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Survey of Apple Mosaic Virus in Apple-Growing Provinces of East Anatolia (Malatya and Van) by Rna Probe Hybridization Assay and Rt-Pcr

dc.authorscopusid 55859813300
dc.authorscopusid 13611411000
dc.authorscopusid 15830471300
dc.authorwosid Usta, Mustafa/Cag-7521-2022
dc.authorwosid Sipahioglu, Hikmet/Aaa-6085-2020
dc.contributor.author Korkmaz, Gulustan
dc.contributor.author Sipahioglu, Hikmet Murat
dc.contributor.author Usta, Mustafa
dc.date.accessioned 2025-05-10T16:48:09Z
dc.date.available 2025-05-10T16:48:09Z
dc.date.issued 2013
dc.department T.C. Van Yüzüncü Yıl Üniversitesi en_US
dc.department-temp [Korkmaz, Gulustan] Minist Agr, Rural Affairs Van, Dept Plant Protect, Van, Turkey; [Sipahioglu, Hikmet Murat; Usta, Mustafa] Yuzuncu Yil Univ, Fac Agr, Dept Plant Protect, Van, Turkey en_US
dc.description.abstract Two main apple growing provinces (Van and Malatya) of East Anatolia were surveyed for the presence of the Apple mosaic virus (ApMV). Dot-blot hybridization and RT-PCR tests were implemented to investigate the incidence of ApMV, testing a total of 481 samples collected from commercial apple orchards. Digoxigenin-labeled RNA probes of the ApMV were synthesized from the cloned PCR products and applied in dot-blot hybridization to detect the virus in RNA extracts isolated from fresh leaf tissues. A validated RNA probe (dot-blot) hybridization method was adopted to investigate the presence of ApMV infections in the apple orchards of East Anatolia. In order to determine the most suitable mass extraction methods and to ascertain the presence of virus, 3 RNA preparation procedures (QIAGEN RNA extraction kit, silica capture, and citric buffer) were tested. Among the tested extraction methods, silica capture was determined as the most suitable extraction method for dot-blot hybridization assays. ApMV was found in the surveyed locations with an average incidence of 0.8%. The infected trees showed apparent disease symptoms on the leaves of apple trees. The coat protein (CP) genes of 2 viral isolates selected from Malatya (ApMV-G and ApMV-M) were cloned and their complete nucleotide sequences and deduced amino acids were determined (GenBank acc. nos. JX155668 and JX155669). The CP cistron of the ApMV-G and M isolates contained 224 amino acid residues. Phylogenetic trees based on nucleic acid sequences were constructed by the neighbor-joining and the unweighted pair-group mean arithmetic methods with 100 bootstrap replicates. The CP sequence of ApMV-G and ApMV-M varied among the 21 isolates, with overall identity ranging from 88% to 99% and ranging from 91% to 99% at the nucleotide level. en_US
dc.description.sponsorship Yuzuncu Yil University [2009-FBE-YL019] en_US
dc.description.sponsorship This study was a part of the MSc study of Gulustan Korkmaz and was supported by a grant from the Research Fund of Yuzuncu Yil University (Project No.: 2009-FBE-YL019). en_US
dc.description.woscitationindex Science Citation Index Expanded
dc.identifier.doi 10.3906/tar-1212-5
dc.identifier.endpage 718 en_US
dc.identifier.issn 1300-011X
dc.identifier.issn 1303-6173
dc.identifier.issue 6 en_US
dc.identifier.scopus 2-s2.0-84884368495
dc.identifier.scopusquality Q2
dc.identifier.startpage 711 en_US
dc.identifier.uri https://doi.org/10.3906/tar-1212-5
dc.identifier.uri https://hdl.handle.net/20.500.14720/1470
dc.identifier.volume 37 en_US
dc.identifier.wos WOS:000324574800006
dc.identifier.wosquality Q1
dc.language.iso en en_US
dc.publisher Tubitak Scientific & Technological Research Council Turkey en_US
dc.relation.publicationcategory Makale - Uluslararası Hakemli Dergi - Kurum Öğretim Elemanı en_US
dc.rights info:eu-repo/semantics/openAccess en_US
dc.subject Apple Mosaic Virus en_US
dc.subject Eastern Anatolia en_US
dc.subject Molecular Hybridization en_US
dc.subject Rt-Pcr en_US
dc.subject Survey en_US
dc.title Survey of Apple Mosaic Virus in Apple-Growing Provinces of East Anatolia (Malatya and Van) by Rna Probe Hybridization Assay and Rt-Pcr en_US
dc.type Article en_US

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