Adult, embryonic and fetal hemoglobin are expressed in human glioblastoma cells
- Authors:
- Published online on: November 22, 2013 https://doi.org/10.3892/ijo.2013.2186
- Pages: 514-520
Abstract
Introduction
Globins are hemo-containing proteins, have the ability to bind gaseous ligands [oxygen (O2), nitric oxide (NO) and carbon monoxide (CO)] reversibly. They have been described in prokaryotes, fungi, plants and animals with an enormous diversity of structure and function (1). To date, hemoglobin, myoglobin, neuroglobin (Ngb) and cytoglobin (Cygb) represent the vertebrate globin family with distinct function and tissue distributions (2). During ontogeny, developing erythroblasts sequentially express embryonic {[Gower 1 (ζ2ε2), Gower 2 (α2ε2), and Portland 1 (ζ2γ2)] to fetal [Hb F(α2γ2)] and then adult [Hb A (α2β2), 97%; Hb A2 (α2δ2), <3%]} hemoglobin (3). Adult hemoglobin, the most well studied globin in terms of structure, function and evolution (5), consists of two α and β polypeptides globin chains (heterotetrameric protein) where each globin molecule contains a hydrophobic pocket that non-covalently binds an iron-protoporphyrin IX molecule (4).
In contradiction to previous thought, recently hemoglobin has been reported to be expressed not only in enucleated red cells, but also in other cell types. Hemoglobin expression has been reported in rodent brain (neurons of the cortex, hippocampus and cerebellum but not astrocytes and oligodendrocytes) (6); embryonic and adult mouse endometrium (7); alveolar epithelial type II cells of both rat (8) and human (9); and human breast cancer cells (10). Generally, vertebrate hemoglobin is known to function as a carrier protein of O2 and CO2 (9). However, recently hemoglobin has been reported to generate and transport NO or to scavenge NO and its metabolic derivatives (11,12). As well as, other potential functions, including anti-oxidant and superoxide anion and H2O2 scavenging properties have been reported (13,14).
Glioblastoma multiforme (GBM) is the most common and the most aggressive of astrocytic tumors, constituting 25% of all malignant nervous system tumors (15). Despite aggressive multimodality treatments, GBM is characterized by a very poor prognosis with median survival rate of about one year (16). The capability of GBM cells to infiltrate surrounding normal tissues (17), along with unidentified glial defence mechanisms due to expression of unknown protectant molecules, makes curative treatment by surgery, radiation and chemotherapies difficult, if not impossible.
We have previously reported that Ngb and Cygb are expressed in human GBM cell lines (18–20), as well as in human primary tumors including brain tumors (19). In this study, we examined whether hemoglobins (α, β, γ, δ, ζ and ε) are also expressed in human GBM cell lines.
Materials and methods
Cell lines and in vitro culture conditions
The characterization and origin of the GBM cell lines have been published previously: the M059J (ATCC no. CRL2366, Manassas, VA, USA) is radio-sensitive and hypoxia-sensitive; M059K (ATCC no. CRL-2365) is radio-resistant and hypoxia-tolerant and M006x cell lines are hypoxia-tolerant (21–24). The U87T (tumor) and U87R (invasive) cell lines are established GBM cell lines (25) and were kindly provided by Dr Donna Senger (University of Calgary, Calgary, AB, Canada). All cells were maintained as monolayer cultures in DMEM/F12 media supplemented with 10% fetal calf serum and 1 mM L-glutamine in a humidified atmosphere of 5% CO2 in air at 37°C. All tissue culture supplies were purchased from Gibco (Carlsbad, CA, USA).
RNA extraction and reverse transcription
RNeasy mini kit (Qiagen, Valencia, CA, USA) was used to isolate total RNA from GBM cultured cell lines. Reverse transcription (RT) was carried out with 0.1–1 μg total RNA per 20 μl reaction volume using QuantiTect reverse transcription kit (Qiagen).
Reverse transcription-PCR
Conventional RT-PCR was carried out with GeneAmp PCR system 9700 (Applied Biosystems, Foster City, CA, USA) using Platinum Pfx DNA polymerase (Invitrogen, Carlsbad, CA, USA) for 35 cycles. To detect α, β, γ, δ, ζ and ε globin genes, specific oligonucleotide primer pairs (Table I) were designed using primer 3 plus program (26). For β, γ and ε globin genes, two primer pairs were designed to ensure their presence. For reaction specificity, different annealing temperatures were applied (Table I) where the annealing temperature for each set of primers was determined empirically by repeating the RT-PCR reaction at many different temperatures. Amplified RT-PCR products were separated in 2% agarose gel electrophoresis and visualized by ethidium bromide.
DNA sequencing
Bands of RT-PCR amplicons were excised from the agarose gel and purified using QIAEX II Gel Extraction Kit (Qiagen). Cycle sequencing protocol was carried out using BigDye® Terminator v3.1 (Applied Biosystems), BigDye Terminator v1.1 and v3.1 5X sequencing buffer (Applied Biosystems) and one of the primer pairs used in RT-PCR. The sequence reaction was cycled for 25 cycles (96°C for 1 min, 96°C for 10 sec, 50°C for 5 sec, 60°C for 4 min, rapid thermal ramp to 4°C and hold) using thermal cycler. Sequencing reaction was precipitated (ethanol/EDTA), washed, dried out, resuspended in 10 μl de-ionized formamide (injection buffer) and sequenced using (ABI PRISM® 310 Genetic Analyzer, Applied Biosystems). Sequencing data were analysed by NCBI BLAST engine.
Western blot analysis
To detect globin proteins, M006x cells were washed four times with PBS. Whole-cell lysates were prepared using complete Lysis-M buffer (Roche Diagnostics, Indianapolis, IN, USA) and protein content determined using a protein assay kit (Pierce, Rockford, IL, USA). Equal amounts of protein (50 μg) were resolved using Tris-Tricine-PAGE or 13% SDS-PAGE under reducing condition and electro-transferred to polyvinylidene difluoride (PVDF) membranes (Bio-Rad Laboratories, Hercules, CA, USA). Membranes were blocked with 5% serum derived from the same animal species in which the secondary antibody is raised. Different primary antibodies were used in this study: 1:100 human anti-human hemoglobin monoclonal antibody (HCA042, AbD Serotec, Kidlington, UK); 1:100 goat anti-human hemoglobin (α chain) polyclonal antibody (SC-31110, Santa Cruz Biotechnology Inc, Santa Cruz, CA); 1:100 mouse anti-human hemoglobin monoclonal antibodies, γ chain (SC-21756) and β chain (SC-21757, Santa Cruz Biotechnology); and 1:500 mouse anti-human hemoglobin (ε chain) monoclonal antibodies (10C-CR8008M1, Fitzgerald Industries International Inc, Concord, MA). Membranes were incubated with primary antibodies diluted in 5% serum for 2 h. In consistent with the primary antibodies host species, different secondary antibodies conjugated with horseradish peroxidase were used: 1:1,000 goat anti-human IgG F(ab′)2-polyclonal antibody (0500-0099, AbD Serotec); 1:6,000 goat anti-mouse IgG and 1:4,000 rabbit anti-goat polyclonal antibodies (DakoCytomation Denmark A/S, Glostrup, Denmark). Membranes were incubated with secondary antibodies diluted in 5% serum for 1 h. Bound proteins were detected using chemiluminescence reagents (SuperSignal West Pico Chemiluminescent Substrate, Thermo Scientific, Rockford, IL) and visualized by exposing to X-ray film (Fuji Photo Film, Tokyo, Japan) that was developed using a Kodak X-OMAT 2000A processor (Eastman Kodak Company, Tokyo, Japan).
Mass spectrometry and protein sequencing
M006x cells were lysed in complete Lysis-M buffer (Roche Diagnostics) and the protein content was determined using a protein assay kit (Pierce). Cellular lysates were incubated with the appropriate antibodies; goat anti-human hemoglobin (α chain, SC-31110, and β/γ/δ/ε chain, SC-22718, Santa Cruz Biotechnology); polyclonal antibody, mouse anti-human (γ chain, SC-21756, and β chain, SC21757) hemoglobin monoclonal antibodies (Santa Cruz Biotechnology); and mouse anti-human hemoglobin [ε chain] monoclonal antibodies (10C-CR8008M1, Fitzgerald Industries International). Immunoprecipitation was carried out using an immunoprecipitation kit (Dynabeads Protein G, Invitrogen) according to manufacturer’s instructions. Eluted proteins were reduced, heated and subjected to SDS-PAGE. The gel was stained (Bio-Safe Coomassie Stain, Bio-Rad) and the excised bands were analyzed by mass spectrometry at Institute of Biomolecular Design (IBD), University of Alberta (Edmonton, AB, Canada). In-gel tryptic digestion, peptide extraction and mass spectrometric analysis were done as described by Lopez-Campistrous et al (27) except that the ion trap mass spectrometry (LCQ™ Deca XP ion trap mass spectrometer, Thermo Finnigan, San Jose, CA, USA) was used.
Immunofluorescence cell staining
Cultured cells were grown overnight on sterile coverslips. Cells were washed four times with PBS, fixed in cold methanol for 5 min and air dried for 15 min. The cells were washed with three changes of PBS, incubated with 10% normal serum (serum derived from the same animal species in which the secondary antibody is raised) for 30 min and then washed with PBS. Different primary antibodies were used; goat anti-human hemoglobin (1:75) polyclonal antibody (α chain, SC-31110, Santa Cruz Biotechnology); mouse anti-human (β chain, SC21757) and (γ chain, SC-21756) hemoglobin (1:75) monoclonal antibodies (Santa Cruz Biotechnology) and mouse anti-human hemoglobin (1:250) monoclonal antibodies (ε chain, 10C-CR8008M1, Fitzgerald Industries International). Cells were incubated with primary antibody diluted in 1% serum for 1 h. Different secondary antibodies were used [1:250 goat anti-mouse IgG polyclonal antibody Cy3 conjugated (610-704-124, Rockland Immunochemicals for Research, Gilbertsville, PA, USA); 1:250 donkey anti-goat IgG polyclonal antibody Alexa Flour 488 conjugated (A11055, Molecular Probes Inc., Eugene, OR, USA)]. Cells were washed three times with PBS and then incubated for 45 min with secondary antibody diluted in 1% serum. Cells were washed three with PBS (5 min each) and then the coverslips were mounted on slides with mounting media containing DAPI (ProLong Gold antifade reagent with DAPI, P36935, Invitrogen).
Results
Expression of α, β, γ, δ, ζ and ε globin m RNA in GBM cells in vitro
Amplified RT-PCR products separated on agarose gel revealed clear bands that coincide with their predicted sizes using different primer pairs (Fig. 1). Analysis of the DNA sequences extracted from the agarose bands using the NBCI BLAST engine revealed perfect alignments to their correspondents α, β, γ, δ, ζ and ε globins mRNA in GenBank (Table II).
Expression of α, β, γ, δ, ζ and ε globin proteins in GBM cells in vitro
Western blot analyses of cell-lysate of M006x cells showed the presence of α, β, γ, δ, ζ and ε globin protein (Fig. 2). As shown by others (9,28) and as indicated in the manufacturer’s data sheet (AbD Serotec), adult hemoglobin and globins specific antibodies detected protein bands of 14, 26, 43 kDa and higher in cell lysate and hemoglobin standard protein despite reduction and heat denaturing of the samples. The heterotetramer and globin dimer were more easily detected than monomer globins that require long exposure time accompanied by high background. Mass spectrometry analysis of different globin immunoprecipitates showed peptide match to α, β, δ, and ε globin protein (Table III). The unsuccessful detection of γ and ζ globin protein by mass spectrometry could be due to multiple factors including unsuitability of their relevant antibodies for the application of immunoprecipitation.
Immunofluorescence analysis
To confirm the expression of globin proteins, immunofluorescence experiments were carried out. Anti-human α, β, γ and ε antibody incubated with fixed M006x cells that grown under aerobic conditions (Fig. 3) displayed both cytoplasmic and nuclear staining. This is consistent with the staining pattern of α, β globin previously observed in rat neurons (6,28), murine and human A9 dopaminergic neurons, a subpopulation of cortical and hippocampal astrocytes, and in mature oligodentrocytes (29). Expression of α, β and ε globin was higher in the cytoplasm whereas γ globin was predominant in the nucleus.
Discussion
We have previously reported that two newly discovered globins, neuroglobin and cytoglobin, are expressed in human primary GBM tumors and cell lines (18,19). Here, using conventional RT-PCR and DNA sequencing, western blot analysis, immunofluorescence staining and mass spectrometry, we confirmed the presence of different hemoglobins (α, β, γ, δ, ζ and ε) in GBM cells under normal physiological conditions. Others have reported α and β globin expression in rodent neurons, but not in astrocytes and oligodendrocytes (6,28), whereas Biagioli et al (29) reported their presence in A9 dopaminergic neurons, a subpopulation of cortical and hippocampal astrocytes and in mature oligodentrocytes. However, the heterogeneity of gliomas (30) and ability of gliobalstoma cell lines to co-express glial and neuronal markers (31) may partially explain the presence of neuroprotective globin molecules such as neuroglobin in GBM cells (18), as well as hemoglobin.
The most important functions of erythroid hemoglobin are the transport of O2 and CO2 (9), to bind CO, and to scavenge and release NO (32). Anti-oxidative function of hemoglobin has been manifested by reducing production of hydrogen peroxide-induced intracellular radical oxygen species and enhancing cell viability after overexpression of the detected hemoglobin in rat mesangial cells (14). Moreover, human hemoglobin can detoxify highly oxidizing radicals yielding the respective non-toxic ferric states (33). Interestingly, hemoglobin was detected in breast cancer tissues and MCF7 cell line but not in normal breast tissue (10) suggesting a functional role for hemoglobin in carcinogenesis.
The expression of different types of hemoglobins (α, β, γ, δ, ζ and ε) representing fetal, embryonic and adult hemoglobin in GBM cells may imply an undefined potential role for these hemoglobins at different stages of cellular growth and adaptation, assisting those cells to resist aggressive multimodality treatments and consequently enabling cell survival. In addition, expression of the hemoglobins in all tested cell lines; M006x (hypoxia-tolerant) M059J (radio-sensitive and hypoxia-sensitive), M059K (radio-resistant and hypoxia-tolerant) (21–24) U87T (tumor) and U87R (invasive) cell lines (25) may indicate that hemoglobin expression is not limited to GBM cells with certain cell characteristics but it is a common property of all tested cell lines.
Although α and β globin expression has been reported in many non-erythroid cells, to our knowledge, we are the first to report the expression of α, β, γ, δ, ζ and ε globins in human GBM cell lines under normal physiological conditions. Our results, together with the known non-oxygen transport related functions of hemoglobin suggest that hemoglobin expression in GBM cells may be a part of series of active defence and adaptation mechanisms by which these cells resist even aggressive multimodality treatments. Further experiments are required to investigate whether hemoglobin is upregulated under hypoxic conditions simulating hypoxic tumor microenvironment, and whether those hemoglobins are differentially regulated.
Acknowledgements
We thank Dr Richard Fahlman and Jack Moore for help with mass spectrometry, Dr Xuejun Sun for help with immunofluorescence imaging, and Bonnie Andrais for assistance with tissue culture. This study was supported by an award from the Canadian Cancer Society Research Institute with funds provided by the Canadian Cancer Society.
References
|
Hardison RC: A brief history of hemoglobins: plant, animal, protist, and bacteria. Proc Natl Acad Sci USA. 93:5675–5679. 1996. View Article : Google Scholar : PubMed/NCBI | |
|
Roesner A, Fuchs C, Hankeln T and Burmester T: A globin gene of ancient evolutionary origin in lower vertebrates: evidence for two distinct globin families in animals. Mol Biol Evol. 22:12–20. 2005. View Article : Google Scholar : PubMed/NCBI | |
|
Bunn HF and Forget BG: Hemoglobin: Molecular, Genetic, and Clinical Aspects. WB Saunders Co; Philadelphia, PA: 1986 | |
|
Hardison RC: Globin genes on the move. J Biol. 7:352008. View Article : Google Scholar : PubMed/NCBI | |
|
Pesce A, Bolognesi M, Bocedi A, et al: Neuroglobin and cytoglobin. Fresh blood for the vertebrate globin family EMBO Rep. 3:1146–1151. 2002. | |
|
Schelshorn DW, Schneider A, Kuschinsky W, et al: Expression of hemoglobin in rodent neurons. J Cereb Blood Flow Metab. 29:585–595. 2009. View Article : Google Scholar : PubMed/NCBI | |
|
Dassen H, Kamps R, Punyadeera C, et al: Haemoglobin expression in human endometrium. Hum Reprod. 23:635–641. 2008. View Article : Google Scholar | |
|
Bhaskaran M, Chen H, Chen Z and Liu L: Hemoglobin is expressed in alveolar epithelial type II cells. Biochem Biophys Res Commun. 333:1348–1352. 2005. View Article : Google Scholar : PubMed/NCBI | |
|
Newton DA, Rao KM, Dluhy RA and Baatz JE: Hemoglobin is expressed by alveolar epithelial cells. J Biol Chem. 281:5668–5676. 2006. View Article : Google Scholar : PubMed/NCBI | |
|
Gorr TA, Wichmann D, Pilarsky C, et al: Old proteins - new locations: myoglobin, haemoglobin, neuroglobin and cytoglobin in solid tumours and cancer cells. Acta Physiol (Oxf). 202:563–581. 2011. View Article : Google Scholar : PubMed/NCBI | |
|
Cosby K, Partovi KS, Crawford JH, et al: Nitrite reduction to nitric oxide by deoxyhemoglobin vasodilates the human circulation. Nat Med. 9:1498–1505. 2003. View Article : Google Scholar : PubMed/NCBI | |
|
Huang Z, Shiva S, Kim-Shapiro DB, et al: Enzymatic function of hemoglobin as a nitrite reductase that produces NO under allosteric control. J Clin Invest. 115:2099–2107. 2005. View Article : Google Scholar : PubMed/NCBI | |
|
Masuoka N, Kodama H, Abe T, Wang DH and Nakano T: Characterization of hydrogen peroxide removal reaction by hemoglobin in the presence of reduced pyridine nucleotides. Biochim Biophys Acta. 1637:46–54. 2003. View Article : Google Scholar : PubMed/NCBI | |
|
Nishi H, Inagi R, Kato H, et al: Hemoglobin is expressed by mesangial cells and reduces oxidant stress. J Am Soc Nephrol. 19:1500–1508. 2008. View Article : Google Scholar : PubMed/NCBI | |
|
Brandes AA, Tosoni A, Franceschi E, Reni M, Gatta G and Vecht C: Glioblastoma in adults. Crit Rev Oncol Hematol. 67:139–152. 2008. View Article : Google Scholar | |
|
Lim SK, Llaguno SR, McKay RM and Parada LF: Glioblastoma multiforme: a perspective on recent findings in human cancer and mouse models. BMB Rep. 44:158–164. 2011. View Article : Google Scholar : PubMed/NCBI | |
|
Alves TR, Lima FR, Kahn SA, et al: Glioblastoma cells: A heterogeneous and fatal tumor interacting with the parenchyma. Life Sci. 89:532–539. 2011. View Article : Google Scholar : PubMed/NCBI | |
|
Emara M, Salloum N and Allalunis-Turner J: Expression and hypoxic up-regulation of neuroglobin in human glioblastoma cells. Mol Oncol. 3:45–53. 2009. View Article : Google Scholar : PubMed/NCBI | |
|
Emara M, Turner AR and Allalunis-Turner J: Hypoxic regulation of cytoglobin and neuroglobin expression in human normal and tumor tissues. Cancer Cell Int. 10:332010. View Article : Google Scholar : PubMed/NCBI | |
|
Fang J, Ma I and Allalunis-Turner J: Knockdown of cytoglobin expression sensitizes human glioma cells to radiation and oxidative stress. Radiat Res. 176:198–207. 2011. View Article : Google Scholar | |
|
Allalunis-Turner MJ, Barron GM, Day RS III, Dobler KD and Mirzayans R: Isolation of two cell lines from a human malignant glioma specimen differing in sensitivity to radiation and chemotherapeutic drugs. Radiat Res. 134:349–354. 1993. View Article : Google Scholar : PubMed/NCBI | |
|
Allalunis-Turner MJ, Barron GM, Day RS III, Fulton DS and Urtasun RC: Radiosensitivity testing of human primary brain tumor specimens. Int J Radiat Oncol Biol Phys. 23:339–343. 1992. View Article : Google Scholar : PubMed/NCBI | |
|
Allalunis-Turner MJ, Franko AJ and Parliament MB: Modulation of oxygen consumption rate and vascular endothelial growth factor mRNA expression in human malignant glioma cells by hypoxia. Br J Cancer. 80:104–109. 1999. View Article : Google Scholar : PubMed/NCBI | |
|
Parliament MB, Allalunis-Turner MJ, Franko AJ, et al: Vascular endothelial growth factor expression is independent of hypoxia in human malignant glioma spheroids and tumours. Br J Cancer. 82:635–641. 2000.PubMed/NCBI | |
|
Johnston AL, Lun X, Rahn JJ, et al: The p75 neurotrophin receptor is a central regulator of glioma invasion. PLoS Biol. 5:e2122007. View Article : Google Scholar : PubMed/NCBI | |
|
Untergasser A, Nijveen H, Rao X, Bisseling T, Geurts R and Leunissen JA: Primer3Plus, an enhanced web interface to Primer3. Nucleic Acids Res. 35:W71–W74. 2007. View Article : Google Scholar : PubMed/NCBI | |
|
Lopez-Campistrous A, Semchuk P, Burke L, et al: Localization, annotation, and comparison of the Escherichia coli K-12 proteome under two states of growth. Mol Cell Proteomics. 4:1205–1209. 2005. | |
|
He Y, Hua Y, Liu W, Hu H, Keep RF and Xi G: Effects of cerebral ischemia on neuronal hemoglobin. J Cereb Blood Flow Metab. 29:596–605. 2009. View Article : Google Scholar : PubMed/NCBI | |
|
Biagioli M, Pinto M, Cesselli D, et al: Unexpected expression of alpha- and beta-globin in mesencephalic dopaminergic neurons and glial cells. Proc Natl Acad Sci USA. 106:15454–15459. 2009. View Article : Google Scholar : PubMed/NCBI | |
|
Valtz NL, Hayes TE, Norregaard T, Liu SM and McKay RD: An embryonic origin for medulloblastoma. New Biol. 3:364–371. 1991.PubMed/NCBI | |
|
Rebetz J, Tian D, Persson A, et al: Glial progenitor-like phenotype in low-grade glioma and enhanced CD133-expression and neuronal lineage differentiation potential in high-grade glioma. PLoS One. 3:e19362008. View Article : Google Scholar : PubMed/NCBI | |
|
Schechter AN: Hemoglobin research and the origins of molecular medicine. Blood. 112:3927–3938. 2008. View Article : Google Scholar : PubMed/NCBI | |
|
Goldstein S and Samuni A: Intra- and intermolecular oxidation of oxymyoglobin and oxyhemoglobin induced by hydroxyl and carbonate radicals. Free Radic Biol Med. 39:511–519. 2005. View Article : Google Scholar : PubMed/NCBI |
