Identification of a novel long non-coding RNA within RUNX1 intron 5
Abstract Background RUNX1 gene, a master regulator of the hematopoietic process, participates in pathological conditions as a partner for several genes in chromosomal translocations. One of the most frequent chromosomal translocations found in acute myeloid leukemia patients is the t(8;21), in which...
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doaj-ac1b68fd6cf1490992ed862c477f83392020-11-25T03:33:43ZengBMCHuman Genomics1479-73642019-07-011311910.1186/s40246-019-0219-1Identification of a novel long non-coding RNA within RUNX1 intron 5Nicolás Schnake0Marcela Hinojosa1Soraya Gutiérrez2Laboratory of Epigenetics [EpiGene], Departamento de Bioquímica y Biología Molecular, Facultad de Ciencias Biológicas, Universidad de Concepción, Barrio Universitario s/nLaboratory of Epigenetics [EpiGene], Departamento de Bioquímica y Biología Molecular, Facultad de Ciencias Biológicas, Universidad de Concepción, Barrio Universitario s/nLaboratory of Epigenetics [EpiGene], Departamento de Bioquímica y Biología Molecular, Facultad de Ciencias Biológicas, Universidad de Concepción, Barrio Universitario s/nAbstract Background RUNX1 gene, a master regulator of the hematopoietic process, participates in pathological conditions as a partner for several genes in chromosomal translocations. One of the most frequent chromosomal translocations found in acute myeloid leukemia patients is the t(8;21), in which RUNX1 and ETO genes recombine. In RUNX1 gene, the DNA double-strand breaks that originate the t(8;21) are generated in the intron 5, specifically within three regions designated as BCR1, BCR2, and BCR3. To date, what determines that these regions are more susceptible to DNA double-strand breaks is not completely clear. In this report, we characterized RUNX1 intron 5, by analyzing DNase-seq and ChIP-seq data, available in the ENCODE Project server, to evaluate DNaseI hypersensitivity and the presence of the epigenetic mark H3K4me3 in 124 and 51 cell types, respectively. Results Our results show that intron 5 exhibits an epigenetic mark distribution similar to known promoter regions. Moreover, using the online tool YAPP and available CAGE data from the ENCODE Project server, we identified several putative transcription start sites within intron 5 in regions BCR2 and BCR3. Finally, available EST data was analyzed, identifying a novel uncharacterized long non-coding RNA, which is expressed in hematopoietic cell lines as shown by RT-PCR. Our data suggests that the core promoter of the novel long non-coding RNA locates within the region BCR3. Conclusion We identified a novel long non-coding RNA within RUNX1 intron 5, transcribed from a promoter located in the region BCR3, one of the chromosomal breakpoints of RUNX1 gene.http://link.springer.com/article/10.1186/s40246-019-0219-1RUNX1IntronBreakpoint cluster regionPromoterNon-coding RNA |
collection |
DOAJ |
language |
English |
format |
Article |
sources |
DOAJ |
author |
Nicolás Schnake Marcela Hinojosa Soraya Gutiérrez |
spellingShingle |
Nicolás Schnake Marcela Hinojosa Soraya Gutiérrez Identification of a novel long non-coding RNA within RUNX1 intron 5 Human Genomics RUNX1 Intron Breakpoint cluster region Promoter Non-coding RNA |
author_facet |
Nicolás Schnake Marcela Hinojosa Soraya Gutiérrez |
author_sort |
Nicolás Schnake |
title |
Identification of a novel long non-coding RNA within RUNX1 intron 5 |
title_short |
Identification of a novel long non-coding RNA within RUNX1 intron 5 |
title_full |
Identification of a novel long non-coding RNA within RUNX1 intron 5 |
title_fullStr |
Identification of a novel long non-coding RNA within RUNX1 intron 5 |
title_full_unstemmed |
Identification of a novel long non-coding RNA within RUNX1 intron 5 |
title_sort |
identification of a novel long non-coding rna within runx1 intron 5 |
publisher |
BMC |
series |
Human Genomics |
issn |
1479-7364 |
publishDate |
2019-07-01 |
description |
Abstract Background RUNX1 gene, a master regulator of the hematopoietic process, participates in pathological conditions as a partner for several genes in chromosomal translocations. One of the most frequent chromosomal translocations found in acute myeloid leukemia patients is the t(8;21), in which RUNX1 and ETO genes recombine. In RUNX1 gene, the DNA double-strand breaks that originate the t(8;21) are generated in the intron 5, specifically within three regions designated as BCR1, BCR2, and BCR3. To date, what determines that these regions are more susceptible to DNA double-strand breaks is not completely clear. In this report, we characterized RUNX1 intron 5, by analyzing DNase-seq and ChIP-seq data, available in the ENCODE Project server, to evaluate DNaseI hypersensitivity and the presence of the epigenetic mark H3K4me3 in 124 and 51 cell types, respectively. Results Our results show that intron 5 exhibits an epigenetic mark distribution similar to known promoter regions. Moreover, using the online tool YAPP and available CAGE data from the ENCODE Project server, we identified several putative transcription start sites within intron 5 in regions BCR2 and BCR3. Finally, available EST data was analyzed, identifying a novel uncharacterized long non-coding RNA, which is expressed in hematopoietic cell lines as shown by RT-PCR. Our data suggests that the core promoter of the novel long non-coding RNA locates within the region BCR3. Conclusion We identified a novel long non-coding RNA within RUNX1 intron 5, transcribed from a promoter located in the region BCR3, one of the chromosomal breakpoints of RUNX1 gene. |
topic |
RUNX1 Intron Breakpoint cluster region Promoter Non-coding RNA |
url |
http://link.springer.com/article/10.1186/s40246-019-0219-1 |
work_keys_str_mv |
AT nicolasschnake identificationofanovellongnoncodingrnawithinrunx1intron5 AT marcelahinojosa identificationofanovellongnoncodingrnawithinrunx1intron5 AT sorayagutierrez identificationofanovellongnoncodingrnawithinrunx1intron5 |
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