Molecular Detection of <i>Diaporthe phaseolorum</i> and <i>Phomopsis longicolla</i> from Soybean Seeds

Zhang, A. W.; Hartman, G. L.; Curio-Penny, B.; Pedersen, W. L.; Becker, Kathryn

doi:10.1094/phyto.1999.89.9.796

Cited by 92 publications

(79 citation statements)

References 33 publications

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“…caulivora. Zhang et al (1998) also by using PCRrestriction fragment length polymorphism, detected genomic differences among D. phaseolorum var. caulivora isolates and D. phaseolorum var.…”

Section: Resultsmentioning

confidence: 99%

Molecular Characterization of Phomopsis vexans Isolates of Eggplant of Bangladesh

Islam

Asaduzzaman

Meah³

2013

J Sci Found

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Forty-four isolates of Phomopsis vexans were collected from eggplant producing areas of Bangladesh during the 2008-2009 growing seasons. The polymerase chain reaction (PCR) -variable number of tandem repeats (VNTR) technique was used to develop molecular markers. The MR-20 primer amplified template DNA for all isolates studied and resulted in distinct bands. The banding patterns of P. vexans isolates were separated into five groups after results with Taq polymerase. The highest genomic DNA concentration 50 ng/µl was found in the isolates of 8, 14, 26, 27 and 38, and the lowest concentration of genomic DNA was found 12.5 ng/µl in the isolates of 1, 2, 5, 15, 17, 22, 30, 31, 33, 34, 36, 40, 41, 42 and 43. Based on the fingerprinting the 44 isolates of Phomopsis vexans were categorized into five different groups.

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“…caulivora. Zhang et al (1998) also by using PCRrestriction fragment length polymorphism, detected genomic differences among D. phaseolorum var. caulivora isolates and D. phaseolorum var.…”

Section: Resultsmentioning

confidence: 99%

Molecular Characterization of Phomopsis vexans Isolates of Eggplant of Bangladesh

Islam

Asaduzzaman

Meah³

2013

J Sci Found

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“…Prior to the pathogenicity tests, each isolate of P. longicolla was examined for sporulation, dimension of conidia, pattern of stroma, and presence or absence of hyaline, filiform, and hamate beta conidia and perithecia to confirm identification (Hartman et al, 1999). The identifications of soybean isolates were verified previously by sequence analysis of the ITS regions and the mitochondrial small subunit rRNA genes (Li et al, 2001;Zhang et al, 1998). The identities of 11 other Phomopsis spp.…”

Section: Aggressiveness Of Phomopsis Longicolla and Other Phomopsis Smentioning

confidence: 87%

“…These primers could be used to specifically distinguish PSD-causal pathogens from each other and from other soybean fungal pathogens (Zhang et al, 1997). There were no differences in ITS sequences among seven geographically diverse isolates of P. longicolla (Zhang et al, 1998). Results from analysis of DNA from the Diaporthe -Phomopsis complex using PCR-restriction fragment length polymorphisms (PCR-RFLP) and DNA sequencing in the ITS and the 5.8 ribosomal DNA, along with morphological examination, indicated that P. longicolla is a distinct species, that D. phaseolorum var.…”

Section: Molecular Detection and Identification Of The Pathogensmentioning

confidence: 98%

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Phomopsis Seed Decay of Soybean

Li¹

2011

Soybean - Molecular Aspects of Breeding

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“…In addition, the rapid development of new molecular techniques, combined with the increasing knowledge on structure and function of resistance genes, will help getting new molecular markers for MAS (Hulbert et al 2001). Such methods offer the advantage of reducing or eliminating the need for lengthy culturing and difficult morphological identification procedures (Hamelin et al 1993;Zhang et al 1999). The potential benefits of this technology have been especially recognized in the regulatory field, where time and accuracy of identifications are crucial (Goodwin and Annis 1991;Smith et al 1996).…”

Section: Discussionmentioning

confidence: 99%

Developing of DNA-Marker to the Fusarium Oxysporum F. Sp. Lycopersici Resistance Genes of Tomato

Amini¹

2009

Journal of Plant Protection Research

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Fusarium wilt caused by Fusarium oxysporum f. sp. lycopersici is a destructive disease of tomato crops worldwide. The use of resistant varieties is the best strategy for disease control.In the present study we analyze eight tomato lines and hybrids for Fusarium wilt disease resistance by polymerase chain reaction. Total genomic DNA was extracted from young leaves of three-week-old plants of tomato. Results of PCR of eight tomato lines and hybrids indicated that there are one dominant heterozygote, two recessive homozygotes and five dominant homozygotes. Also, results of polymerase chain reaction showed that it needs less time and is cheaper. Also by using this method, it is possible to determine genotype of plant (homozygote or heterozygote) without presence of the pathogen. Therefore, PCR technique was used in the identification gene I2 conferring resistance to F. oxysporum f. sp. lycopersici.

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Molecular Detection of Diaporthe phaseolorum and Phomopsis longicolla from Soybean Seeds

Cited by 92 publications

References 33 publications

Molecular Characterization of Phomopsis vexans Isolates of Eggplant of Bangladesh

Molecular Characterization of Phomopsis vexans Isolates of Eggplant of Bangladesh

Phomopsis Seed Decay of Soybean

Developing of DNA-Marker to the Fusarium Oxysporum F. Sp. Lycopersici Resistance Genes of Tomato

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