BALR-6 regulates cell growth and cell survival in B-lymphoblastic leukemia

Norma I. Rodríguez-Malavé; Thilini R. Fernando; Parth C. Patel; Jorge R. Contreras; Jayanth Kumar Palanichamy; Tiffany M. Tran; Jaime Anguiano; Michael J. Davoren; Michael O. Alberti; Kimanh T. Pioli; Salemiz Sandoval; Gay M. Crooks; Dinesh S. Rao

doi:10.1186/s12943-015-0485-z

BALR-6 regulates cell growth and cell survival in B-lymphoblastic leukemia

Norma I. Rodríguez-Malavé
, Thilini R. Fernando
, Parth C. Patel
, Jorge R. Contreras
, Jayanth Kumar Palanichamy
, Tiffany M. Tran
, Jaime Anguiano
, Michael J. Davoren
, Michael O. Alberti
, Kimanh T. Pioli
, Salemiz Sandoval
, Gay M. Crooks
, Dinesh S. Rao

Division of Anatomic and Molecular Pathology (AMP)

Research output: Contribution to journal › Article › peer-review

32 Scopus citations

Abstract

Background: A new class of non-coding RNAs, known as long non-coding RNAs (lncRNAs), has been recently described. These lncRNAs are implicated to play pivotal roles in various molecular processes, including development and oncogenesis. Gene expression profiling of human B-ALL samples showed differential lncRNA expression in samples with particular cytogenetic abnormalities. One of the most promising lncRNAs identified, designated B-ALL associated long RNA-6 (BALR-6), had the highest expression in patient samples carrying the MLL rearrangement, and is the focus of this study. Results: Here, we performed a series of experiments to define the function of BALR-6, including several novel splice forms that we identified. Functionally, siRNA-mediated knockdown of BALR-6 in human B-ALL cell lines caused reduced cell proliferation and increased cell death. Conversely, overexpression of BALR-6 isoforms in both human and mouse cell lines caused increased proliferation and decreased apoptosis. Overexpression of BALR-6 in murine bone marrow transplantation experiments caused a significant increase in early hematopoietic progenitor populations, suggesting that its dysregulation may cause developmental changes. Notably, the knockdown of BALR-6 resulted in global dysregulation of gene expression. The gene set was enriched for leukemia-associated genes, as well as for the transcriptome regulated by Specificity Protein 1 (SP1). We confirmed changes in the expression of SP1, as well as its known interactor and downstream target CREB1. Luciferase reporter assays demonstrated an enhancement of SP1-mediated transcription in the presence of BALR-6. These data provide a putative mechanism for regulation by BALR-6 in B-ALL. Conclusions: Our findings support a role for the novel lncRNA BALR-6 in promoting cell survival in B-ALL. Furthermore, this lncRNA influences gene expression in B-ALL in a manner consistent with a function in transcriptional regulation. Specifically, our findings suggest that BALR-6 expression regulates the transcriptome downstream of SP1, and that this may underlie the function of BALR-6 in B-ALL.

Original language	English
Article number	214
Journal	Molecular Cancer
Volume	14
Issue number	1
DOIs	https://doi.org/10.1186/s12943-015-0485-z
State	Published - Dec 22 2015

Keywords

B-ALL
Leukemia
LncRNA
MLL
Microarray
Non-coding RNA
RNA
SP1

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10.1186/s12943-015-0485-z

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Rodríguez-Malavé, N. I., Fernando, T. R., Patel, P. C., Contreras, J. R., Palanichamy, J. K., Tran, T. M., Anguiano, J., Davoren, M. J., Alberti, M. O., Pioli, K. T., Sandoval, S., Crooks, G. M., & Rao, D. S. (2015). BALR-6 regulates cell growth and cell survival in B-lymphoblastic leukemia. Molecular Cancer, 14(1), Article 214. https://doi.org/10.1186/s12943-015-0485-z

@article{2b286be1eb6545c19ebff1215ae9f3b3,

title = "BALR-6 regulates cell growth and cell survival in B-lymphoblastic leukemia",

abstract = "Background: A new class of non-coding RNAs, known as long non-coding RNAs (lncRNAs), has been recently described. These lncRNAs are implicated to play pivotal roles in various molecular processes, including development and oncogenesis. Gene expression profiling of human B-ALL samples showed differential lncRNA expression in samples with particular cytogenetic abnormalities. One of the most promising lncRNAs identified, designated B-ALL associated long RNA-6 (BALR-6), had the highest expression in patient samples carrying the MLL rearrangement, and is the focus of this study. Results: Here, we performed a series of experiments to define the function of BALR-6, including several novel splice forms that we identified. Functionally, siRNA-mediated knockdown of BALR-6 in human B-ALL cell lines caused reduced cell proliferation and increased cell death. Conversely, overexpression of BALR-6 isoforms in both human and mouse cell lines caused increased proliferation and decreased apoptosis. Overexpression of BALR-6 in murine bone marrow transplantation experiments caused a significant increase in early hematopoietic progenitor populations, suggesting that its dysregulation may cause developmental changes. Notably, the knockdown of BALR-6 resulted in global dysregulation of gene expression. The gene set was enriched for leukemia-associated genes, as well as for the transcriptome regulated by Specificity Protein 1 (SP1). We confirmed changes in the expression of SP1, as well as its known interactor and downstream target CREB1. Luciferase reporter assays demonstrated an enhancement of SP1-mediated transcription in the presence of BALR-6. These data provide a putative mechanism for regulation by BALR-6 in B-ALL. Conclusions: Our findings support a role for the novel lncRNA BALR-6 in promoting cell survival in B-ALL. Furthermore, this lncRNA influences gene expression in B-ALL in a manner consistent with a function in transcriptional regulation. Specifically, our findings suggest that BALR-6 expression regulates the transcriptome downstream of SP1, and that this may underlie the function of BALR-6 in B-ALL.",

keywords = "B-ALL, Leukemia, LncRNA, MLL, Microarray, Non-coding RNA, RNA, SP1",

author = "Rodr{\'i}guez-Malav{\'e}, \{Norma I.\} and Fernando, \{Thilini R.\} and Patel, \{Parth C.\} and Contreras, \{Jorge R.\} and Palanichamy, \{Jayanth Kumar\} and Tran, \{Tiffany M.\} and Jaime Anguiano and Davoren, \{Michael J.\} and Alberti, \{Michael O.\} and Pioli, \{Kimanh T.\} and Salemiz Sandoval and Crooks, \{Gay M.\} and Rao, \{Dinesh S.\}",

note = "Publisher Copyright: {\textcopyright} 2015 Rodr{\'i}guez-Malav{\'e} et al.",

year = "2015",

month = dec,

day = "22",

doi = "10.1186/s12943-015-0485-z",

language = "English",

volume = "14",

journal = "Molecular Cancer",

issn = "1476-4598",

number = "1",

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TY - JOUR

T1 - BALR-6 regulates cell growth and cell survival in B-lymphoblastic leukemia

AU - Rodríguez-Malavé, Norma I.

AU - Fernando, Thilini R.

AU - Patel, Parth C.

AU - Contreras, Jorge R.

AU - Palanichamy, Jayanth Kumar

AU - Tran, Tiffany M.

AU - Anguiano, Jaime

AU - Davoren, Michael J.

AU - Alberti, Michael O.

AU - Pioli, Kimanh T.

AU - Sandoval, Salemiz

AU - Crooks, Gay M.

AU - Rao, Dinesh S.

PY - 2015/12/22

Y1 - 2015/12/22

N2 - Background: A new class of non-coding RNAs, known as long non-coding RNAs (lncRNAs), has been recently described. These lncRNAs are implicated to play pivotal roles in various molecular processes, including development and oncogenesis. Gene expression profiling of human B-ALL samples showed differential lncRNA expression in samples with particular cytogenetic abnormalities. One of the most promising lncRNAs identified, designated B-ALL associated long RNA-6 (BALR-6), had the highest expression in patient samples carrying the MLL rearrangement, and is the focus of this study. Results: Here, we performed a series of experiments to define the function of BALR-6, including several novel splice forms that we identified. Functionally, siRNA-mediated knockdown of BALR-6 in human B-ALL cell lines caused reduced cell proliferation and increased cell death. Conversely, overexpression of BALR-6 isoforms in both human and mouse cell lines caused increased proliferation and decreased apoptosis. Overexpression of BALR-6 in murine bone marrow transplantation experiments caused a significant increase in early hematopoietic progenitor populations, suggesting that its dysregulation may cause developmental changes. Notably, the knockdown of BALR-6 resulted in global dysregulation of gene expression. The gene set was enriched for leukemia-associated genes, as well as for the transcriptome regulated by Specificity Protein 1 (SP1). We confirmed changes in the expression of SP1, as well as its known interactor and downstream target CREB1. Luciferase reporter assays demonstrated an enhancement of SP1-mediated transcription in the presence of BALR-6. These data provide a putative mechanism for regulation by BALR-6 in B-ALL. Conclusions: Our findings support a role for the novel lncRNA BALR-6 in promoting cell survival in B-ALL. Furthermore, this lncRNA influences gene expression in B-ALL in a manner consistent with a function in transcriptional regulation. Specifically, our findings suggest that BALR-6 expression regulates the transcriptome downstream of SP1, and that this may underlie the function of BALR-6 in B-ALL.

AB - Background: A new class of non-coding RNAs, known as long non-coding RNAs (lncRNAs), has been recently described. These lncRNAs are implicated to play pivotal roles in various molecular processes, including development and oncogenesis. Gene expression profiling of human B-ALL samples showed differential lncRNA expression in samples with particular cytogenetic abnormalities. One of the most promising lncRNAs identified, designated B-ALL associated long RNA-6 (BALR-6), had the highest expression in patient samples carrying the MLL rearrangement, and is the focus of this study. Results: Here, we performed a series of experiments to define the function of BALR-6, including several novel splice forms that we identified. Functionally, siRNA-mediated knockdown of BALR-6 in human B-ALL cell lines caused reduced cell proliferation and increased cell death. Conversely, overexpression of BALR-6 isoforms in both human and mouse cell lines caused increased proliferation and decreased apoptosis. Overexpression of BALR-6 in murine bone marrow transplantation experiments caused a significant increase in early hematopoietic progenitor populations, suggesting that its dysregulation may cause developmental changes. Notably, the knockdown of BALR-6 resulted in global dysregulation of gene expression. The gene set was enriched for leukemia-associated genes, as well as for the transcriptome regulated by Specificity Protein 1 (SP1). We confirmed changes in the expression of SP1, as well as its known interactor and downstream target CREB1. Luciferase reporter assays demonstrated an enhancement of SP1-mediated transcription in the presence of BALR-6. These data provide a putative mechanism for regulation by BALR-6 in B-ALL. Conclusions: Our findings support a role for the novel lncRNA BALR-6 in promoting cell survival in B-ALL. Furthermore, this lncRNA influences gene expression in B-ALL in a manner consistent with a function in transcriptional regulation. Specifically, our findings suggest that BALR-6 expression regulates the transcriptome downstream of SP1, and that this may underlie the function of BALR-6 in B-ALL.

KW - B-ALL

KW - Leukemia

KW - LncRNA

KW - MLL

KW - Microarray

KW - Non-coding RNA

KW - RNA

KW - SP1

UR - https://www.scopus.com/pages/publications/84951803963

U2 - 10.1186/s12943-015-0485-z

DO - 10.1186/s12943-015-0485-z

M3 - Article

C2 - 26694754

AN - SCOPUS:84951803963

SN - 1476-4598

VL - 14

JO - Molecular Cancer

JF - Molecular Cancer

IS - 1

M1 - 214

ER -

BALR-6 regulates cell growth and cell survival in B-lymphoblastic leukemia

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Keywords

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