Identification of Candida auris and related species by multiplex PCR based on unique GPI protein-encoding genes

被引:23
作者
Alvarado, Maria [1 ]
Bartolome Alvarez, Joaquin [2 ]
Lockhart, Shawn R. [3 ]
Valentin, Eulogio [4 ]
Ruiz-Gaitan, Alba Cecilia [5 ]
Eraso, Elena [6 ]
de Groot, Piet W. J. [1 ]
机构
[1] Univ Castilla La Mancha, Reg Ctr Biomed Res, Castilla La Mancha Sci & Technol Pk, Albacete, Spain
[2] Complejo Hosp Univ Albacete, Serv Salud Castilla La Mancha, Albacete, Spain
[3] Ctr Dis Control & Prevent, Mycot Dis Branch, Atlanta, GA USA
[4] Univ Valencia, Dept Microbiol & Ecol, GMCA Res Unit, Burjassot, Spain
[5] Hlth Res Inst La Fe, Severe Infect Res Grp, Valencia, Spain
[6] Univ Basque Country, UPV EHU, Dept Inmunol Microbiol & Parasitol, Bilbao, Spain
关键词
C. haemulonii complex; Candida; Candida auris; candidosis; PCR identification; yeasts; DESORPTION IONIZATION-TIME; HAEMULONII;
D O I
10.1111/myc.13204
中图分类号
R75 [皮肤病学与性病学];
学科分类号
100206 ;
摘要
Background: The pathogen Candida auris is rapidly gaining clinical importance because of its resistance to antifungal treatments and its persistence in hospital environments. Early and accurate diagnosis of C. auris infections is crucial, and however, the fungus has often been misidentified by commercial systems. Objectives: To develop conventional and real-time PCR methods for accurate and rapid identification of C. auris and its discrimination from closely related species by exploiting the uniqueness of certain glycosylphosphatidylinositol (GPI)-modified protein-encoding genes. Methods: Species-specific primers for two unique putative GPI protein-encoding genes per species were designed for C. auris, C. haemulonii, C. pseudohaemulonii, C. duobushaemulonii, C. lusitaniae and C. albicans. Primers were blind tested for their specificity and efficiency in conventional and real-time multiplex PCR set-up. Results: All primers combinations showed excellent species specificity. In multiplex mode, correct identification was aided by different-sized amplicons for each species. Efficiency of the C. auris primers was validated using a panel of 155 C. auris isolates, including all known genetically diverse clades. In real-time multiplex PCR, different melting points of the amplicons allowed the distinction of C. auris from four related species. C. auris limit of detection was 5 CFU/reaction with a threshold value of 32. The method was also able to detect C. auris in spiked blood and serum. Conclusions: PCR identification based on unique GPI protein-encoding genes allows for accurate and rapid species identification of C. auris and related species without need for expensive equipment when applied in conventional PCR set-up.
引用
收藏
页码:194 / 202
页数:9
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