| Literature DB >> 29709963 |
Fumihiko Kawamori1,2, Yukie Shimazu3, Hiroko Sato4, Naota Monma5, Asaka Ikegaya1, Seigo Yamamoto6, Hiromi Fujita7, Hiroshi Morita8, Yukiko Tamaki9, Naoya Takamoto2, Hongru Su2, Masahiko Shimada2, Yuko Shimamura2, Shuichi Masuda2, Shuji Ando10, Norio Ohashi2.
Abstract
Tsutsugamushi disease and Japanese spotted fever are representative rickettsioses in Japan, and are caused by infection with Orientia tsutsugamushi and Rickettsia japonica, respectively. For molecular-based diagnosis, conventional PCR assays, which independently amplify respective rickettsial DNA, are usually used; however, this approach is time-consuming. Here, we describe a new duplex real-time PCR assay for the simultaneous detection of O. tsutsugamushi and spotted fever group rickettsiae, and its evaluation using several PCR conditions in 6 public health laboratories. The detection limit of the assay was estimated to be 102 copies and the sensitivity was almost identical to that of 3 conventional PCR methods. A total of 317 febrile patients were selected as clinically suspected or confirmed cases of rickettsioses. The detection efficiency of this assay for O. tsutsugamushi from blood or skin (eschar) specimens appeared to be almost the same as that of the conventional PCR method, even when performed in different laboratories, whereas the efficiency for spotted fever group rickettsiae tended to be higher than that of the 2 traditional double PCR assays. Our duplex real-time PCR is thus a powerful tool for the rapid diagnosis of rickettsioses, especially at the acute stage of infection.Entities:
Keywords: Orientia tsutsugamushi; Rickettsia japonica; diagnosis; duplex real-time PCR; rickettsiosis
Mesh:
Year: 2018 PMID: 29709963 DOI: 10.7883/yoken.JJID.2017.447
Source DB: PubMed Journal: Jpn J Infect Dis ISSN: 1344-6304 Impact factor: 1.362