Pooler M R, Myung I S, Bentz J, Sherald J, Hartung J S
US National Arboretum, United States Department of Agriculture, Washington, DC, USA.
Lett Appl Microbiol. 1997 Aug;25(2):123-6. doi: 10.1046/j.1472-765x.1997.00188.x.
A sensitive and specific assay for detecting Xylella fastidiosa in potential insect vectors was developed. This assay involves immunomagnetic separation of the bacteria from the insect, followed by a two-step, nested polymerase chain reaction (PCR) amplification using previously developed oligonucleotide primers specific to X. fastidiosa. A total of 347 leafhoppers representing 16 species were captured and sampled from American elm (Ulmus americana L.) trees growing in a nursery where bacterial leaf scorch caused by X. fastidiosa occurs. Two of these leafhopper species, Graphocephala coccinea and G. versuta, regularly tested positive for X. fastidiosa using this technique. These insects are therefore potential vectors of X. fastidiosa. Using immunocapture and nested PCR, it was possible to detect as few as five bacteria per sample.
开发了一种用于检测潜在昆虫传播媒介中桑氏假单胞菌的灵敏且特异的检测方法。该检测方法包括从昆虫中对细菌进行免疫磁珠分离,随后使用先前开发的针对桑氏假单胞菌的寡核苷酸引物进行两步巢式聚合酶链反应(PCR)扩增。从一个苗圃中生长的美国榆(Ulmus americana L.)树上捕获并采样了总共347只叶蝉,它们代表16个物种,该苗圃中发生了由桑氏假单胞菌引起的细菌性叶焦病。使用该技术,其中两种叶蝉,即红背叶蝉(Graphocephala coccinea)和多变叶蝉(G. versuta),对桑氏假单胞菌的检测经常呈阳性。因此,这些昆虫是桑氏假单胞菌的潜在传播媒介。使用免疫捕获和巢式PCR,每个样本中低至五个细菌都有可能被检测到。
Zotero 插件