Innovative tools for detection of plant pathogenic viruses and bacteria

被引:0
作者
María M. López
Edson Bertolini
Antonio Olmos
Paola Caruso
María Teresa Gorris
Pablo Llop
Ramón Penyalver
Mariano Cambra
机构
[1] Instituto Valenciano de Investigaciones Agrarias,
来源
International Microbiology | 2003年 / 6卷
关键词
Antibodies; Co-operational PCR; DNA microarrays; ELISA; Enrichment; FISH; Multiplex PCR; Nested-multiplex PCR; Real time PCR;
D O I
暂无
中图分类号
学科分类号
摘要
Detection of harmful viruses and bacteria in plant material, vectors or natural reservoirs is essential to ensure safe and sustainable agriculture. The techniques available have evolved significantly in the last few years to achieve rapid and reliable detection of pathogens, extraction of the target from the sample being important for optimising detection. For viruses, sample preparation has been simplified by imprinting or squashing plant material or insect vectors onto membranes. To improve the sensitivity of techniques for bacterial detection, a prior enrichment step in liquid or solid medium is advised. Serological and molecular techniques are currently the most appropriate when high numbers of samples need to be analysed. Specific monoclonal and/or recombinant antibodies are available for many plant pathogens and have contributed to the specificity of serological detection. Molecular detection can be optimised through the automatic purification of nucleic acids from pathogens by columns or robotics. New variants of PCR, such as simple or multiplex nested PCR in a single closed tube, co-operative-PCR and real-time monitoring of amplicons or quantitative PCR, allow high sensitivity in the detection of one or several pathogens in a single assay. The latest development in the analysis of nucleic acids is micro-array technology, but it requires generic DNA/RNA extraction and pre-amplification methods to increase detection sensitivity. The advances in research that will result from the sequencing of many plant pathogen genomes, especially now in the era of proteomics, represent a new source of information for the future development of sensitive and specific detection techniques for these microorganisms.
引用
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页码:233 / 243
页数:10
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