A dual IC-RT-PCR procedure for detection was developed in which the antibodies of LSV and ArMV were mixed and the mixture used RAD001 in vivo to coat the PCR tubes. The particles of the two viruses were captured by the respective antibodies. Interference by other RNA viruses in infected lily was eliminated in the RT-PCR. Also, an RNA extraction step was omitted. The dual IC-RT-PCR products of LSV and ArMV were 521 bp and 691 bp, respectively. The specificity of the method was validated; only LSV and ArMV of four viruses were detected by dual IC-RT-PCR. The sensitivity of the detection method is 1 mg leaf tissue and higher than DAS-ELISA due to enrichment by dual immunocapture. “
“Turnip
mosaic virus (TuMV) is one of the most devastating threats to the vegetable industry. A rapid, stable and sensitive one-step reverse transcription loop-mediated isothermal amplification (RT-LAMP) assay was developed for detecting TuMV. This method is very rapid and sensitive. The sensitivity was c. 10-fold higher than that of conventional RT-PCR in Atezolizumab datasheet detecting TuMV. In addition, it does not require specialized equipment and can be performed under general experimental conditions. This RT-LAMP method has great potential usefulness for TuMV
detection, identification and control strategies. “
“Sorghum ergot is a serious disease that has caused major losses in sorghum growing regions worldwide. Claviceps africana, originally reported from Zimbabwe, is now the most widely
distributed species causing ergot in many countries including the United States of America, whereas both C. africana and Claviceps sorghi exist in India. A third species (Claviceps sorghicola) has been described causing sorghum ergot in Japan. As the three species show morphological similarities, a DNA-based assay is desirable for rapid identification in cases where ergot-infected sorghum is found by regulatory authorities. We designed PCR primers and probes from the intron 3 region of the β-tubulin gene (for C. africana and C. sorghi) and the intron 4 region of EF-1α (for C. sorghicola) and tested them by real-time PCR with purified DNA and ergot samples from the field and greenhouse. The primer and probe sets specifically amplified DNA from the respective species with click here a detection limit of c. 1 pg DNA. Genomic DNA from six other Claviceps species did not amplify in any of the three ergot species-specific assays. The assays we describe will provide useful tools for detecting sorghum ergot pathogens in seed and grain shipments and for determining which species are present in the samples, thereby aiding in the regulatory decision-making process. “
“Avocado scab was recorded as present in New Zealand in international databases on the basis of one isolate (ICMP 10613) identified by morphological features as Sphaceloma perseae.