Transgene silencing and transgene-derived siRNA production in tobacco plants homozygous for an introduced AtMYB90 construct
| dc.contributor.author | Velten, Jeff | |
| dc.contributor.author | Cakir, Cahid | |
| dc.contributor.author | Youn, Eunseog | |
| dc.contributor.author | Chen, Junping | |
| dc.contributor.author | Cazzonelli, Christopher I. | |
| dc.date.accessioned | 2015-10-21T03:00:41Z | |
| dc.date.available | 2015-10-21T03:00:41Z | |
| dc.date.issued | 2012-02-17 | |
| dc.date.updated | 2015-12-09T08:58:47Z | |
| dc.description.abstract | Transgenic tobacco (Nicotiana tabacum) lines were engineered to ectopically over-express AtMYB90 (PAP2), an R2-R3 Myb gene associated with regulation of anthocyanin production in Arabidopsis thaliana. Independently transformed transgenic lines, Myb27 and Myb237, accumulated large quantities of anthocyanin, generating a dark purple phenotype in nearly all tissues. After self-fertilization, some progeny of the Myb27 line displayed an unexpected pigmentation pattern, with most leaves displaying large sectors of dramatically reduced anthocyanin production. The green-sectored 27Hmo plants were all found to be homozygous for the transgene and, despite a doubled transgene dosage, to have reduced levels of AtMYB90 mRNA. The observed reduction in anthocyanin pigmentation and AtMYB90 mRNA was phenotypically identical to the patterns seen in leaves systemically silenced for the AtMYB90 transgene, and was associated with the presence of AtMYB90-derived siRNA homologous to both strands of a portion of the AtMYB90 transcribed region. Activation of transgene silencing in the Myb27 line was triggered when the 35S::AtMYB90 transgene dosage was doubled, in both Myb27 homozygotes, and in plants containing one copy of each of the independently segregating Myb27 and Myb237 transgene loci. Mapping of sequenced siRNA molecules to the Myb27 TDNA (including flanking tobacco sequences) indicated that the 3' half of the AtMYB90 transcript is the primary target for siRNA associated silencing in both homozygous Myb27 plants and in systemically silenced tissues. The transgene within the Myb27 line was found to consist of a single, fully intact, copy of the AtMYB90 construct. Silencing appears to initiate in response to elevated levels of transgene mRNA (or an aberrant product thereof) present within a subset of leaf cells, followed by spread of the resulting small RNA to adjacent leaf tissues and subsequent amplification of siRNA production. | |
| dc.description.sponsorship | Funding for this research is provided by the United States Department of Agriculture. | en_AU |
| dc.identifier.issn | 1932-6203 | en_AU |
| dc.identifier.uri | http://hdl.handle.net/1885/15999 | |
| dc.publisher | Public Library of Science | |
| dc.rights | © This is an open-access article, free of all copyright, and may be freely reproduced, distributed, transmitted, modified, built upon, or otherwise used by anyone for any lawful purpose. The work is made available under the Creative Commons CC0 public domain dedication | |
| dc.source | PLoS ONE | |
| dc.subject | anthocyanins | |
| dc.subject | arabidopsis | |
| dc.subject | arabidopsis proteins | |
| dc.subject | base sequence | |
| dc.subject | dna, bacterial | |
| dc.subject | dna, plant | |
| dc.subject | gene expression regulation, plant | |
| dc.subject | genetic loci | |
| dc.subject | genome, plant | |
| dc.subject | hemizygote | |
| dc.subject | micrornas | |
| dc.subject | molecular sequence data | |
| dc.subject | mutagenesis, insertional | |
| dc.subject | phenotype | |
| dc.subject | pigmentation | |
| dc.subject | plants, genetically modified | |
| dc.subject | rna, messenger | |
| dc.subject | rna, small interfering | |
| dc.subject | tobacco | |
| dc.subject | transcription factors | |
| dc.subject | transcription, genetic | |
| dc.subject | transgenes | |
| dc.subject | gene silencing | |
| dc.subject | homozygote | |
| dc.title | Transgene silencing and transgene-derived siRNA production in tobacco plants homozygous for an introduced AtMYB90 construct | |
| dc.type | Journal article | |
| dcterms.dateAccepted | 2011-12-10 | |
| local.bibliographicCitation.issue | 2 | en_AU |
| local.bibliographicCitation.startpage | e30141 | en_AU |
| local.contributor.affiliation | Velten, Jeff, US Department of Agriculture, United States of America | en_AU |
| local.contributor.affiliation | Cakir, Cahid, US Department of Agriculture, United States of America | en_AU |
| local.contributor.affiliation | youn, Eunseog, Texas Tech University, United States of America | en_AU |
| local.contributor.affiliation | Chen , Junping, United States Department of Agriculture, United States of America | en_AU |
| local.contributor.affiliation | Cazzonelli, Christopher, College of Medicine, Biology and Environment, CMBE Research School of Biology, Division of Plant Sciences, The Australian National University | en_AU |
| local.contributor.authoruid | u4354609 | en_AU |
| local.description.notes | Imported from ARIES | en_AU |
| local.identifier.absfor | 060702 | en_AU |
| local.identifier.absfor | 060405 | en_AU |
| local.identifier.absfor | 060404 | en_AU |
| local.identifier.absseo | 820305 | en_AU |
| local.identifier.ariespublication | u4956746xPUB246 | en_AU |
| local.identifier.citationvolume | 7 | en_AU |
| local.identifier.doi | 10.1371/journal.pone.0030141 | en_AU |
| local.identifier.essn | 1932-6203 | en_AU |
| local.identifier.scopusID | 2-s2.0-84857171447 | |
| local.identifier.thomsonID | 000302853600014 | |
| local.publisher.url | https://www.plos.org/ | en_AU |
| local.type.status | Published Version | en_AU |
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