CRISPR/Cas9 screen uncovers functional translation of cryptic lncRNA-encoded open reading frames in human cancer
Caishang Zheng, … , Xi Chen, Yiwen Chen
Caishang Zheng, … , Xi Chen, Yiwen Chen
Published March 1, 2023
Citation Information: J Clin Invest. 2023;133(5):e159940. https://doi.org/10.1172/JCI159940.
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Research Article Genetics Oncology

CRISPR/Cas9 screen uncovers functional translation of cryptic lncRNA-encoded open reading frames in human cancer

Abstract

Emerging evidence suggests that cryptic translation within long noncoding RNAs (lncRNAs) may produce novel proteins with important developmental/physiological functions. However, the role of this cryptic translation in complex diseases (e.g., cancer) remains elusive. Here, we applied an integrative strategy combining ribosome profiling and CRISPR/Cas9 screening with large-scale analysis of molecular/clinical data for breast cancer (BC) and identified estrogen receptor α–positive (ER+) BC dependency on the cryptic ORFs encoded by lncRNA genes that were upregulated in luminal tumors. We confirmed the in vivo tumor-promoting function of an unannotated protein, GATA3-interacting cryptic protein (GT3-INCP) encoded by LINC00992, the expression of which was associated with poor prognosis in luminal tumors. GTE-INCP was upregulated by estrogen/ER and regulated estrogen-dependent cell growth. Mechanistically, GT3-INCP interacted with GATA3, a master transcription factor key to mammary gland development/BC cell proliferation, and coregulated a gene expression program that involved many BC susceptibility/risk genes and impacted estrogen response/cell proliferation. GT3-INCP/GATA3 bound to common cis regulatory elements and upregulated the expression of the tumor-promoting and estrogen-regulated BC susceptibility/risk genes MYB and PDZK1. Our study indicates that cryptic lncRNA-encoded proteins can be an important integrated component of the master transcriptional regulatory network driving aberrant transcription in cancer, and suggests that the “hidden” lncRNA-encoded proteome might be a new space for therapeutic target discovery.

Authors

Caishang Zheng, Yanjun Wei, Peng Zhang, Longyong Xu, Zhenzhen Zhang, Kangyu Lin, Jiakai Hou, Xiangdong Lv, Yao Ding, Yulun Chiu, Antrix Jain, Nelufa Islam, Anna Malovannaya, Yun Wu, Feng Ding, Han Xu, Ming Sun, Xi Chen, Yiwen Chen

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Figure 7

GT3-INCP and GATA3 upregulate MYB and PDZK1 expression.

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GT3-INCP and GATA3 upregulate MYB and PDZK1 expression. (A) Workflow for...
(A) Workflow for identifying the protein-coding genes co-upregulated by GT3-INCP and GATA3 and upregulated in luminal A BC compared with normal breast tissue. (B) Workflow for identifying the key targets that were potentially important for mediating the tumor-promoting function of the GT3-INCP/GATA3 axis in ER+ luminal BC. Venn diagram showing the overlap between the protein-coding genes that were co-upregulated by GT3-INCP/GATA3 and upregulated in luminal BC tumors, and the genes that harbored common GT3-INCP/GATA3 binding site(s). qRT-PCR analysis showing MYB and PDZK1 expression changes in MCF7 cells following (C) GATA3 knockdown or (D) GT3-INCP knockout. (E) Upon LINC00992 knockdown, the rescue effect of ectopic expression of the wild-type or mutant GT3-INCP (Del-M8 or AGG mutation in start codon), with respect to the empty vector control (EV), on MYB and PDZK1 mRNA expression was assessed by qRT-PCR in MCF7 cells. Fisher’s exact test was used to assess the statistical significance of the Venn diagram overlap (B). Data in CE are shown as mean ± SD (n = 3). **P < 0.01 by 1-way ANOVA with Dunnett’s multiple-comparison test. NS, not significant (P > 0.05).