Идентификация Fusarium spp. и Alternaria spp. в семенах некоторых овощных культур

In this paper the results of molecular diagnostics of Fusarium spp. and Alternaria spp. in bell pep-per and eggplant seeds of local genotypes at different time points of storage are presented. The diagnos-tics was effectuated using nested-PCR protocol with genus-specific and species-specific primers to F. ox-ysporum, F. solani, F. nivale, F. equiseti, F. culmorum, F. verticillioides, F. avenaceum, A. alternata, and A. solani. In the samples of studied bell pepper and eggplant genotypes A. alternata was found. In egg-plant seeds certain species of Fusarium spp. were identified.

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Amplification of single bulb mites by nested PCR: Species-specific primers to detect Rhizoglyphus robini and R. setosus (Acari: Acaridae)

Journal of Asia-Pacific Entomology ◽

10.1016/j.aspen.2010.05.002 ◽

2010 ◽

Vol 13 (4) ◽

pp. 267-271 ◽

Cited By ~ 2

Author(s):

Hui-Yi Li ◽

Tsen Hua ◽

Wen-Bin Yeh

Keyword(s):

Nested Pcr ◽

Specific Primers ◽

Rhizoglyphus Robini ◽

Species Specific

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A Nested PCR Assay for Detecting Valsa mali var. mali in Different Tissues of Apple Trees

Plant Disease ◽

10.1094/pdis-05-11-0387-re ◽

2012 ◽

Vol 96 (11) ◽

pp. 1645-1652 ◽

Cited By ~ 12

Author(s):

Rui Zang ◽

Zhiyuan Yin ◽

Xiwang Ke ◽

Xiaojie Wang ◽

Zhengli Li ◽

...

Keyword(s):

Nested Pcr ◽

Detection Rate ◽

Pcr Analysis ◽

Pcr Assay ◽

Apple Trees ◽

Specific Primers ◽

Fungal Isolation ◽

Species Specific ◽

Valsa Mali ◽

Different Tissues

A nested polymerase chain reaction (PCR) assay for detecting Valsa mali var. mali, the causal agent of apple tree Valsa canker, was developed. One pair of genus-specific primers was designed based on the ribosomal DNA internal transcribed spacer conservative sequence of the Valsa genus and one pair of species-specific primers was designed based on the specific sequence of V. mali var. mali. The specificity of the genus-specific and species-specific primers was evaluated against 10 V. mali var. mali isolates, 10 V. mali var. pyri isolates, 4 isolates from closely related Valsa spp., and 8 isolates from fungal species that are commonly isolated from naturally infected apple bark tissue. A distinct band of 348 bp in length was detected in all V. mali var. mali isolates but not in other tested species and the V. mali var. pyri variety. The sensitivity of this assay was evaluated by serial dilutions of DNA extracted from V. mali var. mali pure cultures and apple bark tissues with or without visible symptoms. The results showed that the assay was able to detect as little as 100 fg of DNA in mycelial samples and apple bark tissues with visible symptoms, whereas the lowest detectable concentration was 10 pg of DNA in symptomless apple bark tissues. The efficiency of the nested PCR assay was compared with that of fungal isolation assays. All symptomless and symptomatic samples from which the pathogen was successfully isolated yielded a PCR product of the expected size. The detection rate of nested PCR for symptomless samples was 64.7%, which was much higher than the detection rate of 20.6% by fungal isolation. The PCR analysis of different symptomless tissues showed that the incidence of V. mali var. mali was different in different tissues of apple trees. The average incidence of V. mali var. mali was 89% in terminal buds, 71% in internodes, and 48% in bud scale scars. Moreover, the incidence of V. mali var. mali in nonsymptomatic tissues was higher in orchards where more trees were infected. Taken together, the assay developed in this study can be used for rapid and reliable detection of V. mali var. mali in tissues of apple trees with or without symptoms and also for monitoring the presence of the pathogen at an early stage of disease development.

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Detection of Ustilaginoidea virens in rice panicles before and after heading in the field using nested-PCR technique with species-specific primers.

Japanese Journal of Phytopathology ◽

10.3186/jjphytopath.71.16 ◽

2005 ◽

Vol 71 (1) ◽

pp. 16-19 ◽

Cited By ~ 10

Author(s):

T. ASHIZAWA ◽

Y. KATAOKA

Keyword(s):

Nested Pcr ◽

Specific Primers ◽

Ustilaginoidea Virens ◽

Before And After ◽

Species Specific ◽

Rice Panicles

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Supplementary data for: Development of Species-Specific Primers for Agronomical Thrips and Multiplex Assay for Quarantine Identification of Western Flower Thrips

Journal of Economic Entomology ◽

10.1603/ec14027sf1 ◽

2014 ◽

Keyword(s):

Western Flower Thrips ◽

Multiplex Assay ◽

Supplementary Data ◽

Specific Primers ◽

Flower Thrips ◽

Species Specific

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Distribution Analysis of Six PredominantBacteroidesSpecies in Normal Human Feces Using 16S rDNA-Targeted Species-Specific Primers

Microbial Ecology in Health and Disease ◽

10.3402/mehd.v14i3.8239 ◽

2002 ◽

Vol 14 (3) ◽

Cited By ~ 1

Author(s):

Yukiko Miyamoto ◽

Koichi Watanabe ◽

Ryuichiro Tanaka ◽

Kikuji Itoh

Keyword(s):

16S Rdna ◽

Distribution Analysis ◽

Human Feces ◽

Specific Primers ◽

Normal Human ◽

Species Specific

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Possibilities of modified atmosphere packaging to prevent the occurrence of internal fruit rot in bell pepper fruit (Capsicum annuum) caused by Fusarium spp

Postharvest Biology and Technology ◽

10.1016/j.postharvbio.2021.111545 ◽

2021 ◽

Vol 178 ◽

pp. 111545

Author(s):

M. Frans ◽

R. Aerts ◽

N. Ceusters ◽

S. Luca ◽

J. Ceusters

Keyword(s):

Capsicum Annuum ◽

Modified Atmosphere Packaging ◽

Bell Pepper ◽

Fruit Rot ◽

Modified Atmosphere ◽

Fusarium Spp ◽

Pepper Fruit ◽

Internal Fruit Rot

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Development and Validation of a Nested-PCR-Denaturing Gradient Gel Electrophoresis Method for Taxonomic Characterization of Bifidobacterial Communities

Applied and Environmental Microbiology ◽

10.1128/aem.69.11.6380-6385.2003 ◽

2003 ◽

Vol 69 (11) ◽

pp. 6380-6385 ◽

Cited By ~ 52

Author(s):

R. Temmerman ◽

L. Masco ◽

T. Vanhoutte ◽

G. Huys ◽

J. Swings

Keyword(s):

Nested Pcr ◽

Gel Electrophoresis ◽

Denaturing Gradient Gel Electrophoresis ◽

Temporal Changes ◽

Rrna Gene ◽

Specific Pcr ◽

Gradient Gel Electrophoresis ◽

Species Specific ◽

Taxonomic Characterization

ABSTRACT The taxonomic characterization of a bacterial community is difficult to combine with the monitoring of its temporal changes. None of the currently available identification techniques are able to visualize a “complete” community, whereas techniques designed for analyzing bacterial ecosystems generally display limited or labor-intensive identification potential. This paper describes the optimization and validation of a nested-PCR-denaturing gradient gel electrophoresis (DGGE) approach for the species-specific analysis of bifidobacterial communities from any ecosystem. The method comprises a Bifidobacterium-specific PCR step, followed by purification of the amplicons that serve as template DNA in a second PCR step that amplifies the V3 and V6-V8 regions of the 16S rRNA gene. A mix of both amplicons is analyzed on a DGGE gel, after which the band positions are compared with a previously constructed database of reference strains. The method was validated through the analysis of four artificial mixtures, mimicking the possible bifidobacterial microbiota of the human and chicken intestine, a rumen, and the environment, and of two fecal samples. Except for the species Bifidobacterium coryneforme and B. indicum, all currently known bifidobacteria originating from various ecosystems can be identified in a highly reproducible manner. Because no further cloning and sequencing of the DGGE bands is necessary, this nested-PCR-DGGE technique can be completed within a 24-h span, allowing the species-specific monitoring of temporal changes in the bifidobacterial community.

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Species-specific duplex PCR for the detection of Pratylenchus penetrans

Nematology ◽

10.1163/156854109x428016 ◽

2009 ◽

Vol 11 (6) ◽

pp. 847-857 ◽

Cited By ~ 21

Author(s):

Lieven Waeyenberge ◽

Nicole Viaene ◽

Maurice Moens

Keyword(s):

Internal Control ◽

Dna Sequences ◽

Rrna Gene ◽

Duplex Pcr ◽

Specific Primers ◽

5.8S Rrna Gene ◽

5.8S Rrna ◽

Wide Range ◽

Pcr Products ◽

Species Specific

Abstract ITS1, the 5.8S rRNA gene and ITS2 of the rDNA region were sequenced from 20 different Pratylenchus species. Additionally, the same region was sequenced from seven populations of P. penetrans. After purifying, cloning and sequencing the PCR products, all sequences were aligned in order to find unique sites suitable for the design of species-specific primers for P. penetrans. Since ITS regions showed variability between and even within populations of P. penetrans, only three small DNA sequences were suitable for the construction of three potentially useful species-specific primers. New species-specific primers were paired with existing universal ITS primers and tested in all possible primer combinations. The best performing primer set, supplemented with a universal 28S rDNA primer set that served as an internal control, was tested in duplex PCR. The ideal annealing temperature, Mg2+ concentration and primer ratios were then determined for the most promising primer set. The optimised duplex PCR was subsequently tested on a wide range of different Pratylenchus spp. and 25 P. penetrans populations originating from all over the world. To test the sensitivity, the duplex PCR was conducted on DNA extracted from a single P. penetrans nematode mixed with varying amounts of nematodes belonging to another Pratylenchus species. Results showed that a reliable and sensitive P. penetrans species-specific duplex PCR was constructed.

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