ECB-ART-50267
Toxics
2022 Jun 14;106:. doi: 10.3390/toxics10060325.
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Gene Expression Analysis of the Stress Response to Lithium, Nickel, and Zinc in Paracentrotus lividus Embryos.
Bonaventura R
,
Costa C
,
Deidda I
,
Zito F
,
Russo R
.
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Many anthropogenic pollutants such as metals are discharged into the marine environment through modern sources. Among these, lithium (Li), nickel (Ni), and zinc (Zn) can interfere with biological processes in many organisms when their concentration rises. These metals are toxic to sea urchin embryos, affecting their development. Indeed, animal/vegetal and dorso/ventral embryonic axes are differently perturbed: Li is a vegetalizing agent, Ni can disrupt dorso-ventral axis, Zn can be animalizing. To address the molecular response adopted by embryos to cope with these metals or involved in the gene networks regulating embryogenesis, and to detect new biomarkers for evaluating hazards in polluted environments in a well-known in vivo model, we applied a high-throughput screening approach to sea urchin embryos. After fertilization, Paracentrotus lividus embryos were exposed to Li, Ni, and Zn for 24/48 h. At both endpoints, RNAs were analyzed by NanoString nCounter technology. By in silico analyses, we selected a panel of 127 transcripts encoding for regulatory and structural proteins, ranked in categories: Apoptosis, Defense, Immune, Nervous, Development, and Biomineralization. The data analysis highlighted the dysregulation of many genes in a metal-dependent manner. A functional annotation analysis was performed by the KEEG Orthology database. This study provides a platform for research on metals biomarkers in sea urchins.
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Figure 1. Morphologies of P. lividus embryos treated with Li, Ni, and Zn. (A) Schematic drawing of Li, Ni and Zn treatment experiments. Black line, hpf, in the upper part; the first vertical arrow indicates addition of 30 mM LiCl (Li), 0.5mM NiCl2 (Ni), 0.1mM ZnSO4 (Zn) at 0.5 hpf. Periods of treatment with Li, orange line; Ni, red line; Zn, yellow line. Untreated embryos (CTR), blue line. s/o indicates sampling (s) for NanoString nCounter gene expression assay and qPCR analyses and (o) microscopic observation. Embryos were observed at 24 (BâE) and 48 (FâI) hours post-fertilization (hpf). Untreated embryos: (B) control gastrula; (F) control pluteus. (C,G) Li-embryos; (D,H) Ni-embryos; (E,I) Zn-embryos. Blue ellipses in (D,H) indicate short archenteron. Black arrows in (D,E) indicate cells grouped inside the blastocoelic cavity. Red arrows in (F,G) indicate pigment cells. Schemes of embryos at 48 hpf: control pluteus, CTR (J); Li-embryo, Li (K); Ni-embryo, Ni (L); Zn-embryo, Zn (M). Animal/Vegetal (A/V), Dorso/Ventral (D/V) axes are indicated in the scheme of pluteus embryo. (NâQ) Anti-Sox2 antibody (red); (RâU) Ab-295 (green); (VâY) Merged images (yellow) of the relative Anti-Sox2 (NâQ) and Ab-295 (RâU) images, respectively. The image in the white frame in (N) indicates 1.4à magnification of the pluteus apex, where brightness and contrast have been increased. White arrows in (NâQ) indicate Sox2-positive cells. White ellipses in (R) indicate small central ganglionic structures. White arrows in (RâT) and (VâX) indicate ciliary band. Bar 20 μm for (BâI) and (NâY). |
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Figure 2. Heat map of the 127 genes analyzed following metal treatments. The heat map was generated using conditional formatting on Microsoft Excel. Genes are reported in alphabetical order. Violet, green, and light yellow indicate fold values <â2, >+2 and between â2 and +2, respectively; light blue indicates not quantifiable genes. Li, embryos treated with 30 mM LiCl; Ni, embryos treated with 0.5 mM NiCl2; Zn, embryos treated with 0.1 mM ZnSO4. Hpf, hours post-fertilization. |
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Figure 3. Percentages of genes modulated by metal treatments. Percentages of genes modulated by Li (30 mM LiCl), Ni (0.5 mM NiCl2) and Zn (0.1 mM ZnSO4) treatments at 24 and 48 hpf (hours post-fertilization). The fill colors indicate the upregulated genes in green (>+2), downregulated genes in violet (<â2), not responsive in light yellow (between â2 and +2), and not quantifiable (nq) in light blue. |
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Figure 4. Apoptosis, Defense, Immune, and Nervous genes are modulated by Li, Ni, and Zn treatments. The grey boxes indicate the threshold for insignificant changes following Li, Ni, and Zn treatments, i.e., fold values between â2 and + 2 at 24 (A) and 48 (B) hours post-fertilization (hpf). Symbols in the plot at 24 hpf (A): light blue rhombus, Li-embryos; orange square, Ni-embryos; light green triangle, Zn-embryos. Symbols in the plot at 48 hpf (B): blue rhombus, Li-embryos; red square Ni-embryos; green triangle, Zn-embryos. Ap, Apoptosis genes; Def, Defense genes; Imm, Immune genes; Ner, Nervous genes. |
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Figure 5. Development genes modulated by Li, Ni, and Zn treatments. The grey boxes indicate the threshold for insignificant changes following Li, Ni, and Zn treatments, i.e., fold values between â2 and + 2 at 24 (A) and 48 (B) hours post-fertilization (hpf). Symbols in the plot at 24 hpf (A): light blue rhombus, Li-embryos; orange square, Ni-embryos; light green triangle, Zn-embryos. Symbols in the plot at 48 hpf (B): blue rhombus, Li-embryos; red square Ni-embryos; green triangle, Zn-embryos. Some Development genes were organized considering their dorsal and ventral ectoderm expression. Asterisks (*) indicate genes also expressed in other territories. |
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Figure 6. Development and Biomineralization genes with endomesoderm and mesoderm (primary mesenchyme cells, PMCs) expression modulated by Li, Ni, and Zn treatments. The grey boxes indicate the threshold for insignificant changes following Li, Ni, and Zn treatments, i.e., fold values between â2 and + 2, at 24 (A) and 48 (B) hours post-fertilization (hpf). Symbols in the plot at 24 hpf (A): light blue rhombus, Li-embryos; orange square, Ni-embryos; light green triangle, Zn-embryos. Symbols in the plot at 48 hpf (B): blue rhombus, Li-embryos; red square Ni-embryos; green triangle, Zn-embryos. The Development genes here considered have endomesoderm expression. Biomineralization genes, mainly expressed by the PMCs, were organized taking into consideration their functions, i.e., transcription factors (TFs), signaling molecules (signaling), and skeleton structures (skeleton). Asterisks (*) indicate genes also expressed in other territories. |
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Figure 7. Comparison of qPCR data of gene transcription levels in Li-, Ni-, and Zn-embryos with NanoString data. Pl-alx1, Pl-can, Pl-gal8, Pl-jun, Pl-mt, and Pl-sox9 mRNA levels were analyzed compared to control embryos using the endogenous gene Pl-Z12-1 for normalization. The gray boxes indicate the threshold for insignificant changes following Li, Ni, and Zn treatments, i.e., fold values between â2 and + 2, at 24 (A) and 48 (B) hours post-fertilization (hpf). Symbols: NanoS, NanoString data, blue bars; qPCR data, red bars; Li, Li-embryos; Ni, Ni-embryos, Zn, Zn-embryos. The light blue triangles indicate not quantifiable values. Each bar of qPCR data represents the mean of three independent experiments of qPCR ± SD. QPCR mean values were significantly different according to the one-way ANOVA (p < 0.05), followed by the Tukeyâs test. The asterisks (*) indicate statistically not significant variations to the relative control. |
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Figure 8. Venn diagrams reporting the numbers of modulated genes in different subgroups, i.e., in Li, Ni, Zn, Li/Ni, Li/Zn, Ni/Zn, and Li/Ni/Zn. Modulated genes at 24 (A) and 48 (B) hours post-fertilization (hpf). The table below reports the numbers of down- and up-regulated genes in each group. |
References [+] :
Andrikou,
Myogenesis in the sea urchin embryo: the molecular fingerprint of the myoblast precursors.
2013, Pubmed,
Echinobase
Andrikou, Myogenesis in the sea urchin embryo: the molecular fingerprint of the myoblast precursors. 2013, Pubmed , Echinobase
Anishchenko, SoxB2 in sea urchin development: implications in neurogenesis, ciliogenesis and skeletal patterning. 2018, Pubmed , Echinobase
Arshinoff, Echinobase: leveraging an extant model organism database to build a knowledgebase supporting research on the genomics and biology of echinoderms. 2022, Pubmed , Echinobase
Barsi, Genome-wide assessment of differential effector gene use in embryogenesis. 2015, Pubmed , Echinobase
Beere, Death versus survival: functional interaction between the apoptotic and stress-inducible heat shock protein pathways. 2005, Pubmed
Blewett, Mechanisms of nickel toxicity to fish and invertebrates in marine and estuarine waters. 2017, Pubmed
Bonaventura, Combined Effects of Cadmium and UVB Radiation on Sea Urchin Embryos: Skeleton Impairment Parallels p38 MAPK Activation and Stress Genes Overexpression. 2015, Pubmed , Echinobase
Bonaventura, A preliminary gene expression analysis on Paracentrotus lividus embryos exposed to UVB, Cadmium and their combination. 2021, Pubmed , Echinobase
Bonaventura, Stress response gene activation protects sea urchin embryos exposed to X-rays. 2011, Pubmed , Echinobase
Bonaventura, Nickel toxicity in P. lividus embryos: Dose dependent effects and gene expression analysis. 2018, Pubmed , Echinobase
Caito, Neurotoxicity of metals. 2015, Pubmed
Ch Ho, Perturbation of gut bacteria induces a coordinated cellular immune response in the purple sea urchin larva. 2016, Pubmed , Echinobase
Costa, Phylogenetic analysis and expression patterns of p16 and p19 in Paracentrotus lividus embryos. 2012, Pubmed , Echinobase
Croce, ske-T, a T-box gene expressed in the skeletogenic mesenchyme lineage of the sea urchin embryo. 2001, Pubmed , Echinobase
Croce, Coquillette, a sea urchin T-box gene of the Tbx2 subfamily, is expressed asymmetrically along the oral-aboral axis of the embryo and is involved in skeletogenesis. 2003, Pubmed , Echinobase
Cui, Specific functions of the Wnt signaling system in gene regulatory networks throughout the early sea urchin embryo. 2014, Pubmed , Echinobase
da Silva, Overexpression and mechanistic characterization of blastula protease 10, a metalloprotease involved in sea urchin embryogenesis and development. 2006, Pubmed , Echinobase
Davidson, A provisional regulatory gene network for specification of endomesoderm in the sea urchin embryo. 2002, Pubmed , Echinobase
Davidson, Specification of cell fate in the sea urchin embryo: summary and some proposed mechanisms. 1998, Pubmed , Echinobase
DeForest, Species sensitivity distribution evaluation for chronic nickel toxicity to marine organisms. 2013, Pubmed , Echinobase
Duloquin, Localized VEGF signaling from ectoderm to mesenchyme cells controls morphogenesis of the sea urchin embryo skeleton. 2007, Pubmed , Echinobase
Fujita, Purification of EGIP-D-binding protein from the embryos of the sea urchin Anthocidaris crassispina. 1997, Pubmed , Echinobase
Ghiglione, Cell-autonomous expression and position-dependent repression by Li+ of two zygotic genes during sea urchin early development. 1993, Pubmed , Echinobase
Goldstone, The chemical defensome: environmental sensing and response genes in the Strongylocentrotus purpuratus genome. 2006, Pubmed , Echinobase
Hardin, Commitment along the dorsoventral axis of the sea urchin embryo is altered in response to NiCl2. 1992, Pubmed , Echinobase
Hinman, Embryonic neurogenesis in echinoderms. 2018, Pubmed , Echinobase
Hwang, Differential gene expression patterns during embryonic development of sea urchin exposed to triclosan. 2017, Pubmed , Echinobase
Jaishankar, Toxicity, mechanism and health effects of some heavy metals. 2014, Pubmed
Karakostis, Characterization of an Alpha Type Carbonic Anhydrase from Paracentrotus lividus Sea Urchin Embryos. 2016, Pubmed , Echinobase
Kavanagh, Lithium in the Natural Waters of the South East of Ireland. 2017, Pubmed
Kozmik, Pax genes in eye development and evolution. 2005, Pubmed
Lapraz, RTK and TGF-beta signaling pathways genes in the sea urchin genome. 2006, Pubmed , Echinobase
Livak, Analysis of relative gene expression data using real-time quantitative PCR and the 2(-Delta Delta C(T)) Method. 2001, Pubmed
López-Landavery, Transcriptomic response and hydrocarbon accumulation in the eastern oyster (Crassostrea virginica) exposed to crude oil. 2019, Pubmed
Manji, Signaling: cellular insights into the pathophysiology of bipolar disorder. 2000, Pubmed
Martik, Deployment of a retinal determination gene network drives directed cell migration in the sea urchin embryo. 2015, Pubmed , Echinobase
Martik, Developmental gene regulatory networks in sea urchins and what we can learn from them. 2016, Pubmed , Echinobase
Martino, Gadolinium perturbs expression of skeletogenic genes, calcium uptake and larval development in phylogenetically distant sea urchin species. 2018, Pubmed , Echinobase
McIntyre, Short-range Wnt5 signaling initiates specification of sea urchin posterior ectoderm. 2013, Pubmed , Echinobase
Molina, Nodal: master and commander of the dorsal-ventral and left-right axes in the sea urchin embryo. 2013, Pubmed , Echinobase
Molina, Maternal factors regulating symmetry breaking and dorsal-ventral axis formation in the sea urchin embryo. 2020, Pubmed , Echinobase
Nemer, An altered series of ectodermal gene expressions accompanying the reversible suspension of differentiation in the zinc-animalized sea urchin embryo. 1986, Pubmed , Echinobase
Oliveri, Repression of mesodermal fate by foxa, a key endoderm regulator of the sea urchin embryo. 2006, Pubmed , Echinobase
Pascual-Vargas, A Role for Frizzled and Their Post-Translational Modifications in the Mammalian Central Nervous System. 2021, Pubmed
Piacentino, RNA-Seq identifies SPGs as a ventral skeletal patterning cue in sea urchins. 2016, Pubmed , Echinobase
Poustka, A global view of gene expression in lithium and zinc treated sea urchin embryos: new components of gene regulatory networks. 2007, Pubmed , Echinobase
Poustka, On the origin of the chordate central nervous system: expression of onecut in the sea urchin embryo. 2004, Pubmed , Echinobase
Prokopec, Systematic evaluation of medium-throughput mRNA abundance platforms. 2013, Pubmed
Range, Integration of canonical and noncanonical Wnt signaling pathways patterns the neuroectoderm along the anterior-posterior axis of sea urchin embryos. 2013, Pubmed , Echinobase
Robert, A comprehensive survey of wnt and frizzled expression in the sea urchin Paracentrotus lividus. 2014, Pubmed , Echinobase
Russo, The newly characterized Pl-jun is specifically expressed in skeletogenic cells of the Paracentrotus lividus sea urchin embryo. 2014, Pubmed , Echinobase
Russo, Response to metals treatment of Fra1, a member of the AP-1 transcription factor family, in P. lividus sea urchin embryos. 2018, Pubmed , Echinobase
Russo, Time- and dose-dependent gene expression in sea urchin embryos exposed to UVB. 2014, Pubmed , Echinobase
Russo, Transcriptional increase and misexpression of 14-3-3 epsilon in sea urchin embryos exposed to UV-B. 2010, Pubmed , Echinobase
Ryu, Identification of nickel response genes in abnormal early developments of sea urchin by differential display polymerase chain reaction. 2012, Pubmed , Echinobase
Saudemont, Ancestral regulatory circuits governing ectoderm patterning downstream of Nodal and BMP2/4 revealed by gene regulatory network analysis in an echinoderm. 2010, Pubmed , Echinobase
Shimada, Neuroprotective function of 14-3-3 proteins in neurodegeneration. 2013, Pubmed
Solek, An ancient role for Gata-1/2/3 and Scl transcription factor homologs in the development of immunocytes. 2013, Pubmed , Echinobase
Suh, Hypoxia-modulated gene expression profiling in sea urchin (Strongylocentrotus nudus) immune cells. 2014, Pubmed , Echinobase
Thibon, Large-scale survey of lithium concentrations in marine organisms. 2021, Pubmed
Thompson, From sea squirts to squirrelfish: facultative trace element hyperaccumulation in animals. 2018, Pubmed
Tu, Sea urchin Forkhead gene family: phylogeny and embryonic expression. 2006, Pubmed , Echinobase
Wakamatsu, The many faces of Sox2 function in neural crest development. 2021, Pubmed
Wang, Metalloimmunology: The metal ion-controlled immunity. 2020, Pubmed
Yılmaz, Review of heavy metal accumulation on aquatic environment in Northern East Mediterrenean Sea part I: some essential metals. 2017, Pubmed
Zito, Expression of univin, a TGF-beta growth factor, requires ectoderm-ECM interaction and promotes skeletal growth in the sea urchin embryo. 2003, Pubmed , Echinobase
Zito, Pl-nectin, a discoidin family member, is a ligand for betaC integrins in the sea urchin embryo. 2010, Pubmed , Echinobase
Zito, Ectoderm cell--ECM interaction is essential for sea urchin embryo skeletogenesis. 1998, Pubmed , Echinobase