Molecular tracking of Acidovorax citrulli: Unveiling pathogen dynamics and blotch disease outbreaks through specific markers-Reference-Cited by-同舟云学术

Molecular tracking of Acidovorax citrulli: Unveiling pathogen dynamics and blotch disease outbreaks through specific markers

Published:2024 Issue:1 Volume:56 Page:169-185
ISSN:0534-0012
Container-title:Genetika
language:en
Short-container-title:Genetika

Author:

Silme Ragıp¹^ORCID,Zerbo Marcello²^ORCID,Mercati Francesco²^ORCID,Karataş Ali³^ORCID,Baştaş Kubilay⁴^ORCID,Carimi Francesco²^ORCID,Baysal Ömür⁵^ORCID

Affiliation:

1. Center for Research and Practice in Biotechnology and Genetic Engineering, Istanbul University, Fatih-Istanbul, Türkiye

2. National Research Council, Institute of Biosciences and Bioresources (IBBR), Palermo, Italy

3. Biological Control Research Institute, Kışla Street, Yüreğir/Adana, Türkiye

4. Selçuk University, Faculty of Agriculture, Department of Plant Protection, Konya, Türkiye

5. Muğla Sıtkı Koçman University, Faculty of Science, Department of Molecular Biology and Genetics, Molecular Microbiology Unit, Kötekli-Muğla, Türkiye + Molecular Plant and Microbial Biosciences Research Unit (MPMB-RU), University of Worcester, Henwick Grove, Worcester, WR AJ, United Kingdom

Abstract

Acidovorax citrulli (Ac), a gram-negative bacterium, is the causal agent of bacterial fruit blotch (BFB), which poses a significant threat to cucurbit crop production worldwide. Understanding the genetic diversity of Ac is crucial for identifying sources of resistance and implementing effective disease management strategies. In this study, we conducted the first genetic characterization of Ac strains collected in Turkey using Inter-Simple Sequence Repeat (ISSR) markers. These markers were selected based on repetitive domains mapped on the complete reference genome sequence of Acidovorax citrulli strain NWB SC196. The identity of the Turkish strains was confirmed through molecular (PCR) and serological (Immunofluorescence test and ELISA) methods, while the selected ISSRs, which exhibited similarity to flanked regions in the pathogen's whole genome sequence, were employed to assess the genetic diversity among Ac strains. We compared the profiles of Turkish strains with those of a collection of Ac strains from various countries, including the US, to explore a possible common origin. Specifically, we considered the dissemination of these strains through rootstocks used for grafted seedling production (Cucurbita maxima ? Cucurbita moschata). The results demonstrated a shared genetic profile, suggesting a potential link between Ac strains collected in Turkey and foreign strains. The Mauve analysis, utilizing whole genome sequences of various Ac strains available in the NCBI database, displayed similar clustering patterns to those obtained using our selected molecular markers, confirming the discriminatory efficiency of our method. Based on the high discriminatory power of the selected markers, our proposed method offers a rapid and straightforward approach for genetic analysis of intraspecific variation and monitoring Ac gene flow across countries. The characterized strains and markers presented in this study serve as valuable resources and reference materials for further genetic investigations and tracking contamination sources associated with Ac.

Publisher

National Library of Serbia

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