TY - JOUR
T1 - Comparison of Leishmania typing results obtained from 16 European clinical laboratories in 2014
AU - Van der Auwera, Gerard
AU - Bart, Aldert
AU - Chicharro, Carmen
AU - Cortes, Sofia
AU - Davidsson, Leigh
AU - Di Muccio, Trentina
AU - Dujardin, Jean-Claude
AU - Felger, Ingrid
AU - Paglia, Maria Grazia
AU - Grimm, Felix
AU - Harms, Gundel
AU - Jaffe, Charles L
AU - Manser, Monika
AU - Ravel, Christophe
AU - Robert-Gangneux, Florence
AU - Roelfsema, Jeroen
AU - Töz, Seray
AU - Verweij, Jaco J
AU - Chiodini, Peter L
N1 - FTX; DOAJ
PY - 2016
Y1 - 2016
N2 - Leishmaniasis is endemic in southern Europe, and in other European countries cases are diagnosed in travellers who have visited affected areas both within the continent and beyond. Prompt and accurate diagnosis poses a challenge in clinical practice in Europe. Different methods exist for identification of the infecting Leishmania species. Sixteen clinical laboratories in 10 European countries, plus Israel and Turkey, conducted a study to assess their genotyping performance. DNA from 21 promastigote cultures of 13 species was analysed blindly by the routinely used typing method. Five different molecular targets were used, which were analysed with PCR-based methods. Different levels of identification were achieved, and either the Leishmania subgenus, species complex, or actual species were reported. The overall error rate of strains placed in the wrong complex or species was 8.5%. Various reasons for incorrect typing were identified. The study shows there is considerable room for improvement and standardisation of Leishmania typing. The use of well validated standard operating procedures is recommended, covering testing, interpretation, and reporting guidelines. Application of the internal transcribed spacer 1 of the rDNA array should be restricted to Old World samples, while the heat-shock protein 70 gene and the mini-exon can be applied globally.
AB - Leishmaniasis is endemic in southern Europe, and in other European countries cases are diagnosed in travellers who have visited affected areas both within the continent and beyond. Prompt and accurate diagnosis poses a challenge in clinical practice in Europe. Different methods exist for identification of the infecting Leishmania species. Sixteen clinical laboratories in 10 European countries, plus Israel and Turkey, conducted a study to assess their genotyping performance. DNA from 21 promastigote cultures of 13 species was analysed blindly by the routinely used typing method. Five different molecular targets were used, which were analysed with PCR-based methods. Different levels of identification were achieved, and either the Leishmania subgenus, species complex, or actual species were reported. The overall error rate of strains placed in the wrong complex or species was 8.5%. Various reasons for incorrect typing were identified. The study shows there is considerable room for improvement and standardisation of Leishmania typing. The use of well validated standard operating procedures is recommended, covering testing, interpretation, and reporting guidelines. Application of the internal transcribed spacer 1 of the rDNA array should be restricted to Old World samples, while the heat-shock protein 70 gene and the mini-exon can be applied globally.
U2 - 10.2807/1560-7917.ES.2016.21.49.30418
DO - 10.2807/1560-7917.ES.2016.21.49.30418
M3 - A1: Web of Science-article
C2 - 27983510
SN - 1560-7917
VL - 21
SP - 9
EP - 19
JO - Eurosurveillance
JF - Eurosurveillance
IS - 49
M1 - pii=30418
ER -