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Screening and chromosome localization of two cotton BAC clones

Abstract. Two (BAC) clones (350B21 and 299N22) of Pima 90-53 cotton [Gossypium barbadense Linnaeus, 1753 (2n=4x=52)] were screened from a BAC library using SSR markers. Strong hybridization signals were detected at terminal regions of all A genome (sub-genome) chromosomes, but were almost absent in...

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Autores principales: Cui, Xinglei, Liu, Fang, Liu, Yuling, Zhou, Zhongli, Wang, Chunying, Yanyan Zhao, Meng, Fei, Wang, Xingxing, Cai, Xiaoyan, Wang, Yuhong, Peng, Renhai, Wang, Kunbo
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Pensoft Publishers 2016
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4856921/
https://www.ncbi.nlm.nih.gov/pubmed/27186333
http://dx.doi.org/10.3897/CompCytogen.v10i1.5304
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author Cui, Xinglei
Liu, Fang
Liu, Yuling
Zhou, Zhongli
Wang, Chunying
Yanyan Zhao,
Meng, Fei
Wang, Xingxing
Cai, Xiaoyan
Wang, Yuhong
Peng, Renhai
Wang, Kunbo
author_facet Cui, Xinglei
Liu, Fang
Liu, Yuling
Zhou, Zhongli
Wang, Chunying
Yanyan Zhao,
Meng, Fei
Wang, Xingxing
Cai, Xiaoyan
Wang, Yuhong
Peng, Renhai
Wang, Kunbo
author_sort Cui, Xinglei
collection PubMed
description Abstract. Two (BAC) clones (350B21 and 299N22) of Pima 90-53 cotton [Gossypium barbadense Linnaeus, 1753 (2n=4x=52)] were screened from a BAC library using SSR markers. Strong hybridization signals were detected at terminal regions of all A genome (sub-genome) chromosomes, but were almost absent in D genome (sub-genome) chromosomes with BAC clone 350B21 as the probe. The results indicate that specific sequences, which only exist at the terminal parts of A genome (sub-genome) chromosomes with a huge repeat number, may be contained in BAC clone 350B21. When utilizing FISH with the BAC clone 299N22 as probe, a pair of obvious signals was detected on chromosome 13 of D genome (sub-genome), while strong dispersed signals were detected on all A genome (sub-genome) chromosomes. The results showed that peculiar repetitive sequence, which was distributed throughout all A genome (sub-genome) chromosomes, may exist in BAC clone 299N22. The absence of the repetitive sequences, which exist in the two BAC clones, in D genome may account for the genome-size variation between A and D genomes. In addition, the microcolinearity analysis of the clone 299N22 and its homologous region on Gossypium raimondii Ulbrich, 1932 chromosome 13 (D(5)13) indicated that the clone 299N22 might come from A sub-genome of sea island cotton (Gossypium barbadense), and a huge number of small deletions, illegitimate recombination, translocation and rearrangements may have occurred during the genus evolution. The two BAC clones studied here can be used as cytological markers but will be also be helpful to research in cotton genome evolution and comparative genomics.
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spelling pubmed-48569212016-05-16 Screening and chromosome localization of two cotton BAC clones Cui, Xinglei Liu, Fang Liu, Yuling Zhou, Zhongli Wang, Chunying Yanyan Zhao, Meng, Fei Wang, Xingxing Cai, Xiaoyan Wang, Yuhong Peng, Renhai Wang, Kunbo Comp Cytogenet Research Articles Abstract. Two (BAC) clones (350B21 and 299N22) of Pima 90-53 cotton [Gossypium barbadense Linnaeus, 1753 (2n=4x=52)] were screened from a BAC library using SSR markers. Strong hybridization signals were detected at terminal regions of all A genome (sub-genome) chromosomes, but were almost absent in D genome (sub-genome) chromosomes with BAC clone 350B21 as the probe. The results indicate that specific sequences, which only exist at the terminal parts of A genome (sub-genome) chromosomes with a huge repeat number, may be contained in BAC clone 350B21. When utilizing FISH with the BAC clone 299N22 as probe, a pair of obvious signals was detected on chromosome 13 of D genome (sub-genome), while strong dispersed signals were detected on all A genome (sub-genome) chromosomes. The results showed that peculiar repetitive sequence, which was distributed throughout all A genome (sub-genome) chromosomes, may exist in BAC clone 299N22. The absence of the repetitive sequences, which exist in the two BAC clones, in D genome may account for the genome-size variation between A and D genomes. In addition, the microcolinearity analysis of the clone 299N22 and its homologous region on Gossypium raimondii Ulbrich, 1932 chromosome 13 (D(5)13) indicated that the clone 299N22 might come from A sub-genome of sea island cotton (Gossypium barbadense), and a huge number of small deletions, illegitimate recombination, translocation and rearrangements may have occurred during the genus evolution. The two BAC clones studied here can be used as cytological markers but will be also be helpful to research in cotton genome evolution and comparative genomics. Pensoft Publishers 2016-01-22 /pmc/articles/PMC4856921/ /pubmed/27186333 http://dx.doi.org/10.3897/CompCytogen.v10i1.5304 Text en Xinglei Cui, Fang Liu, Yuling Liu, Zhongli Zhou, Chunying Wang, Yanyan Zhao, Fei Meng, Xingxing Wang, Xiaoyan Cai, Yuhong Wang, Renhai Peng, Kunbo Wang http://creativecommons.org/licenses/by/4.0 This is an open access article distributed under the terms of the Creative Commons Attribution License (CC BY 4.0), which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
spellingShingle Research Articles
Cui, Xinglei
Liu, Fang
Liu, Yuling
Zhou, Zhongli
Wang, Chunying
Yanyan Zhao,
Meng, Fei
Wang, Xingxing
Cai, Xiaoyan
Wang, Yuhong
Peng, Renhai
Wang, Kunbo
Screening and chromosome localization of two cotton BAC clones
title Screening and chromosome localization of two cotton BAC clones
title_full Screening and chromosome localization of two cotton BAC clones
title_fullStr Screening and chromosome localization of two cotton BAC clones
title_full_unstemmed Screening and chromosome localization of two cotton BAC clones
title_short Screening and chromosome localization of two cotton BAC clones
title_sort screening and chromosome localization of two cotton bac clones
topic Research Articles
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4856921/
https://www.ncbi.nlm.nih.gov/pubmed/27186333
http://dx.doi.org/10.3897/CompCytogen.v10i1.5304
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