TY - JOUR
T1 - ATP citrate lyase 1 (acl1) gene-based loop-mediated amplification assay for the detection of the Fusarium tricinctum species complex in pure cultures and in cereal samples
AU - Niessen, Ludwig
AU - Gräfenhan, Tom
AU - Vogel, Rudi F.
N1 - Funding Information:
This work was financially supported by grant R416 from the Wissenschaftsförderung der Deutschen Brauwirtschaft e.V., Berlin, Germany . We thank Daniela Buchner, Karolina Müller and Jana Violetta Kolew for technical assistance. We are grateful to the curators of the BBA (Julius-Kühn-Institute, Berlin, Germany), CBS (Centraalbureau voor Schimmelcultures, Utrecht, The Netherlands), DAOM (Canadian National Mycological Herbarium and Culture Collection, AAFC, Ottawa, Ontario, Canada) and TMW (Technische Mikrobiologie Weihenstephan, Freising, Germany) culture collections for providing and preserving cultures for our study.
PY - 2012/9/3
Y1 - 2012/9/3
N2 - The combined data set of the acl1 and tef-1α gene sequences of 61 fungal strains assigned to Fusarium tricinctum, Fusarium avenaceum, Fusarium acuminatum, Fusarium arthrosporioides, Fusarium flocciferum and Fusarium torulosum were used to study the phylogenetic relations between taxa. F. tricinctum, F. acuminatum and F. avenaceum formed distinct clades. Members of the F. tricinctum/. F. acuminatum clade fall into three well supported lineages, of which the largest includes the epitype of F. tricinctum. Loop-mediated isothermal amplification (LAMP) was used to amplify a 167. bp portion of the acl1 gene in F. tricinctum (Corda) Saccardo. DNA amplification was detected in-tube by indirect calcein fluorescence under black light after 60. min of incubation at 65.5 °C. The assay had a detection limit of 0.95. pg of purified genomic DNA of F. tricinctum CBS 410.86 per reaction, corresponding to ca. 18 genomic copies of the acl1 gene. Specificity of the assay was tested using purified DNA from 67 species and subspecies of Fusarium as well as 50 species comprising 22 genera of other filamentous fungi and yeasts. The assay detected 21 of the 23 F. tricinctum strains tested. Cross reactivity was observed with eight out of 13 strains in F. acuminatum but with none of 17 F. avenaceum strains tested. Specificity was further confirmed by conventional PCR with primers designed from the same gene. Detection of F. tricinctum from culture scrapings directly added to the reaction master mix, in DNA extracts from wheat, in single barley grains or in washings of bulk grain samples are proposed as possible applications showing the suitability of the method for food analysis. Finally it was demonstrated that the LAMP reaction can be run using simple lab equipment such as a heating block, water bath, hybridization oven or household equipment, e.g. a microwave oven.
AB - The combined data set of the acl1 and tef-1α gene sequences of 61 fungal strains assigned to Fusarium tricinctum, Fusarium avenaceum, Fusarium acuminatum, Fusarium arthrosporioides, Fusarium flocciferum and Fusarium torulosum were used to study the phylogenetic relations between taxa. F. tricinctum, F. acuminatum and F. avenaceum formed distinct clades. Members of the F. tricinctum/. F. acuminatum clade fall into three well supported lineages, of which the largest includes the epitype of F. tricinctum. Loop-mediated isothermal amplification (LAMP) was used to amplify a 167. bp portion of the acl1 gene in F. tricinctum (Corda) Saccardo. DNA amplification was detected in-tube by indirect calcein fluorescence under black light after 60. min of incubation at 65.5 °C. The assay had a detection limit of 0.95. pg of purified genomic DNA of F. tricinctum CBS 410.86 per reaction, corresponding to ca. 18 genomic copies of the acl1 gene. Specificity of the assay was tested using purified DNA from 67 species and subspecies of Fusarium as well as 50 species comprising 22 genera of other filamentous fungi and yeasts. The assay detected 21 of the 23 F. tricinctum strains tested. Cross reactivity was observed with eight out of 13 strains in F. acuminatum but with none of 17 F. avenaceum strains tested. Specificity was further confirmed by conventional PCR with primers designed from the same gene. Detection of F. tricinctum from culture scrapings directly added to the reaction master mix, in DNA extracts from wheat, in single barley grains or in washings of bulk grain samples are proposed as possible applications showing the suitability of the method for food analysis. Finally it was demonstrated that the LAMP reaction can be run using simple lab equipment such as a heating block, water bath, hybridization oven or household equipment, e.g. a microwave oven.
KW - Acl1
KW - Cereals
KW - Detection
KW - F. tricinctum
KW - LAMP
KW - Taxonomy
UR - http://www.scopus.com/inward/record.url?scp=84865560843&partnerID=8YFLogxK
U2 - 10.1016/j.ijfoodmicro.2012.06.021
DO - 10.1016/j.ijfoodmicro.2012.06.021
M3 - Article
C2 - 22867849
AN - SCOPUS:84865560843
SN - 0168-1605
VL - 158
SP - 171
EP - 185
JO - International Journal of Food Microbiology
JF - International Journal of Food Microbiology
IS - 3
ER -