GSE4, a Small Dyskerin- and GSE24.2-Related Peptide, Induces Telomerase Activity, Cell Proliferation and Reduces DNA Damage, Oxidative Stress and Cell Senescence in Dyskerin Mutant Cells

Dyskeratosis congenita is an inherited disease caused by mutations in genes coding for telomeric components. It was previously reported that expression of a dyskerin-derived peptide, GSE24.2, increases telomerase activity, regulates gene expression and decreases DNA damage and oxidative stress in dyskeratosis congenita patient cells. The biological activity of short peptides derived from GSE24.2 was tested and one of them, GSE4, that probed to be active, was further characterized in this article. Expression of this eleven amino acids long peptide increased telomerase activity and reduced DNA damage, oxidative stress and cell senescence in dyskerin-mutated cells. GSE4 expression also activated c-myc and TERT promoters and increase of c-myc, TERT and TERC expression. The level of biological activity of GSE4 was similar to that obtained by GSE24.2 expression. Incorporation of a dyskerin nuclear localization signal to GSE24.2 did not change its activity on promoter regulation and DNA damage protection. However, incorporation of a signal that increases the rate of nucleolar localization impaired GSE24.2 activity. Incorporation of the dyskerin nuclear localization signal to GSE4 did not alter its biological activity. Mutation of the Aspartic Acid residue that is conserved in the pseudouridine synthase domain present in GSE4 did not impair its activity, except for the repression of c-myc promoter activity and the decrease of c-myc, TERT and TERC gene expression in dyskerin-mutated cells. These results indicated that GSE4 could be of great therapeutic interest for treatment of dyskeratosis congenita patients.


Introduction
Telomere maintenance alterations are in the origin of an increasing number of diseases such as dyskeratosis congenita, aplastic anemia or pulmonary fibrosis (recently reviewed by S.A. Savage [1]). Telomeres are structures located at the end of the chromosomes that play essential roles in chromosome replication and stability [2,3]. The sequence of their DNA consists of hundreds of repeats of the TTAGGG motif. The DNA replication machinery cannot complete the synthesis of the chromosome ends that is accomplished by a RNA-protein complex with reverse transcriptase activity named telomerase [4]. The telomerase protein with reverse transcriptase activity is encoded by the TERT gene and uses as template the RNA molecule encoded by the TERC (also named TR) gene that is another component of the telomerase complex [5]. A third essential component is dyskerin, encoded by the dkc1 gene [6,7]. Additional components of the telomerase complex include the proteins NOP10, GAR and NHP2 [8]. Telomeres acquire a very specialized structure since the terminal region of the DNA stays single-stranded and folds back to get inter winged with a close telomere region to form a circular structure (Tcircle) [9]. In addition, the telomere DNA binds to a specific protein complex, named shelterin complex, which protects telomeres from degradation [10]. This structure also avoids the recognition of telomeres as damaged DNA by the DNA-repair signalling system. The correct structure of the telomeres is therefore essential for the maintenance of chromosome integrity and cell cycle progression [11]. Telomere shortening that occurs during proliferation of non-stem or transformed cells results in genome instability, the fusion of chromosomes and induces apoptotic cell death or senescence [11].
Mutations in the genes coding for components of the telomerase (TERT, TERC, DKC, NOP10, NH2) or shelterin (TINF2) complexes cause a number of diseases known as telomeropathies or Telomere Biology Disorders. Among them are dyskeratosis congenita, premature aging syndromes, aplastic anemia, pulmonary fibrosis and cancer (see Savage, S.A. [1] and Glousker, G. et al [12] for recent reviews).
Dyskeratosis congenita is a rare disorder characterized by bone marrow failure and increased susceptibility to cancer [13]. Mutations in DKC1 produce the predominant X-linked form of this disease. The encoded protein, dyskerin, is a pseudouridine synthase required for the postranscriptional modification of ribosomal, small nuclear and nucleolar RNAs and some mRNAs [7,14] [15,16]. In addition, is an essential component of the telomerase complex as previously indicated. Dyskerin has three conserved domains, the Dyskerin Like Domain (DKLD), the pseudouridine synthase domain (TRUB domain) and the RNA binding domain (PUA domain) [7]. Mutations in these domains produce X-linked dyskeratosis congenita [7,17]. We have previously described that a 55 amino acids-long fragment of the dyskerin TRUB domain, named GSE24.2, has protective effects on cells derived from dyskeratosis congenita patients [18]. GSE24.2 treatment increases telomerase activity of patient cells. This peptide also protects cells from treatment with the anticancer drug cisplatin, that induces intra-and interstrand DNA bridges, and from telomerase inhibitors. Expression of GSE24.2 from plasmid or viral vectors or direct transfection of cells with the peptide, produced in bacteria or chemically synthesized, have similar effects [19]. GSE24.2 increases TERT and c-myc expression through transcriptional activation and stabilizes TERC RNA in dyskerin mutant cells [19]. This peptide protects cells from basal DNA damage, which is increased in dyskeratosis congenita patients [20]. These activities make of GSE24-2 a good candidate for a therapeutic approach to dyskeratosis congenita and related telomeropathies. Actually, the EMA recently approved GSE24.2 as an orphan drug for dyskeratosis congenita treatment (EU/3/12/1070-EMA/OD/136/11).
In this article we describe that a smaller peptide of just eleven amino acids, named GSE4, corresponding to the N-terminal region of GSE24.2, maintains the same capacity to regulate gene expression, to protect cells from DNA damage and to decrease oxidative stress as GSE24.2. In addition, GSE24.2 and GSE4 protect dyskeratosis congenita patient's cell from cell senescence.

Materials and Methods
Cell culture and transfection The previously described F9 and dyskerin-mutated F9 cells (F9-A353V) [19,21], were cultured in Dulbecco Modified Eagle Medium (DMEM) supplemented with 10% foetal bovine serum, 2 mM glutamine (Gibco) and 1.5 gr/ml of sodium bicarbonate. HEK293T cells (ATCC) were cultured in DMEM media supplemented with 10% foetal bovine serum and 2 mM glutamine. DC-C and DC-3 cells (Coriell Cell Repository) were cultured in Roswell Park Memorial Institute (RPMI) media supplemented with 20% foetal bovine serum and 2 mM glutamine. XDC-1787-C (Corriel Cell Repository) and F26IIB cells (generated in our laboratory), were cultured in Minimum Essential Medium Eagle (MEM) media supplemented with 15% foetal bovine serum and 2 mM glutamine. Cells were transfected with 10 μg of DNA/10 6 cells using lipofectamine plus (Invitrogene, Carlsbad, USA) or the K2 transfection kit (Biontex Lab, Planegg/ Martinsried, GE) according to the manufacturers' instructions. 15 μg of peptides per 35 mm dish were transfected using the ProteoJuice Protein Transfection Reagent (Merck Millipore, Billerica, MA, USA) or the K2 transfection kit.

Vector constructions and in vitro mutagenesis
The localization signal KRKR (amino acids 446-449) was incorporated to the 3' end of the GSE 24.2 expression vector by PCR using the oligonucleotides 5'-GGGAATTCTGGTTTGAT TAATCTTGACAAGC-3' and 5'-GGTCTAGACTCGCTTCCGCTTCTTCACCAAGCGAG TGGCTCG-3'. The amplified product was cloned between the EcoRI and XbaI sites of the pcDNA3-myc vector to generate the GSE24.

Gene-reporter assays
Cells were transfected with 10 μg/10 6 cells of expression vectors for GSE24.2, GSE4 and derived peptides and the corresponding luciferase reporter vectors (1 μg/10 6 cells). The TERT and cmyc (px3.2) promoter constructs have been described previously [18,22]. Twenty four hours after transfection protein extracts were prepared and luciferase activity determined using a commercial kit (Promega Corporation, Madison, WI, USA). Luciferase activity was expressed as arbitrary units by μg of protein concentration, determined with the Bradford Reagent (BioRad, Berkeley, CA, USA).

Immunofluorescence and immunocytochemistry
Cells were grown on coverslips, fixed, permeabilized and incubated with the corresponding antibodies as previously described [20]. Nucleoli were stained incubating the cells for 20 min with 0,5 μM of the SYTO RNA Select Green Fluorescent Cell Stain (Molecular Probes). DNA damage foci were identified by the presence of γH2AX as previously described [20]. Oxidative stress was determined using the anti-8-oxoguanine antibody, clone 483.15 (MAB3560, Merck-Millipore). Images were acquired using a Zeiss Confocal microscope and processed using ZEN 2011 Light Edition and ImageJ software. DNA synthesis was determined by immunocytochemistry using anti-Ki67 antibodies (RM9106-50; NeoMarkers Inc. Fremont, CA, USA).

Telomeric Repeat Amplification Protocol (TRAP) assay
The TRAPeze kit (Millipore, Billerica, MA, USA) [23] was used to determine telomerase activity. The activity of each sample was normalized using the internal control provided in the kit.

Determination of reactive oxygen species (ROS) content with dihydroethidium
Cells were washed 2 times with pre-warmed PBS medium, dihydroethidium (Dihydroethidium, D7008-Sigma, St. Louis, MI. USA) was added and the cells incubated at 37°C for 25 min. The fluorescence was measured using FACS SCAN II (BD, USA), with 530 nm of excitation wavelength and 630 nm of emission wavelength.

Determination of cell senescence
Cells were plated on 6-well plates at a density of 1x10 4 cells/well. After 4 days of culture cells were fixed and the acid-β-galactosidase activity detected using the Senescence Detection Kit (BioVision, USA). Six images were taken from each well using a Nikon Eclipse TS100 microscope (Nikon, USA) and the percentage of senescent cells calculated for each of them.

Quantitative RT-PCR analyses of gene expression
Total RNA was obtained from the cell cultures using the Trizol Reagent (Invitrogen, Carlsbad, CA, USA). One microgram of RNA was converted to cDNA using random primers and the High-Capacity cDNA Archive Kit (Applied Biosystems, Foster City, CA, USA). Quantitative PCR was done using the Power SYBR Green kit (Applied Biosystems, Foster City, CA, USA). The programs used have been described by Machado-Pinilla, et al. [19]. SOD1(Cu/Zn SOD) and SOD2 (Mn SOD) mRNA levels were determined using the TaqMan Universal PCR Master Mix. The StepOne Plus Real Time PCR System (Applied Biosystems, Foster City, CA, USA) was used for analyses of the PCR products. Relative gene expression was calculated according to the comparative threshold cycle method [25] using β-actin as endogenous control.

Primers used for quantitative RT-PCR
The following primers were used: m-cmyc-S:

Statistical analyses
Experiments were repeated, at least, three times with triplicate samples. Statistical significance was calculated using the Unpaired t-test (two-tailed). The significance has been considered at Ã p<0.05, ÃÃ p<0.01 and ÃÃÃ p<0.001. GraphPad software v5.0 was used for statistical analysis and graphic representations.

1.
Functional study of the GSE24.2-derived peptide GSE4 on DNA damage rescue, telomerase activity and cell proliferation in dyskeratosis congenita cells Many of the previous functional studies were done with GSE24.2 peptides produced in E. coli. The analysis of these preparations by mass spectroscopy indicated the presence of several smaller peptides probably originated by GSE24.2 partial degradation. The more abundant peptide was an eleven amino acids long peptide corresponding to the N-terminal region of GSE24.2 (GSE4, Fig 1A). The functional activity of this peptide was compared to that of GSE24.2 in several analyses. We have previously reported that the GSE24.2 peptide reduced DNA damage [20]. We transfected F9 or the F9-derived dyskerin-mutant F9A353V cells with pRRL-CMV-IRES-GFP vector, either empty (vector) or expressing GSE24.2 or GSE4 to study their possible effect on basal DNA damage by measuring γH2AX phosphorylation ( Fig  1A). We found that the amount of γH2AX in F9A353V cells decreased to similar levels after transfecting both peptides (40 and 30%, respectively). The possible effect of GSE4 expression on telomerase activity was assayed on the fibroblastoid cell line F26IIB, derived from a dyskeratosis congenita patient carrying the Ala2Val hemizygous mutation [26]. Cells were transfected with the above-mentioned vectors and their telomerase activity determined, as shown in Fig 1B. Quantification of the extension products indicated a significant increase in telomerase activity upon GSE24.2 and GSE4 expression. The proliferation capacity of the transfected cells was estimated by the expression of the Ki67 nucleolar protein, as shown in

Oxidative stress and senescence are decreased in X-DC cells by GSE4 expression
Oxidative stress is one of the causes of DNA damage producing both single-strand breaks (SSBs) and double-strand breaks (DSBs). Cells obtained from dyskeratosis congenita patients showed high levels of oxidative stress and reactive oxygen species (ROS) production that decreased upon treatment with GSE24.2 [20]. We therefore tested the activity of GSE4 on oxidative stress on a cellular model of dyskeratosis congenita. Oxidative stress was first determined by the presence of α-8-oxoguanine on the cellular DNA. F9-A353V cells were transfected with the pRRL-CMV-IRES-GFP vector expressing GSE24.2, GSE4 or the empty vector and the amount of α-8-oxoguanine present on the cells determined by immunohistochemistry. F9 cells that do not carry any DKC mutation were used as control. The quantification of α-8-oxoguanine expression is shown in Fig 2A. Expression of GSE24.2 and GSE4 decreased α-8-oxoguanine levels of F9-A353V cells. Oxidative stress was also measured in cells derived from dyskeratosis congenita patients (DC-3, carrying the Thr66Ala mutation in dkc1) and healthy relatives (DC-C) by determining ROS levels using dihydroethidium, as shown in Fig 2B. Dyskeratosis-congenita patient cells infected with the empty vector showed higher levels of ROS than those of the healthy controls. Expression of GSE24.2 and GSE4 in the patient cells significantly decreased ROS levels. ROS production is associated with decreased expression of antioxidant enzymes such as the Cu/Zn-and Mn-dependent Superoxide Dismutases (SOD) [20]. The expression levels of the mRNAs coding for these two enzymes was determined by RT-qPCR, as shown in Fig 2C. Patient cells expressing the empty vector (DC-3 vector) showed decreased levels of both mRNAs, as compared to cells from the healthy control (Control cells). Expression of GSE24-2 and GSE4 greatly increased Cu/Zn SOD and Mn SOD mRNA expression levels in agreement with their capacity to decrease ROS production.
Telomere shortening has been described to result in cell senescence [27]. Therefore, the possible effect of GSE24.2 and GSE4 expression in senescence of dyskeratosis congenita patient's cells has been studied. One fibroblastoid cell line established from a dyskeratosis congenita patient (F26IIB) was transfected with the pRRL-CMV-IRES-GFP vector, either empty or expressing GSE24.2 or GSE4. After four days of culture senescent cells were identified by the expression of acidic β-galactosidase and the percentage of senescent (SA-β-gal) cells determined, as shown in Fig 2D. A fibroblastoid cell line established from a healthy relative of a DC patient (XDC-1787-C) was used as internal control. Expression of GSE4 and GSE24.2 significantly decreased cell senescence.

and GSE4 biological activity
Dyskerin is a nucleolar protein and different cellular localization regions have been described [28]. Two of them were analyzed because their deletion or mutation altered the subcellular localization of dyskerin [28]. The first one (KRKR, named NLS1 in this article) is required for nuclear import while the second one (KKEKKKSKK, NLS2) increases the rate of nuclear and nucleolar import. Since GSE24.2 does not contain any of these regions, both were independently incorporated to the C-terminal region of the peptide to determine their possible contribution to the cellular localization and activity of the peptide. We used plasmid expression vectors with an N-terminal 6xmyc epitope (pcDNA3-myc). Cellular localization was studied by immunohystochemistry using α-myc antibodies after their expression in HeLa cells ( Fig  3A). In some of these experiments nucleoli were identified using the specific SYTO RNA Select probe (Fig 3A, lower panels). The results showed that NLS1 incorporation increased the nuclear localization of GSE24.2, with low expression in nucleoli. In contrast, NLS2 incorporation resulted in an even expression in all nuclear regions. NLS1 and NLS2 incorporation to the N terminal region of GSE24.2 did not change the cellular localization (S1 Fig). The functionality of the fusion peptides was determined by expressing them from the pcDNA3-myc vector in F9-A353V, F9 and HEK293T cells. We have previously described that expression of GSE24.2 activated TERT and c-myc promoters [18] [29]. Therefore, we studied the activity of the different constructions on the human c-myc and TERT promoters (Fig 3B). Both GSE24.2 and GSE24.2-NLS1.3 activated c-myc and TERT promoters in the three cell lines analyzed to similar levels although some of the activity increases were not statistically significant in F9 cells. However, GSE24.2-NLS2.3 only activated the TERT promoter. The effects of GSE24.2-NLS2.3 on the c-myc promoter were variable, a significant increase was observed in HEK293T cells and a significant decrease in F9 cells. None of the localization signals improved the transcriptional activity of GSE24.2. The possible activity on DNA damage was also studied using F9-A353V cells. The amount of DNA damage was estimated by evaluating the expression levels of phosphorylated γH2AX and Chk2Thr68 proteins. Quantification of DNA damage was made by Western blot using anti γH2AX and p-Chk2Thr68 antibodies ( Fig  3C). In addition, the localization of DNA damage foci was observed by immunohistochemistry, evaluating the amount of γH2AX-associated foci/cell (Fig 3D). GSE24.2 expression rescued the cells from DNA damage decreasing 40 and 30% respectively of γH2AX and p-Chk2 levels ( Fig  3C), as previously described [20]. NLS1.3 incorporation did not alter GSE24.2 activity while addition of NLS2.3 partially impaired this activity (Fig 3C and 3D).
The nuclear localization signal NLS1 was also added to the C-terminus of GSE4 to determine their possible influence on the activity of the peptide. GSE4 is similar to the conserved  pseudouridine synthase active centre of other enzymes, where the Aspartic acid homologous to the one present at position 6 in GSE4 is always conserved [30]. Therefore, this Aspartic acid was changed to Alanine to test its possible functional relevance. These different peptides were either chemically synthesized or expressed in the cells from plasmid or lentiviral vectors, as indicated in each specific experiment.
The cellular localization of the GSE4 and GSE4-NLS1 peptides was studied by transfecting fluorescein-labelled peptides into HeLa cells. Both peptides showed a predominant cytoplasmic localization, as shown in Fig 4A, although the incorporation of NLS1 increased the presence of the peptide in the perinuclear region. The biological activity of the peptides was determined by expressing them from the lentiviral vector pRRL-CMV-IRES-GFP in different cell lines. Transcriptional activity was determined by using the previously mentioned reporter vectors containing the human c-myc and TERT promoters. The results obtained in F9-A353V, F9 and HEK293T cells are shown in Fig 4B. GSE24.2 activity was also determined to further compare the activity of the diverse peptides. GSE4 and GSE4-NLS1 peptides showed similar capacity than GSE24.2 to activate c-myc and TERT promoters in the cell lines analyzed, including the F9-A353V mutant cells. In HEK293T cells GSE4 and GSE4-NLS1 peptides were more active than GSE24.2 but that was not the case in F9 and F9-A353V cells. The mutated GSE4-NLS1-DA peptide was also active in these assays, with the exception of the c-myc promoter in F9-A353V cells where the activity was actually decreased, indicating that this Aspartic acid residue is not required for GSE4 activity. The activity of GSE4-NLS1-DA was, however, lower than that of GSE24.2, GSE4 and GSE4-NLS1 in F9-A353V cells. The addition of the nuclear localization signal NLS1 to GSE4 resulted in increased TERT promoter activity in the three cell lines analyzed (Fig 4B).
The expression of c-myc and TERT mRNAs, and TERC (TR) RNA, in transfected F9-A353V cells was determined by Reverse Transcription and quantitative PCR (Fig 4C). The results obtained are in general agreement with the reporter expression analyses (Fig 4B). GSE24.2, GSE4 and GSE4-NLS1 induced c-myc, TERT and TERC (TR) expression while GSE4-NLS1-DA repressed the expression of these RNAs in F9-A353V cells. GSE4 was more efficient in inducing TERT and less efficient in inducing TERC (TR) than GSE24.2 and GSE4-NLS1 in these experiments.
The possible effect of the expression of GSE4 and derived peptides on DNA damage was also studied. F9-A353V cells were transfected with the expression vectors mentioned above. The amount of DNA damage in transfected cells was determined by quantification of γH2AXassociated foci/cell (Fig 5A and 5B). In addition, Western blot analyses allowed the quantification of γH2AX and p-Chk2Thr68 expression (Fig 5C). GSE4 and GSE4-NLS1 showed a protective effect on DNA damage similar to that of GSE24.2 in both assays. The mutant GSE4-NLS1-DA did not protect F9 A353V cells from DNA damage to the same extend under these experimental conditions. Altogether our results indicated that the functional activity of effect of pcDNA3_GSE24.2, GSE24.2_NLS13 and GSE24.2_NLS23 on the activity of c-myc and TERT promoters in F9_A353V, F9 and 293T cells. These three cell lines were cotransfected with pcDNA3 empty vector (Vector), GSE24.2 and GSE24.2-derived constructions (10 μg DNA/10 6 cells) and c-myc-lucor hTERT-luc -reporter vectors (1 μg/10 6 cells). Luciferase activity was measured following 24 hours of transfection. Data were normalized by protein concentration and referred to the empty vector. Data points represent the mean and standard deviations of 3 experiments performed in triplicate (statistical significance: * p<0.05, **p<0.01, ***p<0.001). Panels C, D, analyses of cellular DNA damage. (C) F9_A353V cells were transfected with the pRRL-CMV-IRES-EGFP empty vector (Vector), or expressing GSE24.2, GSE24.2-NLS13 and GSE24.2-NLS23 (10 μg DNA/10 6 cells). After 24 hours of transfection cells were lysed and the amount of γH2AX, α-tubulin (loading control), phosphorylated Chk2 (p-Chk2) and total Chk2 (Chk2) analyzed by western blot. The relative amounts of γH2AX/α-tubulin and p-Chk2/Chk2, normalized to the relation obtained for cells transfected with the empty vector, are indicated under each blot. (D) Upper panel. F9_A353V cells were transfected with the vectors indicated above and the presence of γH2AX analyzed by Immunofluorescence (red). Nuclear DNA was counterstained with DAPI (blue). Lower panel. Percentage of nuclei containing 0-9, 10-29 or more than 30 foci of γH2AX. More than 200 cells were analyzed for each transfection. Experiments were repeated 3 times with similar results. Asterisks indicate the statistical significance in relation to cells transfected with the empty vector (vector).  GSE4 peptide was similar to that GSE24.2 in all the biological assays performed in dyskeratosis congenita cells. Besides the addition of nuclear locations signals did not significantly increase the transcriptional activity of these peptides or their protection to DNA damage. In addition, the GSE4 Aspartic acid residue conserved in the pseudouridine synthase active centre of other enzymes, although not essential, is required for maximal activity of the peptide on dyskerinmutant cells.

Discussion
Telomere biology disorders, including dyskeratosis congenita, are characterized by the progressive shortening of the telomeres and by a number of cellular responses. In particular, telomere shortening and/or low telomerase activity induces in the cells a DNA damage response [31], and oxidative stress [32]. Therefore, the p53-dependent DNA damage response pathway is activated resulting in cell cycle arrest and cellular senescence [33,34]. These responses have an important contribution to the pathology of the diseases through the deprivation of stem cells in the more proliferative tissues. We describe in this article that a dyskerin-derived peptide of eleven amino acids (GSE4) increases telomerase activity and decreases oxidative stress and the DNA damage response in cellular models of dyskeratosis congenita. Expression of GSE4 also regulates the global response of dyskeratosis congenita cells, increasing cell proliferation and reducing cellular senescence. A fibroblastoid cell line derived from a patient carrying the Ala2-Val mutation in dkc1(patient 26 in ref [26]) was used for these studies.
The results described in the present article confirm those previously shown for the 55 amino acids long fragment of dyskerin, GSE24.2, that contains GSE4. GSE24.2 increases telomerase activity and decreases oxidative stress and the DNA damage response in dyskeratosis congenita patient cells [18,19]. In addition, GSE4 protects F9-A353V dyskerin-mutant mouse cells from DNA damage and reduces oxidative stress, also as GSE24.2 [20]. Furthermore, we show in this article that GSE24.2 also increases cell proliferation and decreases cell senescence, which had not been reported previously. Therefore, we show that GSE4 presents the same biological activity than the longer peptide GSE24.2, which has been approved as an orphan drug for the treatment of dyskeratosis congenita. However, GSE4 presents some advantages over GSE24.2, derived from its smaller size. One of them is the lower cost of chemical synthesis. In addition, it could be easier to deliver into the cells. It would be also easier to develop variants that could have improved pharmaceutical characteristics.
The data presented also provide information about the mechanisms of action of these peptides. GSE4 increases telomerase activity in DKC1-mutated F9-A353V cells, increases expression of c-myc and the TERT and TERC telomerase components and the activity of TERT and c-myc promoters, as previously reported for GSE24.2 [19]. The activity of the TERT promoter has been shown to be higher in cancer cell lines than in transformed cells lines similar to those used in the present study [35] therefore, the possible effects of GSE4 on TERT expression in tumour cells should be tested in future studies. The structural studies indicate that GSE24.2 and c-myc-luc reporter or TERT-luc reporter vectors (1 μg/10 6 cells). Luciferase activity was measured 24 hours after transfection. Data were normalized by protein concentration and referred to the activity of the control vector. Data points represent the mean and standard deviations of 3 experiments performed in triplicate. Panel C, F9-A353V cells were transfected with vectors indicated on panel B. Total RNA was extracted 24 h later and the levels of c-myc, TERT and TR(TERC) expression determined by reverse transcription and quantitative PCR. Expression levels were normalized by β-actin expression and referred to the expression levels of the cells transfected with the empty vector (Vector). The data shown represent the mean and standard deviations of 3 experiments performed in triplicate. Statistical significance: * p<0.05, **p<0.01, ***p<0.001.
doi:10.1371/journal.pone.0142980.g004 and GSE4 do not require nuclear localization signals for activity. The incorporation of nuclear or nucleolar localization signals to GSE24.2 increase nuclear or nucleolar localization but the transcriptional activity of the peptide and the protective role on DNA damage are not increased. Actually, the incorporation of the nucleolar localization signal NLS2 decreases GSE24.2 activity. The GSE4 peptide containing a nuclear localization signals (GSE4-NLS1) also show a biological activity similar to that of GSE4. These observations do not discard a nuclear function for GSE24.2 or GSE4 since the localization experiments indicate that GSE24.2 and GSE4, at a lower extend, are present both at the nucleus and the cytoplasm in the absence of nuclear localization signals, probably due to their small size.
Expression of GSE24.2 and GSE4 produces biological effects on several cell types expressing either Wild type or mutated dyskerin indicating that these peptides do not just complement dyskerin mutations. They seem to play several roles in the cell. It would be interesting to determine if there is a common mechanism for these activities or not. The data reported in this article indicate that some peptide variants differ in their activities depending on the assay and/or cell type studied. For example, GSE24.2-NLS2.3 activates TERT promoter at the same extend as GSE24.2 and GSE24.2-NLS1.3 but is less effective on c-myc promoter activation and on the protection of F9 A353V basal DNA damage. In the same sense, the GSE4-NLS1-DA variant increases transcriptional activity in F9 and HEK293T cells but is not active in the dyskerinmutated F9-A353V cells neither in transcription activation nor in basal DNA damage protection. These data could indicate that these peptides participate in different cellular processes through different mechanisms. Some of the variant studied, like GSE4-NLS1-DA could require the presence of Wild-type dyskerin for some of their activities but other variants and the unmodified GSE24.2 and GSE4 peptides do not seem to be dependent on dyskerin for any of their biological activities.
In summary, the eleven amino acids long GSE4 peptide shows a protective effect on dyskerin mutated cells similar to the one previously shown for GSE24.2. Protection is mediated by increased telomerase activity and cell proliferation but also by decreased oxidative stress, DNA damage and cell senescence. These properties make of GSE4 a good candidate as a drug for dyskeratosis congenita treatment with some practical advantages over the already approved GSE24.2 peptide.
Supporting Information S1 Fig. Cellular localization of the GSE24.2 peptide containing nuclear localization signals at the N-terminal region. pcDNA3 vectors were generated coding for the GSE24.2 peptide fused to the NLS1 nuclear localization signal (KRKR) or the NLS2 signal (KKEKKKSKK) fused to the N-terminal region, named 24.2-NLS1-5 and 24.2-NLS2.5 respectively. The nuclear localization signals were placed between the N-terminal 6xmyc epitope and the GSE24.2 peptide in the proteins expressed from these vectors. HeLa cells were transformed with the pcDNA3 vectors expressing GSE24.2, 24.2-NLS1.5 and 24.2-NLS2.5, fixed, permeabilized and incubated with a c-myc antibody. Immunofluorescence staining was observed after incubation of the preparations with a secondary antibody conjugated with Alexa fluor 488 using a Nikon 90i microscope. (PDF)