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LIN28A Modulates Splicing and Gene Expression Programs in Breast Cancer Cells.

Molecular and cellular biology (2015-07-08)
Jun Yang, Brian D Bennett, Shujun Luo, Kaoru Inoue, Sara A Grimm, Gary P Schroth, Pierre R Bushel, H Karimi Kinyamu, Trevor K Archer
ABSTRACT

LIN28 is an evolutionarily conserved RNA-binding protein with critical functions in developmental timing and cancer. However, the molecular mechanisms underlying LIN28's oncogenic properties are yet to be described. RNA-protein immunoprecipitation coupled with genome-wide sequencing (RIP-Seq) analysis revealed significant LIN28 binding within 843 mRNAs in breast cancer cells. Many of the LIN28-bound mRNAs are implicated in the regulation of RNA and cell metabolism. We identify heterogeneous nuclear ribonucleoprotein A1 (hnRNP A1), a protein with multiple roles in mRNA metabolism, as a LIN28-interacting partner. Subsequently, we used a custom computational method to identify differentially spliced gene isoforms in LIN28 and hnRNP A1 small interfering RNA (siRNA)-treated cells. The results reveal that these proteins regulate alternative splicing and steady-state mRNA expression of genes implicated in aspects of breast cancer biology. Notably, cells lacking LIN28 undergo significant isoform switching of the ENAH gene, resulting in a decrease in the expression of the ENAH exon 11a isoform. The expression of ENAH isoform 11a has been shown to be elevated in breast cancers that express HER2. Intriguingly, analysis of publicly available array data from the Cancer Genome Atlas (TCGA) reveals that LIN28 expression in the HER2 subtype is significantly different from that in other breast cancer subtypes. Collectively, our data suggest that LIN28 may regulate splicing and gene expression programs that drive breast cancer subtype phenotypes.

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Cloruro di magnesio, anhydrous, ≥98%
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DL-Dithiothreitol solution, 1 M in H2O
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Glicerolo, ≥99.5%
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Acido formico, puriss., meets analytical specifications of DAC, FCC, 98.0-100%
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