Abstract
Investigating the in vivo role of tumor suppressor genes in cancer is technically challenging due to their essential requirement during early animal development. To address this bottleneck, we generated genetic mosaic adult zebrafish using TALEN genome editing and demonstrate somatic inactivation of the tumor suppressor retinoblastoma1 (rb1) induces tumorigenesis at high frequency. 11–33% of 1-cell stage embryos injected with TALEN mRNAs targeting rb1 exon 2 or 3 develop tumors beginning as early as 3.5 months of age. Lesions predominantly arise in the brain and show features of neuroectodermal-like and glial-like tumors. Mutant allele analysis is consistent with tumor initiation due to somatic inactivation of rb1, revealing a conserved role for rb1 in tumor suppression across vertebrates. In contrast to genetic mosaics, heterozygous rb1−/+ adults show no evidence of neoplasia, while homozygous mutant rb1−/− are larval lethal. This is the first demonstration that somatic inactivation of a tumor suppressor causes cancer in zebrafish and highlights the utility of site-specific nucleases to create genetic mosaic zebrafish for tumor suppressor gene discovery. Somatic inactivation with site-directed nucleases in zebrafish presents a rapid and scalable strategy to study tumor suppressor gene function in cancer.
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Introduction
Targeted somatic inactivation of tumor suppressor genes in genetic mosaic animals enables investigation of their roles in carcinogenesis if they are embryonic lethal. Mouse and zebrafish models of human cancer frequently require crosses with multiple transgenic lines to create conditional gene knockouts in predisposed mutant backgrounds1,2,3,4. Genome editing nucleases are emerging as a highly efficient alternative strategy for inactivating gene function in somatic tissues. TAL effector nucleases (TALENs) were first used for somatic gene inactivation to study vascular system development in zebrafish embryos5. Adult phenotypes have also been created in zebrafish and mice with CRISPR/Cas9 nuclease genome editing. In zebrafish, tissue specific CRISPR/Cas9s have been used for targeted gene knockout in the hematopoietic system6. Nuclease targeted somatic inactivation was successfully used in adult mice to investigate cooperating genes during liver and lung carcinogenesis7,8. Most recently, malignant brain tumor models were developed using CRISPR/Cas9 somatic inactivation of multiple tumors suppressors in embryonic and neonatal mouse brain9. Multiplex gene targeting with site directed nucleases simplifies the process of creating complex genotypes that normally require numerous genetic crosses. In addition, targeting nucleases allow for introduction of a range of loss of function alleles in addition to complete gene knockouts10,11.
The central role of the retinoblastoma tumor suppressor Rb1 in human cancer is well established. The Rb protein family’s main tumor suppressive role is in regulation of cell cycle entry through interaction with E2F transcription factors12. Rb1 function also intersects with pathways controlling cellular senescence, apoptosis, DNA repair and chromosome integrity13,14. Mutation or alteration of the Rb1 pathway is detected in the majority of human adult gliomas15,16. The role of Rb1 in specific cancers has been studied in mice by germline mutation17,18 and somatic inactivation with conditional or tissue specific knockouts19,20. Targeted and conditional knockout of Rb1 in combination with tp53, PTEN, or Nf1 tumor suppressors in astrocytes and neural progenitors in adult mice induces malignant brain tumors21,22,23,24,25,26, consistent with the predicted role for these genes in preventing cellular transformation in progenitor cell populations in the brain. Combinatorial deletion of tumor suppressors with or without Rb1 was shown to influence brain tumor phenotypes, indicating genetic disruption of cell cycle regulation in progenitors favors formation of primitive neuroectodermal tumors over glioma26.
Here we present a proof of principle study in zebrafish that shows genome editing nucleases can be used to study tumor suppressor gene function by targeted somatic inactivation. We demonstrate that TALEN-mediated targeting of rb1 results in highly penetrant tumor formation in genetic mosaic adults. The zebrafish rb1 tumor suppressor is an essential gene that functions in retinal neural progenitor proliferation and cell fate specification27. However, its role in cancer has not been previously studied in zebrafish. Heterozygous adult fish with stable germline rb1 frameshift alleles did not develop lesions or tumors. In contrast, genetic mosaic adults develop tumors, predominantly in the brain, with varying degrees of proliferation and histological features of neuroectodermal-like or glial-like tumors. The majority of mutant rb1 alleles in somatic, germline and brain tumor tissues were frameshift mutations. In tumor tissue only one or two frameshift alleles were present and overrepresented compared to wild type tissue. Together, the data indicate that biallelic inactivation of rb1 in somatic tissue underlies neoplastic transformation and tumor initiation. Predisposing zebrafish to brain tumors by somatic inactivation of rb1 with site-specific nucleases will be useful for investigating pathways cooperating in brain tumorigenesis. Nuclease gene targeting in zebrafish presents a rapid and simple method to screen potentially hundreds of candidate tumor suppressor genes that impact carcinogenesis.
Results and Discussion
We used TALEN targeting to isolate germline mutations in the zebrafish retinoblastoma1 (rb1) tumor suppressor gene. Single cell embryos were injected with 150 or 200 pg of TALEN mRNA targeting rb1 exon 2 or 12.5 to 50 pg of TALEN mRNA targeting rb1 exon 3 (Supplementary Figure S1). rb1 exon 2 TALENs were highly efficient, obtaining up to 100% biallelic inactivation in 50% of injected embryos. Lower mutagenesis efficiency was observed with rb1 exon 3 TALENs and increased doses caused high toxicity and mortality. We screened three adults for germline transmission and recovered four new rb1 alleles in exon 2, two frameshift deletions Δ4 and Δ7 and two in frame deletion Δ9 and Δ12 (Supplementary Figure S1). Homozygous Δ4 and Δ7 larvae failed to develop a swim bladder and died at ~7 days post fertilization, as reported previously for the rb1 mutant space cadet27. Normal development and viability was observed in the in frame deletion Δ9 and Δ12 homozygotes.
During the course of this study, we observed that the genetic mosaic adults generated by somatic inactivation of rb1 in embryos develop tumors in the head region at high frequency (Fig. 1). Beginning at 3.5 months of age, fish that were injected with rb1 TALENs as embryos presented with tissue masses protruding out over the eyes and causing malformation of the skull (Fig. 1b, arrows). At 1.5 years post fertilization, tumor penetrance in rb1 exon 2 and exon 3 TALEN injected fish was 33% (29/87 adults) and 11% (29/275), respectively (Table 1). The heads from 52/58 adults were dissected and revealed abnormal brain morphology disrupted by large masses. The remaining 6 adults with lesions in the head region were not further analyzed (Table 1, “unknown”). Adults often displayed abnormal swimming behavior before overt appearance of masses in the head region, providing an early indicator of brain lesions in the affected animal. In contrast, heterozygous rb1−/+ adults carrying either of the established rb1 frameshift alleles do not develop tumors and are behaviorally normal.
Serial sections of 14/52 dissected brains in eight exon 2-targeted and six exon 3-targeted fish revealed 12 neoplastic mass lesions that infiltrated and effaced the neuropil and two brains with expanded glial rests (Table 1). The remaining dissected brains were not analyzed by histology for tumor characterization (Table 1 “not analyzed by histology)”. Most tumors exhibited numerous mitoses and variable numbers of individually apoptotic cells. Prominent vasculature was generally not a feature of individual tumors. Tumors exhibited a range of histological features (Fig. 2 and Table 1), but the majority (7/12) exhibited histological features suggestive of neuroectodermal-like tumors, including hyperchromatic or oval/wedge-shaped nuclei with rosette formation (Fig. 2a,b) or multilayered tubular structures (Fig. 2c). Four of 12 tumors contained features more consistent with glial-like tumors (Fig. 2d) or mixed glial-like tumors (Fig. 2e). The remaining two brains revealed proliferative cell populations that appeared to arise from glial rests (glial cells that are retained from embryonal neurogenesis), without formation of a clear mass lesion (Fig. 2f).
Two brain tumors from exon 2 and exon 3 targeted fish were analyzed by immunohistochemistry for identification of proliferating cells and expression of glial and neuronal markers. Consistent with the observation of mitotic figures in hematoxylin and eosin sections (Fig. 2d), many cells expressing phospho-histone H3 were observed in different regions of each tumor (Fig. 3d,e; Supplementary Figure 2). In one brain, the overall structure appeared mostly normal, but the lateral division of the valvula cerebelli contained numerous proliferating cells not observed in wild type (Supplementary Figure 2). Images of glial and neuronal differentiation markers labeling wild type brain and a representative brain tumor are shown in Fig. 3. The glial marker S100 and neuronal markers HuC/D and SV2 were detected within less disrupted regions of the tumor positive brain including the parenchyma (Fig. 3g,j,m), which may represent non-neoplastic cells. These regions frequently showed infiltration of neoplastic cells (Fig. 3g,j,m). Expression of S100 within densely cellular regions of the tumors was limited to a few cells with similar appearance to astrocytes (Fig. 3h), although the presence of stellate astrocytes in the midbrain of adult zebrafish has not been reported28. Little to no expression of neuronal markers HuC/D and SV2 was observed in these tumor regions (Fig. 3k,n). The lack of expression of differentiation markers for glia (S100) and neurons (HuC/D and SV2) suggests the tumors may lack differentiated cell types, but this is not definitive. Together, the data suggest that somatic inactivation of rb1 results in brain tumors that are highly infiltrative with diverse histological features.
The frequency of rb1 mutant alleles in tumor and adult tissues was examined to confirm that rb1 somatic inactivation correlated with brain tumor induction in adult fish (Fig. 4). Targeted rb1 exons 2 and 3 were sequenced in tumor, retina, muscle and germline tissue from four tumor positive fish ranging in age from 3.5 months to one year. In all tumor tissues (4/4) the frequency of rb1 mutant alleles was consistently higher than wild type alleles (68%–87% of cloned amplicons represented indels; Supplementary Table 1). Only one or two specific rb1 alleles were present in 3 out of 4 tumors. Of the 10 alleles recovered in the tumor tissue, 8 of the 10 were frameshift mutations. In contrast, the mutation frequency in retinal, muscle and germline tissues was highly variable (3%–100%) and was as high as 7 different mutant rb1 alleles in one fish (Supplementary Table 1). The presence of predominantly loss of function alleles in genetic mosaic fish that develop tumors is consistent with biallelic inactivation of rb1 initiating the pathway to transformation. However, the possibility that additional mutations in the genome caused by off targeting contributed to tumor induction cannot be ruled out. The high efficiency of TALENs targeting rb1 exon 2 produced 19 different indels, with five specific to tumor tissue (Fig. 4a). Remarkably, only two exon 3 frameshift alleles, Δ11 and Δ19, were recovered in the normal and tumor tissues from fish targeted with the low efficiency exon 3 TALENs (Fig. 4b). The high degree of mutagenesis was consistent with tumor growth from a neoplastic cell population transformed by inactivation of rb1.
In summary, we demonstrate that targeted somatic inactivation of the rb1 tumor suppressor in zebrafish embryos using two independent TALEN pairs results in genetic mosaic adults that develop tumors at high frequency, predominantly located in the brain. Pathological and immunohistochemical analyses of the head in affected individuals indicate zebrafish can be predisposed to neuroectodermal-like and glial-like tumors by somatic inactivation of rb1 with site-specific nucleases. In contrast to genetic mosaic animals, adult rb1–/+ heterozygotes with a stable germline rb1 mutation do not develop tumors. This suggests that nuclease targeting induces biallelic inactivation at the rb1 locus and sensitizes cells to transformation. It has been proposed that in the case of epithelial cancers, tumor initiating cells may arise from a dedifferentiating progenitor population of transit amplifying cells29. Similar mechanisms may drive neoplasms derived from the neurogenic cell populations in the brain. In support of this, mouse models of pediatric and adult brain tumors have been created by targeting tumor suppressor gene knockout, oncogene activation and insertional transposon mutagenesis to neural stem and progenitor cells in the brain21,22,23,24,25,26,30,31,32,33. Our observations are consistent with previously published zebrafish models of brain cancer generated by driving overexpression of activated Ras34,35 in neural and glial progenitor cells. Adapting a tissue specific CRISPR targeting method6 to inactivate genes in neural progenitors in combination with zebrafish brain cancer models35,36,37 will be useful for investigating cooperating pathways promoting tumorigenesis. Our study demonstrates the potential for rapid large scale screening of candidate tumor suppressors in zebrafish using genome-editing nucleases to generate genetic mosaics.
Methods
Zebrafish care and husbandry
Zebrafish were reared in an Aquatic Habitat system from Aquatic Ecosystems, Inc. and maintained at 27 oC on a 14 hr light/10 hr dark cycle. The WIK wild type strain used in this study was obtained from the Zebrafish International Research Center (http://zebrafish.org/zirc/home/guide.php). Experimental protocols were approved by the Iowa State University Institutional Animal Care and Use Committee (Log # 11-06-6252-I). The protocols are in compliance with American Veterinary Medical Association and the National Institutes of Health guidelines for the humane use of laboratory animals in research. Adult fish were anesthetized and euthanized in MS-222 Tricaine Methanesulfonate and tissue dissection was carried out according to experimental protocols approved by the Iowa State University Institutional Animal Care and Use Committee (Log # 11-06-6252-I) in compliance with the American Veterinary Medical Association and the National Institutes of Health guidelines for the humane use of laboratory animals in research. NIH/Office of Animal Care and Use/Animal Research Advisory committee (ARAC) Guidelines for endpoint in neoplasia studies (oacu.od.nih.gov/ARAC/Guidelines for Endpoints in Animal Study Proposals) were used to establish a humane endpoint in the zebrafish rb1 TALEN injected fish. Adult fish were monitored for general appearance, size, length, viability and morbidity relative to control siblings daily during routine feeding. Fish were closely monitored bi-weekly for gross presentation of cranial tumors. Fish from each injection experiment were sacrificed before tumor burden reached 3 mm in size/25 mg in weight, constituting less than 10% of the total body weight of an adult fish (300–500 mg), as outlined for mouse and rat studies38, or by 1.5 year of age, whichever endpoint was reached first. The swimming behavior of some rb1 TALEN injected fish was adversely affected before gross presentation of cranial tumors, possibly due to tumor location. These fish were sacrificed although tumor burden was less than 3 mm/10% of body weight.
rb1 TALEN assembly, targeting and allele analysis
TALENs targeting rb1 exon 2 or exon 3 were designed using TAL Effector Nucleotide Targeter 2.0 at https://tale-nt.cac.cornell.edu/node/add/talen-old39 and assembled in the modified GoldyTALEN scaffold5. 150–200 pg of exon 2 or 12.5–50 pg of exon 3 TALEN mRNA was injected into 1-cell stage wild type WIK embryos. TALEN efficiency was determined by assaying individual injected embryos for disruption of restriction enzyme sites in a PCR amplicon spanning the target site. Genomic DNA was extracted from embryos and adult fin clips by placing tissue in 50 μl 50 mM NaOH and heating at 95 oC for 30 minutes. For rb1 allele frequency analysis, genomic DNA was isolated from tumor, somatic and germline tissues using a DNeasy Blood and Tissue Kit (Qiagen). Amplicons were TOPO cloned (Invitrogen) and 50–100 individual clones sequenced per sample. Primers used for amplification of rb1 exons: exon 2 F-5’- TTTCCAGACACAAGGACAAGG-3’, R-5’-GCGGTAAAGCAGATATCAGAAGA -3’; exon 3 F-5’-TTTCCAGACACAAGGACAAGG-3’, R-5’-CCTCACAAGACTGATGAACTGC-3’ or F-5’-TTACCGCACTTGTGTTTTGG-3’, R-5’-TGCCACACATACCTCAGACC-3’.
Histopathology and Immunohistochemistry
Adult zebrafish were sacrificed and head tissue processed for histopathology and immunohistochemistry as described previously40. For histopathology tissues fixed in Davidson’s or 10% Formalin (Fisher) were decalcified in Cal-Ex (Fisher) and paraffin embedded at the Iowa State University Clinical Histopathology Laboratory. 6 um sections were stained with Hematoxylin 7211 Richard-Allan Scientific (Fisher) and 3% Eosin Y (Argos Organics). For immunohistochemistry heads were fixed in 4% paraformaldehyde, decalcified in 12% EDTA and embedded in Tissue-Tek optimal cutting temperature medium (Sakura). 14 um tissue sections were labeled with antibodies anti-phosphohistone-H3 (1:100, Upstate), anti-S100 (1:250, Dako). Secondary antibodies were conjugated with HRP. Tissues were counterstained with modified Mayer’s Hematoxylin (Fisher) and eosin. Slides were photographed on a Zeiss Axiophot using a Nikon Rebel camera and on a Zeiss confocal LSM 700.
Additional Information
How to cite this article: Solin, S. L. et al. Rapid tumor induction in zebrafish by TALEN-mediated somatic inactivation of the retinoblastoma1 tumor suppressor rb1. Sci. Rep. 5, 13745; doi: 10.1038/srep13745 (2015).
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Acknowledgements
The authors thank Dr. Stephen Ekker and Dr. Stephen Johnson for discussion of this work. Jordan Welker, Jennifer Groeltz-Thrush, Laura Schultz and Jasmine Linn assisted with experiments. This work was supported by grant #14-4418 from the Roy J. Carver Charitable Trust (M. McGrail).
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S.L.S. and M.M. wrote the manuscript; S.L.S. performed experiments; H.R.S. and K.D.W. performed histopathological analysis; S.L.S., J.J.E. and M.M. conceived and designed experiments.
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Solin, S., Shive, H., Woolard, K. et al. Rapid tumor induction in zebrafish by TALEN-mediated somatic inactivation of the retinoblastoma1 tumor suppressor rb1. Sci Rep 5, 13745 (2015). https://doi.org/10.1038/srep13745
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DOI: https://doi.org/10.1038/srep13745
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