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Differential response of cassava genotypes to infection by cassava mosaic geminiviruses

Mitigation of cassava mosaic disease (CMD) focuses on the introgression of resistance imparted by the polygenic recessive (CMD1), dominant monogenic (CMD2) and CMD3 loci. The mechanism(s) of resistance they impart, however, remain unknown. Two CMD susceptible and nine CMD resistant cassava genotypes...

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Autores principales: Kuria, Paul, Ilyas, Muhammad, Ateka, Elijah, Miano, Douglas, Onguso, Justus, Carrington, James C., Taylor, Nigel J.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Elsevier Science 2017
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5130204/
https://www.ncbi.nlm.nih.gov/pubmed/27693919
http://dx.doi.org/10.1016/j.virusres.2016.09.022
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author Kuria, Paul
Ilyas, Muhammad
Ateka, Elijah
Miano, Douglas
Onguso, Justus
Carrington, James C.
Taylor, Nigel J.
author_facet Kuria, Paul
Ilyas, Muhammad
Ateka, Elijah
Miano, Douglas
Onguso, Justus
Carrington, James C.
Taylor, Nigel J.
author_sort Kuria, Paul
collection PubMed
description Mitigation of cassava mosaic disease (CMD) focuses on the introgression of resistance imparted by the polygenic recessive (CMD1), dominant monogenic (CMD2) and CMD3 loci. The mechanism(s) of resistance they impart, however, remain unknown. Two CMD susceptible and nine CMD resistant cassava genotypes were inoculated by microparticle bombardment with infectious clones of African cassava mosaic virus Cameroon strain (ACMV-CM) and the Kenyan strain K201 of East African cassava mosaic virus (EACMV KE2 [K201]). Genotypes carrying the CMD1 (TMS 30572), CMD2 (TME 3, TME 204 and Oko-iyawo) and CMD3 (TMS 97/0505) resistance mechanisms showed high levels of resistance to ACMV-CM, with viral DNA undetectable by PCR beyond 7 days post inoculation (dpi). In contrast, all genotypes initially developed severe CMD symptoms and accumulated high virus titers after inoculation with EACMV KE2 (K201). Resistant genotypes recovered to become asymptomatic by 65 dpi with no detectable virus in newly formed leaves. Genotype TMS 97/2205 showed highest resistance to EACMV KE2 (K201) with <30% of inoculated plants developing symptoms followed by complete recovery by 35 dpi. Deep sequencing of small RNAs confirmed production of 21–24 nt virus derived small RNAs (vsRNA) that mapped to cover the entire ACMV-CM and EACMV KE2 (K201) viral genomes in both polarities, with hotspots seen within gene coding regions. In resistant genotypes, total vsRNAs were most abundant at 20 and 35 dpi but reduced significantly upon recovery from CMD. In contrast, CMD susceptible genotypes displayed abundant vsRNAs throughout the experimental period. The percentage of vsRNAs reads ranked by class size were 21nt (45%), 22 nt (28%) and 24 nt (18%) in all genotypes studied. The number of vsRNA reads directly correlated with virus titer and CMD symptoms.
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spelling pubmed-51302042017-01-02 Differential response of cassava genotypes to infection by cassava mosaic geminiviruses Kuria, Paul Ilyas, Muhammad Ateka, Elijah Miano, Douglas Onguso, Justus Carrington, James C. Taylor, Nigel J. Virus Res Article Mitigation of cassava mosaic disease (CMD) focuses on the introgression of resistance imparted by the polygenic recessive (CMD1), dominant monogenic (CMD2) and CMD3 loci. The mechanism(s) of resistance they impart, however, remain unknown. Two CMD susceptible and nine CMD resistant cassava genotypes were inoculated by microparticle bombardment with infectious clones of African cassava mosaic virus Cameroon strain (ACMV-CM) and the Kenyan strain K201 of East African cassava mosaic virus (EACMV KE2 [K201]). Genotypes carrying the CMD1 (TMS 30572), CMD2 (TME 3, TME 204 and Oko-iyawo) and CMD3 (TMS 97/0505) resistance mechanisms showed high levels of resistance to ACMV-CM, with viral DNA undetectable by PCR beyond 7 days post inoculation (dpi). In contrast, all genotypes initially developed severe CMD symptoms and accumulated high virus titers after inoculation with EACMV KE2 (K201). Resistant genotypes recovered to become asymptomatic by 65 dpi with no detectable virus in newly formed leaves. Genotype TMS 97/2205 showed highest resistance to EACMV KE2 (K201) with <30% of inoculated plants developing symptoms followed by complete recovery by 35 dpi. Deep sequencing of small RNAs confirmed production of 21–24 nt virus derived small RNAs (vsRNA) that mapped to cover the entire ACMV-CM and EACMV KE2 (K201) viral genomes in both polarities, with hotspots seen within gene coding regions. In resistant genotypes, total vsRNAs were most abundant at 20 and 35 dpi but reduced significantly upon recovery from CMD. In contrast, CMD susceptible genotypes displayed abundant vsRNAs throughout the experimental period. The percentage of vsRNAs reads ranked by class size were 21nt (45%), 22 nt (28%) and 24 nt (18%) in all genotypes studied. The number of vsRNA reads directly correlated with virus titer and CMD symptoms. Elsevier Science 2017-01-02 /pmc/articles/PMC5130204/ /pubmed/27693919 http://dx.doi.org/10.1016/j.virusres.2016.09.022 Text en © 2016 The Authors http://creativecommons.org/licenses/by/4.0/ This is an open access article under the CC BY license (http://creativecommons.org/licenses/by/4.0/).
spellingShingle Article
Kuria, Paul
Ilyas, Muhammad
Ateka, Elijah
Miano, Douglas
Onguso, Justus
Carrington, James C.
Taylor, Nigel J.
Differential response of cassava genotypes to infection by cassava mosaic geminiviruses
title Differential response of cassava genotypes to infection by cassava mosaic geminiviruses
title_full Differential response of cassava genotypes to infection by cassava mosaic geminiviruses
title_fullStr Differential response of cassava genotypes to infection by cassava mosaic geminiviruses
title_full_unstemmed Differential response of cassava genotypes to infection by cassava mosaic geminiviruses
title_short Differential response of cassava genotypes to infection by cassava mosaic geminiviruses
title_sort differential response of cassava genotypes to infection by cassava mosaic geminiviruses
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5130204/
https://www.ncbi.nlm.nih.gov/pubmed/27693919
http://dx.doi.org/10.1016/j.virusres.2016.09.022
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