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A Polyphasic Approach to Compare the Genomic Profiles of Aflatoxigenic and Non-Aflatoxigenic Isolates of Aspergillus Section Flavi

Tapani Yli-Mattila; Taha Hussien; Asmaa Abbas

dc.contributor.authorTapani Yli-Mattila
dc.contributor.authorTaha Hussien
dc.contributor.authorAsmaa Abbas
dc.date.accessioned2022-10-28T14:23:50Z
dc.date.available2022-10-28T14:23:50Z
dc.identifier.urihttps://www.utupub.fi/handle/10024/171114
dc.description.abstract<p>Aflatoxins (AF) are highly toxic compounds produced by Aspergillus section Flavi. They<br />spoil food crops and present a serious global health hazard to humans and livestock. The aim of<br />this study was to examine the phylogenetic relationships among aflatoxigenic and non-aflatoxigenic<br />Aspergillus isolates. A polyphasic approach combining phylogenetic, sequence, and toxin analyses was<br />applied to 40 Aspergillus section Flavi isolates collected from eight countries around the world (USA,<br />Philippines, Egypt, India, Australia, Indonesia, China, and Uganda). This allows one to pinpoint the<br />key genomic features that distinguish AF producing and non-producing isolates. Based on molecular<br />identification, 32 (80%) were identified as A. flavus, three (7.5%) as A. parasiticus, three (7.5%) as<br />A. nomius and one (2.5%) as A. tamarii. Toxin analysis showed that 22 (55%) Aspergillus isolates<br />were aflatoxigenic. The majority of the toxic isolates (62.5%) originated from Egypt. The highest<br />aflatoxin production potential was observed in an A. nomius isolate which is originally isolated<br />from the Philippines. DNA-based molecular markers such as random amplified polymorphic DNA<br />(RAPD) and inter-simple sequence repeats (ISSR) were used to evaluate the genetic diversity and<br />phylogenetic relationships among these 40 Aspergillus isolates, which were originally selected from<br />80 isolates. The percentage of polymorphic bands in three RAPD and three ISSR primers was 81.9%<br />and 79.37%, respectively. Analysis of molecular variance showed significant diversity within the<br />populations, 92% for RAPD and 85% for ISSR primers. The average of Polymorphism Information<br />Content (PIC), Marker Index (MI), Nei’s gene diversity (H) and Shannon’s diversity index (I) in ISSR<br />markers are higher than those in RAPD markers. Based on banding patterns and gene diversities<br />values, we observed that the ISSR-PCR provides clearer data and is more successful in genetic<br />diversity analyses than RAPD-PCR. Dendrograms generated from UPGMA (Unweighted Pair Group<br />Method with Arithmetic Mean) cluster analyses for RAPD and ISSR markers were related to the<br />geographic origin.<br /></p>
dc.language.isoen
dc.publisherMDPI
dc.titleA Polyphasic Approach to Compare the Genomic Profiles of Aflatoxigenic and Non-Aflatoxigenic Isolates of Aspergillus Section Flavi
dc.identifier.urlhttps://www.mdpi.com/2072-6651/12/1/56
dc.identifier.urnURN:NBN:fi-fe2021042826371
dc.relation.volume12
dc.contributor.organizationfi=PÄÄT Biokemia|en=PÄÄT Biochemistry|
dc.contributor.organizationfi=mat.-luonn.t. tdk yhteiset|en=Mat.-luonn.t. tdk yhteiset|
dc.contributor.organizationfi=PÄÄT Molekulaarinen kasvibiologia|en=PÄÄT Molecular Plant Biology|
dc.contributor.organization-code2606201
dc.contributor.organization-code2606205
dc.contributor.organization-code2606000
dc.converis.publication-id45183865
dc.converis.urlhttps://research.utu.fi/converis/portal/Publication/45183865
dc.identifier.eissn2072-6651
dc.identifier.jour-issn2072-6651
dc.okm.affiliatedauthorAbbas, Asmaa
dc.okm.affiliatedauthorYli-Mattila, Tapani
dc.okm.discipline1182 Biochemistry, cell and molecular biologyen_GB
dc.okm.discipline1183 Kasvibiologia, mikrobiologia, virologiafi_FI
dc.okm.discipline1172 Environmental sciencesen_GB
dc.okm.discipline1183 Plant biology, microbiology, virologyen_GB
dc.okm.discipline1172 Ympäristötiedefi_FI
dc.okm.discipline1182 Biokemia, solu- ja molekyylibiologiafi_FI
dc.okm.internationalcopublicationinternational co-publication
dc.okm.internationalityInternational publication
dc.okm.typeJournal article
dc.publisher.countrySveitsifi_FI
dc.publisher.countrySwitzerlanden_GB
dc.publisher.country-codeCH
dc.relation.articlenumber56
dc.relation.doi10.3390/toxins12010056
dc.relation.ispartofjournalToxins
dc.relation.issue1
dc.year.issued2020


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