthesis --- p.62
Chapter 3.1.6. --- Gene chip analysis --- p.65
Chapter 3.1.6.1. --- Scanning --- p.65
Chapter 3.1.6.2. --- Data analysis --- p.65
Chapter 3.2. --- "Identification of disease resistance related genes commonly regulated by Xa2, Xal2 and Xal4 BLB resistance loci" --- p.70
Chapter 3.2.1. --- "Signal perception, transduction and regulatory elements" --- p.71
Chapter 3.2.1.1. --- Proteins involved in reversible phosphorylation cascade --- p.71
Chapter 3.2.1.2. --- Proteins potentiate signal transduction through specific protein-protein interaction --- p.72
Chapter 3.2.1.3. --- Other signal transduction components --- p.73
Chapter 3.2.2. --- Transcriptional and translational regulatory elements --- p.74
Chapter 3.2.2.1. --- Proteins involved in transcriptional regulation --- p.74
Chapter 3.2.2.2. --- Proteins involved in post-transcriptional regulation --- p.75
Chapter 3.2.2.3. --- Proteins involved in translational regulation --- p.76
Chapter 3.2.3. --- "Oxidative burst, stress, apoptotic related genes" --- p.77
Chapter 3.2.3.1. --- Stress related proteins --- p.77
Chapter 3.2.3.2. --- Proteins involved in induction of oxidative burst --- p.78
Chapter 3.2.3.3. --- PR proteins --- p.79
Chapter 3.2.3.4. --- Proteolysis related proteins --- p.79
Chapter 3.2.4. --- Cell maintenance and metabolic genes --- p.80
Chapter 3.2.4.1. --- Antioxidant --- p.80
Chapter 3.2.4.2. --- Metabolic genes --- p.81
Chapter 3.2.4.3. --- Molecular chaperone --- p.82
Chapter 3.2.4.4. --- Cell cycle regulators --- p.82
Chapter 3.2.4.5. --- Cell wall maintenance --- p.83
Chapter 3.2.4.6. --- Proteins involved in protein transport --- p.83
Chapter 3.2.5. --- Unclassified/others --- p.84
Chapter 3.3. --- Expression analysis of disease resistance related genes --- p.88
Chapter 4. --- Discussion --- p.141
Chapter 4.1. --- Differential expression of disease resistance candidates --- p.141
Chapter 4.2. --- Disease resistance signal transduction components --- p.143
Chapter 4.2.1. --- Reversible phosphorylation cascade --- p.143
Chapter 4.2.2. --- Signal transduction potentiated by protein-protein interaction --- p.144
Chapter 4.3. --- Other signaling molecules --- p.145
Chapter 4.3.1. --- PRL1-interacting factor G --- p.145
Chapter 4.3.2. --- Vacuolar-type H+-ATPasen subunit G --- p.146
Chapter 4.4. --- Regulation of expression of disease resistance candidates --- p.146
Chapter 4.4.1. --- Transcriptional regulation of disease resistance related genes --- p.146
Chapter 4.4.1.1. --- G-box binding protein --- p.147
Chapter 4.4.1.2. --- MYB TF --- p.147
Chapter 4.4.2. --- Post-transcriptional modification of disease resistance candidates --- p.148
Chapter 4.4.2.1. --- RNA splicing factor --- p.148
Chapter 4.4.2.2. --- Glycine rich RNA binding proteins --- p.149
Chapter 4.4.3. --- Translational regulation of disease resistance related genes --- p.149
Chapter 4.5. --- Induction of oxidative burst --- p.150
Chapter 4.6. --- PR proteins --- p.151
Chapter 4.7. --- Cell maintenance --- p.152
Chapter 4.7.1. --- Protein folding --- p.152
Chapter 4.7.2. --- Protein degradation --- p.153
Chapter 4.7.3. --- ROS scavenging --- p.154
Chapter 4.7.4. --- Regulation of cell cycle --- p.154
Chapter 4.8. --- "Confirmation and profiling of disease resistance related candidates commonly regulated in Xa2, Xal2 and Xal4 BLB resistance NILs at different time points" --- p.155
Chapter 4.8.1. --- Basal resistance related genes --- p.156
Chapter 4.8.2. --- General disease resistance related genes --- p.161
Chapter 4.8.3. --- Pathogen responsive genes --- p.164
Chapter 4.8.4. --- Prediction of novel genes functions --- p.168
Chapter 4.9. --- Future prospect --- p.169
Chapter 4.10. --- Conclusion --- p.169
References --- p.171
Appendix --- p.187
Behjatnia, Seyyed Ali Akbar. "Characterisation of DNA replication of tomato leaf curl geminivirus / Seyyed Ali Akbar Behjatnia". Thesis, 1997. http://hdl.handle.net/2440/14766.
Texto completo da fontexi, 152 leaves : ill. (some col.), col. map ; 30 cm.
Studies biological relatedness of strains of tomato leaf curl virus and cross-interaction with the replication-associated protein requireed for DNA replication.
Thesis (Ph.D.)--University of Adelaide, Dept. of Crop Protection, 1997
Wilson, Ryan. "Functional studies of the Cf-9/Avr9 interaction". Phd thesis, 2003. http://hdl.handle.net/1885/151590.
Texto completo da fonteSow, Mounirou El-Hassimi. "Genetic diversity of Oryza species in Niger ; screening and breeding for resistance to rice yellow mottle virus (RYMV)". Thesis, 2012. http://hdl.handle.net/10413/8520.
Texto completo da fonteThesis (Ph.D.)-University of KwaZulu-Natal, Pietermaritzburg, 2012.
Mweshi, Mukanga. "Genetic improvement of Zambian maize (Zea mays L.) populations for resistance to ear rots and a survey of associated mycotoxins". Thesis, 2009. http://hdl.handle.net/10413/519.
Texto completo da fonteThesis (Ph.D) - University of KwaZulu-Natal, Pietermaritzburg, 2009.
Barker, Claire Louise. "An Examination of the signalling capacity of the tomato Cf-9 disease resistance protein". Phd thesis, 2002. http://hdl.handle.net/1885/148656.
Texto completo da fonteChakrabarti, Apratim. "Structure-function analysis of Cf-9 and Cf-9B resistance proteins from tomato (Lycopersion [i.e. Lycopersicon] esculentum Mill.)". Phd thesis, 2005. http://hdl.handle.net/1885/149669.
Texto completo da fontePanter, Stephen Neil. "Functional domains, expression and potential dimerisation of the Cf-9 and Cf-9B fungus resistance proteins of tomato (Lycopersicon esculentum Mill.)". Phd thesis, 2001. http://hdl.handle.net/1885/151625.
Texto completo da fonteHuang, Chunyuan. "Mechanisms of Mn efficiency in barley / by Chunyuan Huang". Thesis, 1996. http://hdl.handle.net/2440/18731.
Texto completo da fontexiii, 153 leaves : ill. (some col.) ; 30 cm.
This thesis investigates the mechanisms of manganese (Mn) efficiency (genetic tolerance to Mn-deficient soils) in barley (Hordeum vulgare L.) at both physiological and molecular levels.
Thesis (Ph.D.)--University of Adelaide, Dept. of Plant Science, 1996
Moodley, Vaneson. "Development of a pepper (Capsicum annuum L.) hybrid variety with resistance to potato virus Y (PVY) using molecular breeding". Thesis, 2013. http://hdl.handle.net/10413/10829.
Texto completo da fonteThesis (M.Sc.)-University of KwaZulu-Natal, Pietermaritzburg, 2013.
Mengesha, Wende Abera. "Genetic diversity, stability, and combining ability of maize genotypes for grain yield and resistance to NCLB in the mid-altitude sub-humid agro ecologies of Ethiopia". Thesis, 2013. http://hdl.handle.net/10413/10935.
Texto completo da fonteThesis (Ph.D.)-University of KwaZulu-Natal, Pietermaritzburg, 2013.
Mariote, David. "Response to selection for downy mildew (Peronosclerospora sorghi) and maize streak virus resistance in three quality protein maize populations in Mozambique". Thesis, 2007. http://hdl.handle.net/10413/748.
Texto completo da fonteIbaba, Jacques Davy. "Characterization of potato virus Y (PVY) isolates infecting solanaceous vegetables in KwaZulu-Natal (KZN), Republic of South Africa (RSA)". Thesis, 2009. http://hdl.handle.net/10413/613.
Texto completo da fonteThesis (M.Sc.) - University of KwaZulu-Natal, Pietermaritzburg, 2009.
Kam, Honore. "A study of the diversity of Burkina Faso rice landraces and identification of source of resistance to rice yellow mottle virus (RYMV)". Thesis, 2011. http://hdl.handle.net/10413/8518.
Texto completo da fonteThesis (Ph.D.)-University of KwaZulu-Natal, Pietermaritzburg, 2011.
Bucheyeki, Tulole Lugendo. "Characterization and genetic analysis of maize germplasm for resistance to northern corn leaf blight disease in Tanzania". Thesis, 2012. http://hdl.handle.net/10413/8730.
Texto completo da fonteThesis (Ph.D.)-University of KwaZulu-Natal, Pietermaritzburg, 2012.
Mhora, Terence Tariro. "Genomics of quantitative resistance to brown rust (Puccinia melanocephala) in a sugarcane breeding population". Thesis, 2012. http://hdl.handle.net/10413/10036.
Texto completo da fonteThesis (M.Sc.Agric)-University of KwaZulu-Natal, Pietermaritzburg, 2012.
Mafu, Nothando Fowiza. "Marker-assisted selection for maize streak virus resistance and concomitant conventional selection for Downy Mildew resistance in a maize population". Thesis, 2013. http://hdl.handle.net/10413/10023.
Texto completo da fonteThesis (M.Sc.Agric)-University of KwaZulu-Natal, Pietermaritzburg, 2013.
Gichuru, Lilian Njeri. "Breeding investigations on utility of maize streak virus resistant germplasm for hybrid development in the tropics". Thesis, 2014. http://hdl.handle.net/10413/10694.
Texto completo da fonteThesis (Ph.D.)-University of KwaZulu-Natal, Pietermaritzburg, 2013.
"Studies on brown rust (Puccinia melanocephala) of sugarcane in South Africa". Thesis, 2009. http://hdl.handle.net/10413/2625.
Texto completo da fonteThesis (M.Sc.)-University of KwaZulu-Natal, Pietermaritzburg, 2009.
Chikoti, Patrick Chiza. "Development of cassava (Manihot esculenta Crantz) cultivars for resistance to cassava mosaic disease in Zambia". Thesis, 2011. http://hdl.handle.net/10413/8402.
Texto completo da fonteThesis (Ph.D.)-University of KwaZulu-Natal, Pietermaritzburg, 2011.