Abstract
Most lncRNAs display species-specific expression patterns suggesting that animal models of cancer may only incompletely recapitulate the regulatory crosstalk between lncRNAs and oncogenic pathways in humans. Among these pathways, Sonic Hedgehog (SHH) signaling is aberrantly activated in several human cancer entities. We unravel that aberrant expression of the primate-specific lncRNA HedgeHog Interacting Protein-AntiSense 1 (HHIP-AS1) is a hallmark of SHH-driven tumors including medulloblastoma and atypical teratoid/rhabdoid tumors. HHIP-AS1 is actively transcribed from a bidirectional promoter shared with SHH regulator HHIP. Knockdown of HHIP-AS1 induces mitotic spindle deregulation impairing tumorigenicity in vitro and in vivo. Mechanistically, HHIP-AS1 binds directly to the mRNA of cytoplasmic dynein 1 intermediate chain 2 (DYNC1I2) and attenuates its degradation by hsa-miR-425-5p. We uncover that neither HHIP-AS1 nor the corresponding regulatory element in DYNC1I2 are evolutionary conserved in mice. Taken together, we discover an lncRNA-mediated mechanism that enables the pro-mitotic effects of SHH pathway activation in human tumors.
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Introduction
Sonic hedgehog (SHH) signaling plays a pivotal role in promoting oncogenesis, tumor growth and progression1. It is aberrantly activated in various common cancers in adults, including basal cell carcinoma (BCC)2, but also in pediatric neoplasms, including rhabdomyosarcoma3 and brain tumors such as medulloblastoma (MB) and atypical teratoid/rhabdoid tumors (ATRT)4,5,6,7,8. Pediatric brain tumors, like MB and ATRT, are the most common solid malignancies of childhood and the leading cause of cancer-related death in children9. Both entities are highly heterogeneous and can be segregated into distinct subgroups by virtue of their divergent molecular characteristics. Notably, such classification, which is primarily based on intergroup differences detected at multi-omics level, is of clinical utility, as it correlates with specific and distinct clinico-pathological and prognostic patterns10,11,12. Specifically, MB comprises four main subgroups, designated as Wingless (WNT), SHH, Group 3 and Group 413,14,15,16. WNT and SHH MBs are named according to the signaling pathways that drive their formation and progression17,18. Conversely, the other two MB subgroups are less defined in their molecular etiology19,20, although Group 3 MB recurrently displays MYC amplification and/or overexpression21,22,23,24, while Group 4 MB commonly show activation of receptor tyrosine kinase signaling through aberrant expression of ERBB4 and the phosphorylated form of the tyrosine–protein kinase SRC25. In the case of ATRT, three subgroups have been defined, namely tyrosinase (TYR), MYC and SHH, according to the distinctive overexpression of TYR or MYC genes, or the activation of SHH signaling4,6,26.
Targeting the SHH signaling to extinguish its mitogenic effects in SHH MB has shown efficacy in pre-clinical animal models and in humans27. However, the clinical use of SHH inhibitors, such as the G protein-coupled receptor smoothened (SMO) antagonist Vismodegib (GDC-0449), is limited due to toxicity or emergence of drug resistance in children with SHH MB to date28,29. While mutation and altered expression of several protein-coding genes are well-established drivers of SHH-dependent tumorigenesis, the precise impact of the non-protein coding genome remains largely unexplored. In particular, investigations of the specific role of long non-coding RNAs (lncRNAs) in SHH-driven malignancies are just emerging as an important research field30,31. Most research efforts have so far focused on well-defined and comprehensive murine models of SHH-driven tumors32,33. However, these models fail to offer a faithful representation of the human lncRNAs landscape, because lncRNAs show only poor conservation across species34. Nevertheless, lncRNAs are known to play essential roles in all aspects of cell biology35,36,37 and the regulatory mechanisms orchestrated by lncRNAs are diverse including direct binding to chromatin38, proteins39 or regulating microRNAs40. Conversely, the role of non-coding RNAs in the pathogenesis and disease stratification of ATRT has not been elucidated so far, and non-coding RNA classes also remain poorly characterized in MB.
Here, we explore the role of lncRNAs specifically in SHH-driven tumors with the aim to decipher the impact in SHH signaling regulation and function in these tumors. We show that aberrant expression of the lncRNA Hedgehog Interacting Protein Antisense 1 (HHIP-AS1) is a hallmark of human SHH-driven tumors including MB and ATRT. HHIP-AS1 is actively transcribed from a SHH-responsive bidirectional promoter shared with the SHH signaling intermediate HHIP. HHIP-AS1 knockdown leads to reduced tumor growth in SHH-driven tumors in vitro and in vivo by decreasing cell proliferation and inducing mitotic spindle deregulation. Mechanistically, we show that HHIP-AS1 binds to and stabilizes the mRNA of cytoplasmic dynein 1 intermediate chain 2 (DYNC1I2), a component of the cytoplasmic dynein 1 complex, by preventing hsa-miR-425-5p-mediated degradation. We uncover that neither HHIP-AS1 nor the corresponding regulatory element in DYNC1I2 are evolutionary conserved in mice demonstrating the power of cross-entity transcriptome-wide comparisons to identify regulatory lncRNA circuitries in human cancer. In all, we discover a lncRNA-dependent blockage of endogenous RNA mechanism as an additional layer of epigenetic regulation mediated by HHIP-AS1 as a human-specific target gene in SHH-dependent cell progression.
Results
Overexpression of the long non-coding RNA HHIP-AS1 is a hallmark of human SHH-driven tumors
To discover global SHH-dependent gene expression patterns in cancer, we first determined differentially expressed transcripts in RNA sequencing data by comparing SHH MB (n = 58) to non SHH MB subgroup samples (n = 164) (Platform, R241). Our approach confirmed several known protein-coding SHH mediators including GLI1, GLI2, HHIP and Atonal BHLH Transcription Factor 1, and revealed lncRNAs deregulated in SHH MB (Fig. 1a, Supplementary Data file 1). Among these candidates, we identified HHIP-AS1 as the most specifically overexpressed lncRNA in SHH MB (Fig. 1a, Supplementary Data file 1) without protein-coding potential (Fig. S1a). We next investigated whether HHIP-AS1 was similarly overexpressed in other tumor entities with aberrant activation of the SHH signaling. Comparative expression analysis confirmed specific HHIP-AS1 overexpression in SHH-driven entities including ATRT (Fig. 1b), cutaneous BCC (Fig. S1b) and rhabdomyosarcoma (Fig. S1c) compared to normal and cancerous control tissues. Consistent with its overexpression, we next revealed active transcription of HHIP-AS1 from a hypomethylated promoter shared with HHIP, a well-established regulator of the SHH pathway and whose genomic localization shows a head-to-head orientation with the HHIP-AS1 locus, exclusively in SHH MB using both H3K27ac ChIP-sequencing (Fig. 1c) and high-resolution DNA methylation data (Fig. 1d and S1d). Transcriptome-wide correlation analyses consistently revealed that HHIP and HHIP-AS1 are co-expressed in MB (n = 167, r = 0.990, p < 0.001, Fig. S1e) and in ATRT (n = 49, r = 0.836, p < 0.001, Fig. S1f) cohorts. Furthermore, we could reveal that the two genes exhibited remarkably high and significant correlative co-expression scores in multiple expression datasets, including other cancer entities and control tissues (n = 39,090; p < 0.001, Fig. 1e). These observations prompted us to hypothesize that HHIP-AS1 and HHIP may indeed share a unique bidirectional promoter. Therefore, we performed a luciferase reporter assay and revealed the existence of forward and reverse activity of the promoter region in vitro (Fig. 1f), suggesting that promoter hypomethylation may equally drive overexpression of both HHIP-AS1 and HHIP transcripts in SHH-driven tumors.
Since HHIP-AS1 was not previously described in murine models of SHH-driven tumors and lncRNAs are only partially conserved through species34, we investigated to which extent HHIP-AS1 was conserved across vertebrates. Remarkably, genome-scale comparisons revealed that HHIP-AS1 was only conserved in primates and not in rodents (Fig. 1g and S1g), explaining why this lncRNA has not been identified in animal models so far.
HHIP-AS1 is functionally required in human SHH-driven brain tumors
Since HHIP-AS1 overexpression is a hallmark in SHH-driven tumors, we investigated whether HHIP-AS1 expression was dependent on SHH signaling in tumor cells. Pharmacological activation of SMO receptor using SAG (SMO agonist) increased HHIP-AS1 expression in two independent tumor cell lines, Daoy and CHLA-266, and one primary cell culture, HHU-ATRT1 (Fig. 2a) as well as in non-tumor cells with SHH activation, namely neuronal stem cells (NSC; Fig. S3a). Conversely, inhibition of SMO using cyclopamine (SMO antagonist) significantly reduced HHIP-AS1 in all these cell models (Fig. 2a and S3a). Activation and inhibition of the SHH pathway were confirmed by quantification of GLI expression level through qRT-PCR (Fig. 2a and S3a) and immunoblotting (Fig. S2a–c). GLI proteins are known to function as regulators of the SHH transcriptional response, hence we next examined whether GLI could affect HHIP-AS1 expression. Transient knockdown of GLI1 and GLI2 reduced HHIP-AS1 and HHIP expression in all of the above-mentioned SHH-cancer cell models (Fig. 2b and S2), while on the other hand overexpression of GLI1 (Fig. S2d) resulted in increased expression of HHIP and HHIP-AS1 (Fig. S3b), confirming HHIP-AS1 as a target gene of SHH signaling. To evaluate the functional impact of HHIP-AS1, we silenced its expression in vitro using either siRNAs or shRNAs directed against this lncRNA. Strikingly, knockdown of HHIP-AS1 (Fig. S3c) resulted in reduced proliferation, monitored by EdU incorporation (Fig. 2c), as well as reduced clonogenicity (Fig. 2d) of Daoy, CHLA-266 and HHU-ATRT1. In addition, cell viability, assessed through metabolic assay (CellTiter-Glo), was diminished in the SHH MB cell line Daoy and in ATRT cell line CHLA-266 upon HHIP-AS1 silencing (Fig. S3d). We could verify these phenotypic changes after transient HHIP-AS1 knockdown in additional SHH-driven cell models, namely CHLA-04 (ATRT), RH30 (rhabdomyosarcoma), NSC and UI226 (BCC, Fig. S3e). Importantly, we also confirmed that HHIP-AS1 depletion reduced proliferation and viability in primary cultures from two SHH MB patients (Fig. 2e and f) and impaired proliferation of cultured cells of ICN-MB12 (SHH MB patient derived xenograft model; Fig. 2g). Notably, overexpression of HHIP-AS1 rescued the reduced proliferation and viability (Fig. S3f), highlighting that HHIP-AS1 is not only aberrantly overexpressed in SHH-driven tumors, but also functionally relevant in these malignancies. Conversely, transfection of HHIP-AS1 siRNAs into non SHH MB cells (HD-MB03 and CHLA-01) with low expression of HHIP-AS1 (Fig. S3g) did not result in reduced proliferation and viability (Fig. S3h), ruling out potential off-target effects and confirming that the functional relevance of HHIP-AS1 is restricted to SHH-driven tumors. Remarkably, HHIP expression was not affected on mRNA or protein levels upon stable HHIP-AS1 depletion (Fig. S4a–c). Therefore, we rule out a cis-regulatory effect of HHIP-AS1 on HHIP in our MB and ATRT models.
Identification and functional validation of HHIP-AS1 downstream targets reveals that HHIP-AS1 binds to the mRNA of DYNC1I2
In order to decipher the molecular mechanism controlled by HHIP-AS1, we investigated the impact of HHIP-AS1 knockdown on both transcriptome and proteome in two independent cell models (Daoy and CHLA-266). Interestingly, our integrative proteogenomic analysis identified two candidates that were highly and consistently perturbed upon HHIP-AS1 knockdown in both models, namely hydroxysteroid 17-beta dehydrogenase 10 (HSD17B10) and DYNC1I2 (Fig. 3a, RNA sequencing data: NCBI GenBank #GSE140741 and proteomic data: ProteomeXchange PRIDE database #PXD016550). We decided to focus on DYNC1I2 based on its co-expression with HHIP-AS1 in primary MB samples (r = 0.336; p < 0.001, Fig. 3b), as well as its high expression level specifically in SHH MB subgroup (Fig. S5a) and its known functions in neurodevelopment and cell cycle progression42. HSD17B10 did not show a significant correlation with HHIP-AS1 in primary MB samples (Fig. S5b). We validated by qRT-PCR and immunoblots that HHIP-AS1 depletion reduced the mRNA and protein expression of DYNC1I2 in Daoy, CHLA-266 and HHU-ATRT1 cells (Fig. S5c and d). To determine the underlying molecular mechanism, we investigated a potential interaction between HHIP-AS1 and DYNC1I2 mRNA. First, we uncovered that both RNAs are co-localized in cells using RNA fluorescence in situ hybridization (Fig. 3c and S5e) and this co-localization can be enhanced or disrupted via SHH activation or inhibition, respectively (Fig. S5f). Second, we confirmed a direct interaction in each of our three cell models using an RNA-RNA-centric-pulldown probe set directed against HHIP-AS1 RNA, which led to a specific enrichment for DYNC1I2 mRNA compared to negative controls (Fig. 3d). Finally, we computationally derived the sequence of HHIP-AS1 that is predicted to pair with DYNC1I2 mRNA (Supplementary Table S1), identifying a 24 nucleotides long region (named HHIP-AS1bind) able to bind the 5'UTR of DYNC1I2. Furthermore, using bio-layer interferometry, we found that HHIP-AS1bind could physically interact with DYNC1I2 mRNA (Fig. 3e). In contrast, a negative control sequence of HHIP-AS1 (named HHIP-AS1neg), carrying the same GC content and number of nucleotides as HHIP-AS1bind, but devoid of any in silico pairing potential to DYNC1I2 mRNA, did not show any binding activity (Fig. S5g). Strikingly, we found that in vitro transfection of Daoy or HHU-ATRT1 with HHIP-AS1bind resulted in extended half-life of DYNC1I2 mRNA (Fig. 3f and S5h), compared to a control condition where HHIP-AS1neg was used. All these findings confirm the existence of a functional and direct physical interaction between these two RNAs in vivo and in vitro, which ultimately regulates DYNC1I2 expression levels. In order to elucidate whether the functional interaction between HHIP-AS1 and DYNC1I2 mediates the pro-proliferating phenotype controlled by HHIP-AS1, we evaluated the functional impact of DYNC1I2 depletion in our cell models. Interestingly, transient DYNC1I2 knockdown resulted in reduced proliferation and viability to a similar degree as observed upon HHIP-AS1 depletion (Fig. S6a and b). More importantly, when we overexpressed DYNC1I2 using CRISPR-Cas9-based activation in HHIP-AS1-transiently depleted cells, both proliferation and viability were restored (Fig. 3g and h), indicating that HHIP-AS1 exerts its pro-proliferative effects by controlling DYNC1I2 abundance in tumor cells.
The interaction between HHIP-AS1 and DYNC1I2 promotes mitosis
Cytoplasmic dynein-complex 1 has been implicated in various phenotypes including cargo transport on cytoplasmic microtubules and it was recently reported that DYNC1I2 loss disrupts mitotic spindle organization in zebrafish neural progenitor cells42. Thus, we hypothesized that HHIP-AS1 loss may cause a similar effect in human tumor cells by reducing DYNC1I2 availability. Indeed, we found that transient knockdown of HHIP-AS1 or DYNC1I2 via siRNAs transfection significantly and consistently altered mitotic spindle organization in cells compared to siRNA control-transfected cells (Fig. 4a and b; Fig. S6c and d), leading to more DNA damage in the mitotic cells as well (Fig. S6e). Moreover, using two different shRNAs against HHIP-AS1, we could confirm the alteration in mitotic spindle organization in Daoy and CHLA-266 (Fig. 4c and d) upon stable HHIP-AS1 depletion. More importantly, induced overexpression of DYNC1I2 as well as of HHIP-AS1 with CRISPR-Cas9-based activation, rescued the mitotic spindle organization (Fig. 4e and f) in the context of transient HHIP-AS1 knockdown, supporting that HHIP-AS1 promotes proliferation through mitotic spindle stabilization by controlling DYNC1I2 abundance.
HHIP-AS1 blocks endogenous hsa-miR-425-5p function to maintain DYNC1I2 level
To further mechanistically elucidate how HHIP-AS1 stabilizes DYNC1I2 mRNA, we evaluated the genetic sequence of RNA-RNA interaction. Our analysis revealed six potential miRNA binding sites (Supplementary Table S2) within the predicted interaction region between HHIP-AS1 and DYNC1I2 mRNA (Fig. 5a), suggesting that HHIP-AS1 binding to DYNC1I2 mRNA may interfere with miRNA-dependent regulation of DYNC1I2 expression. Therefore, we correlated the expression of these miRNA candidates with DYNC1I2 using RNA sequencing data of 167 primary MB samples. Out of these six miRNAs, four were not detected in MB patient samples, while two miRNAs showed expression in MB patient samples, namely hsa-miR-425-5p (see binding site in Fig. 5a) and hsa-miR-1915. Notably, hsa-miR-425-5p expression level showed no differences across molecular subgroups of MB patients and cell models (Fig. S7a and b), but demonstrated anti-correlation with DYNC1I2 expression in patient samples (r = −0.312; p < 0.001, Fig. S7c) compared to hsa-miR-1915 (Fig. S7d). After dividing the dataset into SHH and non SHH MB, the anti-correlation was only maintained in non SHH MB samples (r = −0.303; p < 0.001, Fig. S7e). We therefore tested whether a functional relationship existed between hsa-miR-425-5p and DYNC1I2. First, we cloned the 5´UTR of DYNC1I2 in front of a luciferase reporter and found that hsa-miR-425-5p functionally binds this sequence causing a reduction of luciferase expression (Fig. 5b), hence confirming our previous in silico prediction (Fig. 5a). Importantly, this effect was abrogated upon mutation of the miRNA binding sequence on DYNC1I2 5´UTR (Fig. 5b). Second, we demonstrated that hsa-miR-425-5p inhibition significantly increased DYNC1I2 mRNA levels upon stable HHIP-AS1 knockdown in three SHH-driven cell models, while transfection of a negative control miRNA inhibitor did not restore DYNC1I2 expression (Fig. 5c). This effect could be also observed after in vitro transfection of stable sh-HHIP-AS1 Daoy with only HHIP-AS1bind sequence resulting in higher expression of DYNC1I2 mRNA independent of hsa-miR-425-5p inhibition (Fig. S8a), compared to a control condition where HHIP-AS1neg was used. Interestingly, the corresponding regulatory element of DYNC1I2, where hsa-miRNA-425-5p is binding, is not evolutionary conserved in mice (Fig. S9). Third, inhibition of hsa-miR-425-5p rescued the decreased proliferation phenotype in Daoy and CHLA-266 obtained with HHIP-AS1 knockdown (Fig. 5d). Finally, blockage of hsa-miR-425-3p showed no effect on DYNC1I2 expression level (Fig. S8b–d).
Thus, our data unravel a regulatory network requiring HHIP-AS1 to bind to DYNC1I2 mRNA, to prevent DYNC1I2 depletion mediated by binding of hsa-miRNA-425-5p to its 5'UTR. Together, our correlative data analysis approach in primary MB samples combined with in silico predictions and mechanistic validation, uniformly point to a previously poorly explored regulatory function of lncRNAs which consists in binding to a specific mRNA and thereby blocking endogenous miRNA binding sites.
Loss of HHIP-AS1 extends survival in SHH-driven brain tumors in vivo
We next evaluated whether targeting HHIP-AS1 affected tumor growth in vivo. To this end, we initially utilized two well-established orthotopic brain tumor models with aberrant SHH signaling activation. Remarkably, stable knockdown of HHIP-AS1 in both orthotopically engrafted Daoy and CHLA-266 cells significantly extended the survival of recipient mice compared to corresponding isogenic controls (Daoy, p = 0.0045; CHLA-266, p = 0.0011; Fig. 6a and b). Repeated luminescence measurement indicated that the loss of HHIP-AS1 affected tumor formation in vivo consistently (Fig. S10a–c). We next aimed at validating our finding using a well-characterized patient-derived xenograft model of SHH MB. We transduced cells from the SHH-Med-1712-FH PDX model in vitro with sh-HHIP-AS1 or control shRNA prior to transplantation into the cerebella of recipient mice. Knockdown of HHIP-AS1 and corresponding DYCN1I2 reduction was confirmed in this model via qRT-PCR (Fig. S10d). Interestingly, silencing of HHIP-AS1 in injected PDX cells delayed the appearance of signs of morbidity in animals, whose mean survival was significantly extended compared to control mice (p = 0.0011; Fig. 6c). Lastly, HHIP-AS1 depletion markedly reduced cell proliferation index in Med-1712-FH PDX tumors compared to control tumors, when these samples were tested for Ki67-immunoreactivity (Fig. 6d). Accordingly, we observed more differentiated cells in tumor tissue compared to control (Fig. S11a). In line with our in vitro data, we detected no change in caspase activity (cleaved caspase) in Med-1712-FH PDX tumors (Fig. S10e and S11b). However, we observed more DNA damage in tumor tissue compared to control (Fig. 6e) and in NSC (Fig. S9f) after HHIP-AS1 depletion. Overall, these results provide compelling evidence that HHIP-AS1 promotes tumorigenicity of SHH-driven human tumors in vivo.
Discussion
Until now the complexity of the human SHH signaling pathway and regulatory feedback loops is not fully understood. Specifically, the precise knowledge of the molecular mechanisms underlying SHH pathway pro-oncogenic activity in human cells is urgently required. To this aim, the widespread use of genetic animal models of SHH-driven malignancies has been successful at identifying and describing a large number of protein-coding genes and protein post-translational modifications implicated in regulation and downstream functions of SHH signaling in tumors43,44,45,46. Nevertheless, despite accounting for ~70% of the transcribed genome in humans47, mechanistic insights into the role of lncRNAs in SHH-driven cancer biology have been gained only for a very few species. A reason for this poor consideration relies on the general low level of inter-species conservation of lncRNAs, which has inevitably hindered their discovery and functional characterization in the commonly used genetic rodent models. In our study, we employed a large comparative transcriptome analysis approach across several thousands of human normal and cancerous tissues, and identified HHIP-AS1 as a lncRNA that is specifically upregulated in SHH-driven tumors and functionally required for mediating the pro-proliferative effects of oncogenic SHH signaling. Interestingly, we found that HHIP-AS1 constitutes a downstream transcriptional target of SHH signaling, providing an explanation to its restricted and elevated expression in SHH-driven entities. Specifically, we uncovered that HHIP-AS1 transcription is initiated from a bidirectional promoter shared with the known SHH-pathway regulator HHIP. However, unlike HHIP or other key protein-coding gene of the SHH pathway, HHIP-AS1 is poorly conserved across vertebrates, showing high sequence similarity between humans and other primates, but substantially no conservation between humans and rodents. Therefore, our findings pinpoint the importance of species-specific evaluation of oncogenic signaling pathways, and emphasize how some key regulatory networks or pro-oncogenic programs may not be faithfully recapitulated by rodent tumor models, despite their generally well-accepted value to study human pathogenic processes. Furthermore, by using a combined proteomic and RNA sequencing approach, we uncovered that HHIP-AS1 acts in trans by regulating the expression of DYNC1I2, which encodes for an intermediate chain of the cytoplasmic dynein-complex 1, and not in cis by regulating HHIP48. We, among others, could already demonstrate the power of integrated proteogenomic approaches, showing that proteomic combined with transcriptomic profiles provides a profound insight into active oncogenic gene expression regulation in pediatric brain tumors and other cancers16,25. The involvement of the cytoplasmic dynein-complex 1 provides an intriguing aspect of SHH pathway regulation and function. Indeed, dynein motor complexes have been long implicated in the activity of SHH signaling. However, this association was only restricted to cytoplasmic dynein-complex 2, due to its requirement at the level of primary cilia in mediating ciliary retrograde transport49. By characterizing the functional interaction between HHIP-AS1 and DYNC1I2 in cancer cells and in NSC, we unraveled the existence of an additonal layer whereby SHH signaling sustains cell growth and progression. SHH signaling is already known to directly promote cell cycle progression by primarily activating the expression of MYCN and Cyclin D genes, which drive cells toward the G1/S transition50. By sustaining the transcription of HHIP-AS1, the SHH signaling guarantees effective spindle assembly and chromosome segregation through maintenance of appropriate levels of DYNC1I2. Interestingly, we could observe in cells with HHIP-AS1 depletion that the dysregulation of mitosis led to more DNA damage in mitotic cells. Although the DNA damage response and the mitotic cell division pathways were thought to be distinct and unrelated, it was shown in several studies that mitotic cells can experience DNA damage either endogenously due to unrepaired premitotic damage or exogenously from cancer therapies amongst other causes51,52,53. As we demonstrate that SHH exerts a control on cell division during the time of mitosis in cancer cells and in NSC, therapeutic limitations may exist. Targeting the SHH signaling pathway seems to provide a highly innovative therapeutic option for a broad variety of cancers. Nevertheless, as SHH pathway inhibitors seem to be safe in adults, this still remains to be shown in children treated for MB and taking into consideration our findings in NSCs. While the introduction of targeted therapies represents an exciting era in personalized medicine, compounds that target developmental signaling pathways (including SHH signaling) should be carefully evaluated for specific toxicities and their potential benefits.
Depleting cells of HHIP-AS1 or blocking its interaction with DYNC1I2 mRNA exposes the latter to hsa-miRNA-425-5p-mediated degradation, thereby compromising mitotic fidelity and consequently blocking cell progression in vitro and in vivo. As the power of miRNA in regulation of mRNA has been explored elaborately, we are beginning to recognize also the complex interactions of miRNAs and lncRNAs and ensuing RNA regulatory networks. Our work provides a previously unmatched molecular understanding of lncRNA function by actively competing with a miRNA binding site on a target mRNA. We show that the lncRNA HHIP-AS1 constitutes a so far unexplored target gene of SHH signaling, which enables the pro-mitotic effects of this pathway by blocking hsa-miR-425-5p-dependent inhibition of DYNC1I2 expression. This mechanism is of fundamental interest as it describes not only a major mediator of cell progression triggered by SHH activation but also as provides a previously unknown epigenetic regulation of SHH pathway in humans. However, to comprehensively understand the role of the regulatory HHIP-AS1/DYNC1I2/miR425 axis and its potent pro-mitotic effects, further experiments are required to elucidate the relevance in SHH-driven neurogenesis and tumorigenesis.
Methods
Animal models
For the orthotopic brain tumor models we used 8 week old female NMRI-Foxn1nu/nu that were purchased from Janvier Labs, Le Genest-Saint-Isle, France. We followed both European and national regulations for animal housing, care and experimentation (Directive 86/609). The use of animals was approved by the reporting ethical committee and the ministry under the agreement #03130.20. Ethics committee: CCEA-IC, Instances: Higher Education of the Ministry for Education and Research (France).
Cell culture
The cell line Daoy was obtained from American Type Culture Collection (ATCC, Manassas, VA) and was grown in Dulbecco’s Modified Eagle’s medium (DMEM) + GlutaMAX-I high glucose medium (Thermo Fisher Scientific, Waltham, MA, #31966021) supplemented with 10% fetal bovine serum (FBS) (Merck, Darmstadt, Germany #F9665) and 1% penicillin/streptomycin (P/S) (Merck, #P4333). Cell line CHLA-266 was purchased from CCcells (Childhood Cancer Repository) and was grown in 1x Iscove’s Modified Dulbecco’s medium (IMDM; Thermo Fisher Scientific, #12440053) supplemented with 20% FBS, 4 mM L-glutamine (Thermo Fisher Scientific, #25030032) and 1% insulin transferrin selenium (Thermo Fisher Scientific, #41400045). HHU-ATRT1 cells were generated at the University Hospital Düsseldorf (ethical permission #2018-102) and were grown in Neurobasal-A medium (Thermo Fisher Scientific, #10888022) complemented with 2 mM L-glutamine, 1% P/S, 0,0075% bovine serum albumin (BSA), B-27 supplement 1x (Thermo Fisher Scientific, #12587001), heparin (4 µg/ml, StemCell, #07980), recombinant epidermal growth factor (EGF, 10 ng/ml, Thermo Fisher Scientific, #RP-10914) and basic fibroblast growth factor (FGF, 10 ng/ml, Biomol, #HZ-1285). The cell line HD-MB03 was a generous gift of Dr. Till Milde, KiTZ, Hopp Children´s Cancer Center Heidelberg, and was grown in RPMI1640 (Thermo Fisher Scientific, #22400089) supplemented with 10% FBS and 1% MEM non-essential amino acids (Thermo Fisher Scientific, #11140050). Cell lines CHLA-01 and CHLA-04 were purchased from ATCC (CHLA-01, #ATCC CRL-3021 and CHLA-04, #ATCC CRL-3036) and grown in DMEM/F12 (Thermo Fisher Scientific, #11330-032) complemented with 2% B27, 20 ng/mL EGF and FGF. Neuronal stem cells (NSCs, H9 hESC-Derived) were purchased from Thermo Fischer Scientific (#GIBCO N7800100) and cultivated according to manufactures’ protocol. The cell line RH30 was a generous gift of Prof Simone Fulda, Head of Christian-Albrechts-University Kiel, Germany, and was grown in RPMI1640 (Thermo Fisher Scientific, #22400089) complemented with 10% FBS, 1% P/S, 1% Sodium Pyruvate (100 mM, Thermo Fisher Scientific, #11360-070). UI226 cell line was a generous gift of Prof Anthony Oro and Dr. Francois Kuonen, Department of Dermatology, Stanford University, USA, and was grown in KO-DMEM F12 cell culture media (Thermo Fisher Scientific, #A10509-01) and complemented with 1x supplement (Thermo Fisher Scientific, # A10509-01), 200nM L-glutamine and 20 ng/ml of FGF and EGF. All cell lines were incubated at 37 °C and 5% CO2. For SHH activation or inhibition, parental cells were treated with 50 nM smoothened agonist (Merck, #566661) or 1 µM cyclopamine (MedChemExpress, Sollentuna, Sweden, #HY-17024), respectively, for 24 h. SHH MB PDX lines, namely ICN-MB1254 and Med-1712-FH55 were grown in vitro in Neurobasal-A medium supplemented with 2 mM L-glutamine, 1% P/S, 0.45% D-glucose (Merck, #G7528), 0.4% BSA (Merck, #A9165), B27 and N-acetyl-L-cysteine (Merck, #A9576). Orthotopic engraftment was performed as previously described54. PDX cells were cultured in vitro exclusively for the time required for transducing them with lentiviruses. Daoy cells were co-infected with sh-HHIP-AS1 and MSCV-IRES-Luciferase lentiviruses prior orthotopic injection. Tumor growth was followed by Xenogen Ivis Spectrum imaging system (Perkin-Elmer). Patient-derived MB cells were freshly isolated from tissue samples obtained by surgical resection at the Department of Neurosurgery, University Hospital Düsseldorf with informed consent by the patients and approval by the institutional review board (study number: 2018-102). Cells were cultivated for 3 days before transient siRNA knockdown of HHIP-AS1 was performed.
Transient siRNA and miRNA transfection
Parental Daoy, CHLA-266, HHU-ATRT1, HD-MB03, CHLA-01, CHLA-04, RH30, NSC and patient-derived MB cells were transfected with 10 nmol siPOOLs (HHIP-AS1, DYNC1I2, see “Oligonucleotides” section in Table S3) using Lipofectamine RNAiMAX reagent (Thermo Fisher Scientific, #13778150) and harvested for RNA isolation after 48 and/or 72 h after transfection or were used for further analyses including EdU incorporation, colony formation assays, CTG and immunoblotting. For miRNA inhibition experiments, shRNA models of each cell line (included scramble as control, sh-HHIP-AS1#1 and sh-HHIP-AS1#2) were seeded into six-well plates. After reaching about 80% confluency, cells were transfected using Lipofectamine RNAiMAX either with the miRNA inhibitor for miR-425-5p, miR-425-3p or the negative miRNA inhibitor control (see “Oligonucleotides” in Table S3).
shRNA cloning and lentiviral transduction
shRNAs of indicated sequences (see “Oligonucleotides” in Table S3) were cloned into pLK0.1-TRC-Puro (Addgene, Watertown, MA, #10878). Pseudotyped lentivirus was generated as previously described31, and HEK293T cells were transfected with a packaging plasmid, envelope plasmid, and the generated shRNA vector plasmid using polyethylenimine (Merck, #408727). Virus was collected 48 h and 72 h after transfection, 0.4 μm filtered, and used directly for transduction with polybrene (Merck, #TR-1003-G). Successfully infected cells were selected in puromycin (0.8–1.5 μg/ml; Merck, #P8833) containing medium.
Overexpression
For the overexpression of DYNC1I2, GLI and HHIP-AS1 in Daoy, we used a transcriptional activation by an engineered CRISPR-Cas9 complex referred to as “SAM”. Cloning of SAM sgRNA was performed as previously described56; for sequence details, see “gDYNC OE”, “gGLI OE” and “gHHIP-AS1 OE” in “Oligonucleotides” section in Table S3. After stable transduction of the sgRNAs, we performed a transient knockdown of HHIP-AS1 as described in section “Transient siRNA and miRNA transfection”.
RNA extraction, cDNA synthesis and qRT-PCR
Total RNA was extracted using TRIzol (Thermo Fisher Scientific, #15596018) according to the manufacturer’s instructions or by using the MaxWell system (Promega, #AS1340). Isolated RNA was quantified by spectrophotometry and 500 ng of RNA was retrotranscribed to total cDNA using random hexamer and oligo-dT primer mix (Promega, Madison, WI, #C110A), dNTP mix (Promega, #U1511), M-MLV-RT 5X buffer (Promega, #M3681), M-MLV RT, RNase (H–), point mutant (Promega, #M368C) and RNasin-Plus ribonuclease inhibitor (Promega, #N2511). Resulting cDNA was analyzed by TaqMan-based qRT-PCR containing FAM-labeled probes. All reactions were performed in triplicates using a “CFX384 Touch Real-Time PCR Detection System” (Bio-Rad, Hercules, CA). Relative expression levels of candidate genes were acquired by normalization against the housekeeper genes GUSB, HPRT1 and PPIA.
MiRNA extraction, cDNA synthesis and qRT-PCR
MicroRNAs (miRNA) were extracted using the “Maxwell RSC miRNA Kit” (Promega, #AS1470) according to the manufacturer’s instructions. Afterwards the “Applied Biosystems™ TaqMan™ Advanced miRNA cDNA Synthesis Kit” (Thermo Fisher Scientific, #A28007) was used according to the manufacturer’s instructions. For qRT-PCR analyses singleplex miRNA Assays (Thermo Fisher Scientific) for hsa-miR-425-5p (SM-10204) and hsa-miR191 (SM-20786) as a control were used.
Primers, siRNAs, raPOOLs and shRNAs
TaqMan-based primers were purchased from IDTdna: DYNC1I2 (Hs.PT.58.3736795); GLI1 (Hs.PT.58.26486279), GLI2 (Hs.PT.58.45642781); GUSB (Hs.PT.58 v.27737538); HHIP (Hs.PT.58.40948312); HHIP-AS1 (Hs.PT.58.613732); HPRT1 (Hs.PT.58 v.45621572); MALAT1 (Hs.PT.58.26451167.g); PPIA (Hs.PT.39a.22214851); ppia (Mm.PT.39a.2.gs), b2m (Mm.PT.39a.22214835), gusb (Mm.PT.39a.22214848), hhip (Mm.PT.58.29299649) and gli1 (Mm.PT.58.11933824). siRNA pools, consisting of 30 different siRNAs, were purchased from siTOOLs Biotech (Martinsried, Germany): HHIP-AS1 (#646576- 10 nmol); DYNC1I2 (#1781- 10 nmol); raPOOLs, consisting of 30 biotinylated RNA probes, were also from siTOOLs Biotech: HHIP-AS1 (#raPOOL646576 –5 nmol).
Immunoblots
Immunoblots experiments were performed using the following primary antibodies: anti-DYNC1I2 (Atlas Antibodies, Bromma, Sweden, #HPA040619, 1:1000), mouse anti-β-Actin (C4) (Santa Cruz Biotechnology, Heidelberg, Germany, #sc-47778, 1:1000) or mouse anti-β-Actin (Cell Signaling Technology, Danvers, MA, #3700, 1:1000), mouse anti-HHIP (Abnova Germany; #H00064399-M01; 1:1000); mouse anti-GLI2 (Santa Cruz Biotechnology, Heidelberg, Germany, #sc-271786, 1:500); rabbit anti-GLI1 (Cell Signaling Technology, Danvers, MA, #V812,1:1000).
Luciferase reporter assay
Promoter insert (Chromosome 4: 144,645,400-144,647,801; hg19 coordinates) was subcloned into pGL4.22 [luc2CP/Puro] Vector (Promega, #DQ188841) in two orientations. The forward sequence (“HHIP-fw”) was flipped around for the “HHIP-rv” sequence. The correctness of insert orientations was confirmed by sequencing. The reporter activity was measured by using “Dual-Luciferase Reporter Assay System” (Promega, #E1910) according to the manufacturer’s instructions. The 3'- and 5'-Luciferase reporter gene assays were performed as described previously57 except for transfecting cells with 50 nM of pre-miR miRNA precursor hsa-miR-425-5p (Thermo Fisher Scientific, #17100) and control cells with 50 nM of the pre-miR miRNA precursor negative control #1 (Thermo Fisher Scientific, #AM17110).
RNA fluorescence in situ hybridization (FISH)
FISH was carried out based on the Stellaris RNA FISH protocol according to the manufactory. Daoy and CHLA-266 cells were fixed in 4% formaldehyde (Merck, #100496.8350) at room temperature for 10 min. Cells were permeabilized in 70% ethanol at 4 °C for 1 h followed by hybridization with FITC-labeled HHIP-AS and ATTO655-labeled DYN1I2 probes in hybridization buffer (10% formamide, 10% dextran sulfate, 2x saline sodium citrate) at 37 °C overnight. Nuclei were stained with 4', 6-diamidino-2-phenylindole (DAPI). Images were acquired using a wide field fluorescence microscope Axio Observer.Z1 (Carl Zeiss Microscopy, Jena, Germany) with an ApoTome 2 (Zeiss) attachment.
Bio-Layer interferometry
Bio-Layer interferometry (BLI) has been a promising technique to study the RNA-RNA binding interaction58. We used the “Fortebio Blitz System” (Fortebio, Fremont, CA) to study the interaction between the proposed RNA sequences along with a negative control sequence. We used 1x RNA binding buffer (RBB) containing 10 mM Tris-HCl pH 8.0, 125 mM NaCl, 125 mM KCl & 25 mM MgCl2 to perform all binding studies. We used a modified protocol from58 to study the binding interaction in our system. Basically, SSA biosensor tips were hydrated in RBB for at least 10 min. Next, 200 nM of biotinylated DYNC1I2 sequence (ordered from IDTdna, see section “In silico analysis of RNA binding”) was loaded for 15 min after performing an initial baseline of the unloaded sensors for 30 s in RBB. Subsequently, the loaded sensors were incubated in RBB for 1 min. The loaded sensors were incubated with 200 nM of HHIP-AS1 pos/neg sequence (ordered from IDTdna, see section “In silico analysis of RNA binding”) for 5 min in the association phase, and dissociation of the bound sequences was studied for 5 min again in RBB. All the RNase free buffer components were purchased from “Thermo Fisher Scientific”. The biotinylated and non-biotinylated RNA sequences were ordered from IDTdna. The Super-Streptavidin (SSA) coated biosensors were purchased from Fortebio.
Immunofluorescence for cell proliferation, DNA damage and mitotic spindle evaluation
For immunofluorescence experiments, parental Daoy, CHLA-266, HHU-ATRT1, RH30 and NSC cells were seeded on 8-well glass slides (Nunc™ Lab-Tek™ II Chamber Slide™ System, Thermo Fisher Scientific, #154534). The next day, cells were transfected using siPOOLs as described above for transient knockdown. Stable generated shRNA models for each cell line (included scr as control, sh-HHIP-AS1#1 and sh-HHIP-AS1#2) were also seeded on 8-well glass slides. SHH MB PDX cells of ICN-MB12 were seeded on 8-well glass slides (Millicell EZ slide, Merck, #PEZGS0816) pre-coated with poly-D-lysine (Merck, #A-003-E) and Matrigel (Dutscher, Brumath, France #354230). Lentiviral transduction with shRNA constructs was performed 2 h after seeding. Cells were maintained in culture for 10 days, passing them when confluence was reached. A pulse of 10 μM BrdU (BD Biosciences, #550891) was provided before fixation with 4% PFA for 20 min. For orthotopic SHH MB tumors of Med-1712-FH PDX line, whole mouse brains bearing the tumor were fixed for 10 h in 4% PFA. The tissue was then embedded in paraffin and sagittal sections (3 μm) were obtained using microtome (Leica, Wetzlar, Germany). Proliferation analysis in Daoy, CHLA-266, HHU-ATRT1 and patient-derived MB cells was performed 72 h after transient, siRNA-mediated knockdown of HHIP-AS1 using the “Click-iT EdU Alexa-Fluor 488 Imaging Kit” (Thermo Fisher Scientific, #C10337) according to the manufacturer’s instructions. PDX cells in vitro and orthotopic PDX tissue sections were instead stained with 1:400 rabbit anti-Ki67 (Merck Millipore, Darmstadt, Germany, #AB9260), 1:1000 rabbit anti-NeuN (Abcam, #ab177487), 1:100 Rabbit anti-Cleaved Caspase 3 (D175, Cell Signaling, #9661S), 1:100 mouse anti-phospho-γH2AX (JBW301,Merck Millipore, Darmstadt, Germany, #05-636-I) for in vivo tissue slides or 1:400 rabbit anti-phospho-histone γH2A.X (Cell Signaling, Frankfurt, Germany #9718) for in vitro staining and 1:500 anti-BrdU (Bio-Rad AbD Serotec, Oxford, UK, #OBT0030G) primary antibodies. For DNA damage in vitro studies, neuronal stem cells or Daoy were seeded on 8-well glass slides (Nunc™ Lab-Tek™ II Chamber Slide™ System, Thermo Fisher Scientific, #154534) fixed in paraformaldehyde, rinsed in phosphate-buffered saline, and incubated with γH2AX antibodies and then Alexa 568-conjugated goat anti-rabbit IgG as secondary antibody. Slides mounted with Slow-Fade antifade reagent were imaged on an Zeiss inverted Apotome microscope with a ×63 oil immersion objective (Zeiss). Before counting foci, digital images were processed with ImageJ (LOCI, University of Wisconsin) to adjust brightness and contrast. Cells were evaluated as “positive” for γH2AX foci if they displayed >10 discrete dots of brightness. For tumor sections, only distinct and bright cells for γH2AX were counted as positive cells. Mitotic spindle staining was achieved by staining cells with 1:500 rabbit anti-pericentrin (Abcam, Cambridge, UK, #AB 4448) and 1:500 mouse anti-acetylated tubulin (Merck, #T6793) primary antibodies, detecting the centrosomes and the microtubules of the spindle, respectively.
In all cases, secondary antibodies were species-specific: chicken anti-rabbit IgG (H + L) cross-adsorbed secondary antibody, Alexa-Fluor-488 labeled (Thermo Fisher Scientific, #A-21441) and goat anti-mouse IgG2b cross-adsorbed secondary antibody, Alexa-Fluor-594 labeled (Thermo Fisher Scientific, #A-21145).
Clonogenic, caspase 3/7 activity and cell viability assays
For the analysis of self-renewal capacity, clonogenicity was analyzed. Daoy, CHLA-266 and HHU-ATRT1 were seeded on 10 cm dishes at the appropriate density and cultured for 1–3 weeks. For transient knockdown approach, cells were transfected with siPOOL against HHIP-AS1 as described above after 24 h of seeding. Stable shRNA models of each cell line (included control, sh-HHIP-AS1#1 and sh-HHIP-AS1#2) were also seeded in 10 cm dishes at the appropriate density and cultured for 1–3 weeks. The cells were washed with PBS, fixed in 10% formaldehyde for 30 min at RT and stained in 1% crystal violet for 1 h at RT. Next, cells were washed in ddH2O and the number of colonies was quantified. Caspase 3/7 activity was measured using Caspase-Glo 3/7 Assay System (Promega, Walldorf, Germany, #G8091) and cell viability assessment was determined by metabolic assay, using CellTiter-Glo Luminescent Cell Viability Assay (Promega, Walldorf, Germany, #G7570) according to the manufacturer’s instructions.
In silico analysis of RNA binding
The potential binding between HHIP-AS1 and DYNC1I2 mRNA was analyzed in silico using IntaRNA59,60 and http://rtools.cbrc.jp/ bioinformatics web servers. We detected a 24 nt long sequence (CCCTTGCCTACAACCAGACTGACA) in HHIP-AS1, which binds to the 5´UTR region of DYNC1I2. This sequence we used as a “positive binding” probe for mRNA stability assay and we designed another sequence with a similar G/C content from HHIP-AS1 that was predicted not to bind DYNC1I2, as a negative control (TTCAGCCTCCAAGGGGGCTTTTAA). Secondary structures of two RNAs forming dimers were predicted with RNACOFOLD61, which takes into account intra- as well as intermolecular base pairs of both sequences. Secondary structures of single sequences were predicted with RNAFOLD. All calculations were performed at T = 37 °C and all used programs were from the “ViennaRNA package” v. 2.4.662.
mRNA stability assay
Cells were pretreated either in the presence or absence of positive binding sequence (HHIP-AS1bind; see “in silico analysis of RNA binding”) or “not binding” sequence (HHIP-AS1neg) before the addition of actinomycin D (Hycultek; 10 μg/ml final concentration), a potent inhibitor of mRNA synthesis. Afterwards, total mRNA was extracted at 0–9 h and DYNC1I2 abundance was measured by qRT-PCR.
RNA sequencing and conservation analysis
For RNA sequencing analysis, reads generated from Daoy scr (control), Daoy sh-HHIP-AS1#1, Daoy sh-HHIP-AS1#2, CHLA-266 scr (control), CHLA-266 sh-HHIP-AS1#1and CHLA-266 sh-HHIP-AS1#2 were filtered, normalized and aligned to the human genome hg38 using STAR (v2.4.1d), unaligned reads were further aligned using BOWTIE2 (v2.2.5) and combined reads were quantified using the partek expectation-maximization algorithm against ENSEMBL release 84. For conservation analyses across species, the genomic loci and surrounding genomic regions for the species were analyzed using ECR browser (https://ecrbrowser.dcode.org/) and Ensembl (https://www.ensembl.org/index.html). Annotated species-specific exonic and intronic regions are highlighted in yellow or orange, respectively. Used RefSeq datasets were: zebrafish [danRer7], chicken [galGal3], rat [rn4], mouse [mm10], rhesus macaque [rheMac2], chimpanzee [panTro3] and human [hg19].
Proteomic analyses
Sample preparation
Proteins were extracted from frozen cell pellets as previously described63. Briefly, cells were homogenized in urea buffer with a “TissueLyser” (Qiagen, Hilden, Germany) and subsequent sonication. After centrifugation for 15 min at 14,000 g and 4 °C, supernatants were collected. Protein concentration was determined via pierce 660 nm protein assay (Thermo Fisher Scientific) and 10 µg protein per sample were desalted through electrophoretic migration at 50 V for 10 min on a 4–12% bis-tris polyacrylamide gel (Thermo Fisher Scientific, #NP0322BOX). After silver staining, protein bands were cut out, reduced, alkylated and digested with trypsin before peptide extraction via sonication. Peptides were dissolved and diluted with 0.1% TFA (v/v).
LC-MS analysis
For mass spectrometric analysis, 15 µl peptide solution per sample was analyzed on a nano-high-performance liquid chromatography electrospray ionization mass spectrometer. The analytical system was composed of a “RSLCnano U3000 HPLC” coupled to a “Orbitrap Elite mass spectrometer via a nano-electrospray ion source” (Thermo Fisher Scientific). Injected peptides were concentrated and desalted at a flow rate of 6 µl/min on a trapping column (Acclaim PepMao C18, 2 cm × 100 µm × 3 µm particle size, 100 Å pore size, Thermo Fisher Scientific) with 0.1% TFA (v/v) for 10 min. Subsequently, peptides were separated at a constant flowrate of 300 nl/min over a 120 min gradient on an analytical column (Acclaim PepMap RSLC C18, 25 cm × 75 µm × 2 µm particle size, 100 Å pore size, Thermo Fisher Scientific) at 60 °C. Separation was achieved through a gradient from 4 to 40% solvent B (solvent A: 0.1% (v/v) formic acid in water, solvent B: 0.1% (v/v) formic acid, 84% (v/v) acetonitrile in water). Afterwards, peptides were ionized at a voltage of 1.400 V and introduced into the mass spectrometer operated in positive mode. Mass spectrometry scans were recorded in profile mode in a range from 350–1700 m/z at a resolution of 60,000 while tandem mass spectra were recorded in the ion trap at normal scan rate. Tandem mass spectra were recorded with a data dependent Top 20 method and 35% normalized collision energy. Dynamic exclusion was activated with a repeat count of 1 for 45 s and only charge states 2+ and 3+ were analyzed.
Computational mass spectrometric data analysis
Proteome discoverer (version 1.4.1.14, Thermo Fisher Scientific) was applied for peptide/protein identification with mascot (version 2.4, Matrix Science) as search engine employing the UniProt database (human; including isoforms; date 2016-11-01). A false discovery rate of 1% (p ≤ 0.01) on peptide level was set as the identification threshold. Proteins were quantified with Progenesis QI for Proteomics (Version 2.0, Nonlinear Dynamics, Waters Corporation).
Statistics
Unless otherwise indicated in the figure legends, error bars represent mean ± SD or SEM of at least three independent experiments for each genotype or sample, and the used statistical test is indicated in each figure legend. Graphs were generated by using GraphPad PRISM ® Version 9 Graphpad Software.
Reporting summary
Further information on research design is available in the Nature Research Reporting Summary linked to this article.
Data availability
Previously published gene expression and methylation data used in Fig. 1a–e, 3b, S1b–f, S5a, b, S7a, c–e are available under ‘R2: Genomics Analysis and Visualization Platform (http://r2.amc.nl)’. RNA sequence data that support the findings of this study have been deposited in GenBank with the #GSE140741 accession code and proteomic data have been deposited in ProteomeXchange PRIDE database with the #PXD016550 accession code. The authors declare that the data supporting the findings of this study are available within the paper and its supplementary information files. Proteome discoverer (version 1.4.1.14, Thermo Fisher Scientific) was applied for peptide/protein identification with mascot (version 2.4, Matrix Science) as search engine employing the UniProt database (human; including isoforms; date 2016-11-01). The raw data behind data points in figures and that support the findings of this study are available in the linked. Source data provided with this paper.
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Acknowledgements
We thank especially Prof Simone Fulda and PD Dr Till Milde for their generous gifts of in vitro models. Furthermore, we thank Emilie Indersie for her support and Christophe Alberti, Elodie Belloir, and Adlin Thadal for mouse colony management. We also thank Kanokporn Faguier, Valérie Petit, Guillaume Bourmeau and Laetitia Besse for their help and advice in Histology and Imaging. This work was supported by grants from Deutsche Forschungsgemeinschaft (RE 2857/2-1 to M.R., RE938/4-1 to G.R., KFO 337 to M.R.), the German Cancer Aid (Deutsche Krebshilfe, grant no. 111537 to M.K., S.M.P., M.R. and G.R.), José-Carreras foundation (DJCLS 21R/2019 to U.F., M.R.), Elterninitiative Kinderkrebsklinik e.V. (M.R., J.B.), the Gert-und-Susanna-Meyer foundation (M.R.), Forschungskommission Heinrich Heine University (M.R., N.Q.), the Ministère Français de l’Enseignement Supérieur et de la Recherche (M.Z.), ‘Courir pour la Vie, Courir pour Curie’ and his president Dominique Ancelin, the King Baudouin Foundation (A.F.), ITMO Cancer AVIESAN (National Alliance for Life Sciences and Health), within the framework of the Plan Cancer 2014–2019 and convention “2018, Non-coding RNA in cancerology: fundamental to translational”, “iPC—individualized Pediatric Cure (ref. 826121)”, Robert J. Arceci Innovation Award from St. Baldrick’s Foundation (O.A and J.S), CNRS/INSERM and Institute Curie (O.A.). A.K.B thanks the Novo Nordisk Foundation for support through a NNF Professorship (NNFSA170028392). M.R. was supported by operating funds from the Pediatric Brain Tumor Foundation.
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Open Access funding enabled and organized by Projekt DEAL.
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M.R., J.B., O.A. and G.R. planned and directed the study. J.B. designed and performed in vitro experiments supported by F.B, J.T, G.C., I.M.K., M.W., L.B., D.Pa., V.M., M.K., C.Mö., D.B., F.K., T.B., C.Mu and S.G. F.B., M.Z., and A.F. conducted in vivo experiments with support from G.C. and H.Y. D.Pi. analyzed RNA sequencing data and provided bio-informatics analysis and F-D.M. carried out RNA sequencing sample preparation. N.Q. designed overexpression strategies. Q.G. and P.A.N. provided H3K27ac ChIP-sequencing profile data and visualized data. S.N. carried out Bio-Layer interferometry experiments and design, and analyses were done by A.B., D.W. and G.S. M.L. performed proteomic sample preparation and A.S., K.S. analyzed proteomic data. B.S., B.R., J.T., J.S., S.D., V.R., A.O., U.F., G.L., M.Z., and M.D.T. provided intellectual contributions to the project and to the interpretation of the results. G.S. performed in silico experiments. M.K., H.S., P.L., and S.M.P. provided methylation and RNA sequencing data and supported the analysis of data. J.B., M.Z., M.R., O.A., A.B. and G.R. wrote the manuscript with support of S.M.P, M.K., J.S., J.T., P.L., S.D. and M.D.T. Figures were designed and drafted by J.B., F.B., M.R., G.R., M.Z., and O.A. All authors edited and contributed to the final manuscript.
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Guido Reifenberger received honoraria for advisory boards from Abbvie and Sven Diederichs is co-owner of siTOOLs Biotech, Martinsried, Germany. The remaining authors declare no competing interest.
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Nature Communications thanks Agnieszka Bronisz, Yutaka Kondo, Jer-Yen Yang and the other, anonymous, reviewer(s) for their contribution to the peer review of this work.
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Bartl, J., Zanini, M., Bernardi, F. et al. The HHIP-AS1 lncRNA promotes tumorigenicity through stabilization of dynein complex 1 in human SHH-driven tumors. Nat Commun 13, 4061 (2022). https://doi.org/10.1038/s41467-022-31574-z
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DOI: https://doi.org/10.1038/s41467-022-31574-z