Sp1 and Sp3 Are Oxidative Stress-Inducible, Antideath Transcription Factors in Cortical Neurons

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The Journal of Neuroscience, May 1, 2003, 23(9):3597

Sp1 and Sp3 Are Oxidative Stress-Inducible, Antideath Transcription Factors in Cortical Neurons
Hoon Ryu¹^,⁴, Junghee Lee¹^,⁴, Khalequz Zaman¹^,⁴, James Kubilis⁶^,⁷, Robert J. Ferrante⁶^,⁷, Brian D. Ross⁸, Rachael Neve²^,³^,⁵, and Rajiv R. Ratan¹^,³^,⁴
Departments of ¹ Neurology and ² Psychiatry and the ³ Program in Neuroscience, Harvard Medical School and ⁴ Beth Israel Deaconess Medical Center, Harvard Institutes of Medicine, Boston, Massachusetts 02115, ⁵ McLean Hospital, Belmont, Massachusetts 02478, ⁶ Geriatric Research and Education and Clinical Center, Bedford Veterans Affairs Medical Center, and ⁷ Neurology, Pathology, and Psychiatry Departments, Boston University School of Medicine, Boston, Massachusetts 02118, and ⁸ Department of Radiology, University of Michigan Medical School, Ann Arbor, Michigan 48109

  ABSTRACT

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Neuronal cell death in response to oxidative stress may reflect the failure of endogenous adaptive mechanisms. However, thetranscriptional activators induced by oxidative stress in neuronsthat trigger adaptive genetic responses have yet to be fully elucidated.We report that basal DNA binding of the zinc finger transcriptionfactors Sp1 and Sp3 is unexpectedly low in cortical neurons invitro and is significantly induced by glutathione depletion-inducedor hydrogen peroxide-induced oxidative stress in these cells.The increases in Sp1/Sp3 DNA binding reflect, in part, increasedlevels of Sp1 and Sp3 protein in the nuclei of cortical neurons.Similar induction of Sp1 and Sp3 protein is also observed in neuronsin vivo in a chemical or a genetic model of Huntington's disease,two rodent models in which neuronal loss has been attributed tooxidative stress. Sustained high-level expression of full-lengthSp1 or full-length Sp3, but not the Sp1 zinc finger DNA-bindingdomain alone, prevents death in response to oxidative stress,DNA damage, or both. Taken together, these results establish Sp1and Sp3 as oxidative stress-induced transcription factors in corticalneurons that positively regulate neuronalsurvival.

Key words: Sp1; oxidative stress; neurons; antioxidants; Huntington's disease; DNA damage

  Introduction

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Oxidative damage to proteins, lipids, or DNA is increased in human autopsy tissue and rodent models of a host of neurodegenerativeconditions, including Alzheimer's disease, Parkinson's disease,Friedreich's ataxia, Huntington's disease (HD), multiple sclerosis,and stroke (for review, see Sagara et al., 1998; Atwood et al.,1999; Browne et al., 1999; Castagne et al., 1999; Estevez et al.,1999; Floyd, 1999; Mattson et al., 1999; Ratan, 1999, Albers andBeal, 2000). Free radical damage to cell constituents in diseasestates may reflect a failure of endogenous compensatory mechanismsto oxidative stress. These compensatory mechanisms include enzymesinvolved in detoxifying reactive oxygen species (ROS) and repairingoxidative damage to DNA and protein. Therefore, further understandingof the nature and regulation of compensatory responses to oxidativestress may provide novel insights into the pathogenesis of aswell as therapy for neurologicaldiseases.

Adaptive responses to oxidative stress are most well defined in prokaryotic systems (Mongkolsuk and Helmann, 2002). Bacteriarespond to toxic levels of ROS by increasing the expression ofantioxidant and repair genes. ROS-mediated changes in gene expressionare coordinated by transcription factors. In prokaryotes, thesetranscription factors are directly and transiently modified byoxidants. For example, changes in the redox state of one transcriptionfactor (OxyR) lead to enhanced interaction of this factor withthe basal transcription machinery and increased expression ofgenes involved in detoxification (Zheng and Storz, 2000). In contrast,oxidation of the transcription factor organic hydroperoxide resistance(OhR) results in the oxidation of a single cysteine residue (Cys-15)and loss of DNA binding. The loss of OhR DNA binding leads tothe derepression of genes involved in detoxification (Fuangthongand Helmann, 2002).

Although it has been established that eukaryotic cells, including neurons, also use transcription factors to respond to ROSand activate protective responses (Lezoualc'h and Behl, 1998;Post et al., 1998; Bijur et al., 1999; Scortegagna et al., 1999),our understanding of the nature of these proteins and their modesof activation in neurons is limited. Primary cultures of corticalneurons provide a convenient in vitro preparation for examiningtranscription factors that are induced by oxidative stress (Murphyet al., 1989, 1990). Early in their development in culture, corticalneurons exposed continuously to glutamate succumb through a mechanismindependent of ionotropic glutamate receptors. Degeneration occurssubsequent to the depletion of glutathione, an important antioxidant.Cell death attributable to glutathione depletion can be completelyprevented by a host of classical antioxidants (Murphy et al.,1990) and has many features of apoptosis (Ratan et al., 1994b;Tan et al., 1998; Zaman et al., 1999).

Herein, we use this in vitro model to examine the role of the Sp1 transcription factor family in oxidative stress-inducedcell death in neurons. Sp1 is a member of an extended family ofDNA-binding proteins that have three zinc finger motifs and bindto guanosine- and cytosine-rich DNA (Briggs et al., 1986; Laniaet al., 1997; Suske, 1999; Yang et al., 2000). This family includesmembers homologous to Sp1, such as Sp2-Sp4. Sp1 activities havebeen shown to change in response to apoptosis-inducing stimuli.For example, the induction of apoptosis in B-cells after treatmentwith anti-IgM is associated with the caspase-dependent cleavageof Sp1 (Rickers et al., 1999). Similarly, apoptotic retinoidsinduce the caspase-dependent cleavage of Sp1 in T-cells (Piedrafitaand Pfahl, 1997). Indeed, polyglutamine expansions in the huntingtinprotein can induce neuronal toxicity, in part, by sequesteringSp1 and one of its coactivators, TATA binding protein-associatedfactor (TAF)II130, suggesting a role for Sp1 in neuronal survival(Dunah et al., 2002; Li et al., 2002). Of note, Sp1 has been shownto regulate prosurvival proteins [e.g., the inhibitor of apoptosis(IAP) protein, survivin (Li and Altieri, 1999), and manganesesuperoxide dismutase (Tanaka et al., 2000)] as well as prodeathproteins [e.g., Fas ligand (Xiao et al., 1999; Chou et al., 2000)and 12-lipoxygenase (Liu et al., 1997)]. Like other transcriptionfactors, the role of Sp1 in regulating cell death may depend ona number of factors, such as the cell type and the death stimulus(Lin et al., 1998).

Herein, we demonstrate that oxidative stress significantly induces Sp1 and Sp3 protein levels and DNA binding in neurons invitro and in vivo. Moreover, we demonstrate that the enforcedexpression of Sp1 or Sp3 is neuroprotective. These findings establishSp1 and Sp3 as redox-regulated transcriptional activators thatenhance survival in corticalneurons.

  Materials and Methods

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Primary neuronal culture. Cell cultures were obtained from the cerebral cortex of Sprague Dawley rats (day 17 of gestation)as described previously (Murphy et al., 1990). All experimentswere initiated 24-72 hr after plating. Under these conditions,the cells are not susceptible to glutamate-mediated excitotoxicity.For cytotoxicity studies, cells were rinsed with warm PBS andthen placed in Minimum Essential Medium (MEM; Invitrogen, Gaithersburg,MD) with 5.5 gm/l glucose, 10% FCS, 2 mM L-glutamine, and 100µM cystine, containing the glutamate analog homocysteate (HCA;1 mM). HCA was diluted from 100-fold concentrated solutions thatwere adjusted to pH 7.5.

Sp1 and Sp3 expression in mouse model of HD. Male transgenic HD mice of the R6/2 strain were originally obtained from TheJackson Laboratory (Bar Harbor, ME). The male R6/2 mice and wild-typelittermate control mice used in this study were from the BedfordVeterans Affairs facility and bred with females from their backgroundstrain (B6CBAFI/J). 3-Nitropropionic acid (3-NP; Sigma, St. Louis,MO) was dissolved in PBS, pH adjusted to 7.4, and injected intraperitoneallynine times at 12 hr intervals, using 50 mg/kg per injection inwild-type control mice. The mice were killed 3-5 hr after thelast 3-NP injection. Both R6/2 and 3-NP-treated mice were deeplyanesthetized and transcardially perfused with buffered 4% paraformaldehyde(PFA) and processed for histopathologic evaluation. Glycerol-cryoprotectedbrains were frozen-sectioned at 50 µm and immunostained with Sp1and Sp3 antibodies (1:500 dilution; Santa Cruz Biotechnology,Santa Cruz, CA) using a previously described conjugated secondantibody method (Ferrante et al., 2002).

Generation of recombinant herpes simplex virus vectors. Human Sp1, Sp3, and the Sp1 zinc finger DNA binding domain alone wereeach tagged with an N-terminal FLAG epitope and were individuallysubcloned into replication-defective herpes simplex virus (HSV)vectors (pHSVPrpUC) as described previously (Neve and Geller,1999). Cortical neurons (1 d in vitro) were infected with recombinantHSV 1 d after plating. Multiplicities of infection (MOIs) of 2were used because this MOI resulted in the transduction of 20-25%of neurons in the dish, with no cytotoxicity as measured by MTTreduction, phase contrast microscopy, or 4',6'-diamidino-2-phenylindole(DAPI) staining. Neurons were infected in serum-free medium for3-6 hr; the medium was removed; and standard, serum-containingculture medium was added. In parallel cultures, cells were treatedin the presence and absence of the glutamate analog, and after14-18 hr, they were fixed with 4% PFA in preparation for immunocytochemistry,DAPI staining, and terminal deoxynucleotidyl transferase-mediatedbiotinylated UTP nick end labeling(TUNEL).

Cell damage and death detection. Nuclear fragmentation was assessed by staining nuclear DNA using DAPI. Neuronal cells werewashed with PBS. Cells were fixed in 4% PFA in PBS for 10 minat room temperature. Cells were washed with PBS and stained withDAPI for 15 min at room temperature. More than 300 cells per slidewere scored for the incidence of nuclear fragmentation using afluorescence microscope. Cells with two or more chromatin fragmentsor shrunken condensed nuclei were consideredapoptotic.

In situ detection of nuclear DNA fragmentation by TUNEL. The specimens were rehydrated according to a standard protocol andincubated with proteinase K (Roche Diagnostics, Mannheim, Germany;20 gm/ml) for 15 min at room temperature with intervening washesin PBS. The TUNEL reaction mixture was prepared by adding 5 µlof terminal deoxynucleotidyl transferase to 45 µl of a fluorescein-labelednucleotide mixture per section. After it was washed with PBS,the TUNEL reaction mixture was applied to each section, coveredwith a coverslip, and incubated in a moist chamber for 60 minat 37°C. In control sections, the terminal deoxynucleotidyl transferasewasomitted.

Population measurements of neuronal cell viability were measured using a nonradioactive CellTiter 96 assay kit (Promega, Madison,WI). Tetrazolium dye solution was added to cortical neurons 16-24hr after the treatment of various reagents. Cells were incubatedat 37°C for 4 hr, and a solubilization/stop solution was added.Cell plates were allowed to stand overnight in a humidified atmosphere,and the absorbance was measured at 570 nm using a Molecular Devices(Menlo Park, CA) tunable 96-well platereader.

Immunoblot analysis. Cell lysates were obtained by rinsing cortical neurons with cold PBS and adding 100 mM Tris buffer, pH7.4, containing 1% Triton X-100, 150 mM NaCl, 1 mM sodium orthovanadate,5 mM sodium fluoride, 3 mM PMSF, 3 mM DTT, 0.5 µg/ml leupeptin,and 10 µg/ml aprotinin. Thirty micrograms of protein from celllysates were boiled in Laemmli buffer, and 5 mg of protein waselectrophoresed under reducing conditions on 8% polyacrylamidegels. Proteins were then transferred to a nitrocellulose membrane(Bio-Rad, Hercules, CA). Nonspecific binding was inhibited byincubation in Tris-buffered saline (TBST; 50 mM Tris HCl, pH 8.0,0.9% NaCl, and 0.1% Tween 20) containing 5% nonfat dried milkfor 0.5 hr. Primary antibodies against Sp1 (PEP2), Sp2 (K-20),Sp3 (D-20), or Sp4 (V-20) (all from Santa Cruz Biotechnology)were diluted at 1:1000 in TBST with 1% milk and exposed to membranesovernight at 4°C. Immunoreactive proteins were detected accordingto the enhanced chemiluminescence protocol (Amersham Biosciences,Arlington Heights,IL).

Immunofluorescence staining. Indirect labeling methods were used to determine the levels of endogenous or heterologous Sp1-Sp3and $beta$ -galactosidase in cortical neuronal cultures. Dissociatedcells from the cerebral cortex (3-5 × 10⁵) were seeded onto poly-D-lysine-coated eight-well culture slides(Becton Dickinson Labware, Bedford, MA) and treated with HCA asdescribed above for 4-5 hr. The cells were washed with warm PBSand fixed at room temperature for 15 min with 4% PFA. After washingwith PBS, fixed cells were incubated with blocking solution containing0.3% Triton X-100, 5% BSA, and 3% goat serum for 1 hr, followedby incubation with rabbit Sp1 antibody (1:500 dilution), rabbitanti-Sp2 polyclonal antibody (1:500), or a rabbit anti-Sp3 polyclonalantibody (1:500 dilution). After three washes with PBS, the cellswere incubated for 1 hr with FITC-conjugated goat-anti-rabbitIgG antibody (1:200 dilution) and DAPI. All antibodies were dilutedin PBS. The slides were washed three times with PBS and mountedwith fluorochrome mounting solution (Vector Laboratories, Burlingame,CA). Images were analyzed under a fluorescence microscope (modelAX70TRF; Olympus Optical, Tokyo, Japan). Control experiments wereperformed in the absence of primaryantibody.

Electrophoretic mobility shift assays and supershift analysis. We performed electrophoretic mobility shift assays (EMSAs)on nuclear extracts from cortical neurons using a ³²P-labeled oligonucleotide containing a wild-type (wt) or mutantSp1 binding site (Santa Cruz Biotechnology). The sense strandsequences of the double-stranded wt and mutant oligonucleotidesare 5'-ATTCGATCGGGGCGGGGCGAGC-3' and 5'-ATTCGATCGGTTCGGGGCGAGC-3',respectively. Parallel EMSAs were performed using a radiolabeledOct-1 (5'-TGTCGAATGCAAATGACTAGAA-3'; Santa Cruz Biotechnology)binding site. Embryonic cortical neurons were lightly trypsinized,pelleted, and resuspended in cold PBS. All subsequent steps wereperformed at 4°C as described previously (Lin et al., 1995, Chatterjeeet al., 2001). To evaluate the effects of various agents on Sp1and Sp3 DNA binding, we added deferoxamine mesylate (10 µM), D-aminoacid oxidase (1-5 mU from red yeast), and D-alanine (20 mM).

Promoter activity assay. Cortical neurons were plated onto 24-well culture plates (Nunc, Naperville, IL). The next day, atransfection mixture was prepared by adding 1.5 µg of the reporterexpression vector (pSp1-Luc and pmtSp1-Luc, firefly luciferaseplasmid) into 150 µl of DMEM with a combination of pRL cytomegalovirusor thymidine kinase vector (1 µg, containing the Renilla luciferasegene) (Hsiao et al., 1997). Twenty minutes after the additionof DMRIE-C reagent (6 µl; Invitrogen), the transfection mixturewas combined with 1.0 ml of fresh medium and placed onto the cellsin 24-well plates. The cells were incubated for 24 hr, and thencells were infected with HSV-Flag-Sp1, HSV-Sp3, or HSV-Sp1-ZnF(zinc finger) with or without HCA. The next day, cells were washedwith PBS and then lysed with luciferase assay buffer (Promega).The cell particulate was removed by microcentrifugation, and theprotein concentration was measured using a protein assay kit (Bio-Rad).Twenty microliters of lysate were used for both the firefly andRenilla luciferase readings. Firefly and Renilla luciferase activitieswere measured using a dual-luciferase reporter assay system (Promega)and a TD-20/20 luminometer. Firefly luciferase values were standardizedto Renilla values or total proteinconcentration.

  Results

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Oxidative stress induces Sp1 response element-binding activities in cortical neuronal cultures

To determine the effects of glutathione depletion-induced oxidative stress on Sp1 DNA binding in cortical neurons, we performedEMSAs on nuclear extracts from control cells or cells treatedwith the glutamate analog HCA, using a radiolabeled oligonucleotidecontaining a consensus Sp1 DNA-binding site. Five hours of HCAtreatment, which leads to a 70% reduction in glutathione levelscompared with control (Zaman et al., 1999), significantly increasedthree DNA-binding activities in cortical neurons (Fig. 1A; thethree DNA-binding activities are designated a-c). The inductionof these DNA-binding activities appeared to be related to glutathionedepletion because they were also observed in the presence of buthioninesufloximine (100 µM), an agent that depletes glutathione [to <10%of control levels (Ratan et al., 1994a)] by inhibiting one ofthe enzymes involved in its synthesis rather than by inhibitingthe uptake of its rate-limiting amino acid precursor (data notshown). All three DNA-binding activities were inhibited in a concentration-dependentmanner by cold Sp1 oligonucleotide, and none was inhibited byan oligonucleotide containing mutations in the Sp1-binding site(data not shown). Enhanced DNA binding could be observed as earlyas 2 hr after HCA treatment (Fig. 1C), a time when glutathionelevels are 50% of levels in mock-treated cultures, permittingsufficient time for genes to be expressed before cell death commitment(~12 hr after HCA treatment).

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Figure 1. Glutathione depletion-induced oxidative stress induces Sp1 and Sp3 DNA-binding activity in cortical neurons. A, EMSA performed with increasing amounts of protein from nuclear extracts (NEs) from control (lanes 1, 3, 5) and HCA (a glutamate analog)-treated neurons (lanes 2, 4, 6), 4 hr after the onset of HCA treatment. The three DNA-binding activities induced by oxidative stress are designated a-c. B, Identification of Sp1 in complex a and Sp3 in complexes b and c by supershift analysis using subunit-specific antibodies to Sp1-Sp4. C, Time course of induction of Sp1 and Sp3 DNA-binding activities after HCA (1 mM) treatment. D, The effect of HCA-induced glutathione depletion on Oct-1 DNA-binding activity is shown 4 hr after the onset of HCA treatment. Effects of increasing concentrations of HCA on nuclear Sp1 (E) and Sp3 (F) protein levels 4-5 hr after the onset of HCA treatment are shown. G, Time course of changes of nuclear Sp1 and Sp3 levels after the onset of HCA treatment. Examples are representative of three to five independent experiments.

Identification of Sp1 and Sp3 in nuclear extracts of cortical neurons after treatment with the glutamate analog HCA

To determine whether Sp1 was present in any of the HCA-induced DNA-protein complexes detected by EMSA, we used antibodiesspecific for the Sp1-Sp4 subunits. Sp2-Sp4 share extensive sequencehomology with Sp1, and each of these Sp family members binds specificallyto DNA. The addition of individual subunit-specific antibodiesduring in vitro DNA binding revealed that Sp1 is contained inthe slowest migrating complex (Fig. 1B). This complex did notcontain other Sp family members, including Sp2-Sp4.

In addition to an Sp1-containing complex, two faster-migrating complexes were also induced by HCA-induced glutathione depletion.These complexes were supershifted by a subunit-specific antibodyto Sp3 and were unaffected by Sp1, Sp2, and Sp4 antibodies. Takentogether, these results suggest that one Sp1-containing complexand two Sp3-containing complexes are induced by glutathione depletionin cortical neurons. The differences between nuclear Sp1 and Sp3DNA activity in control and HCA-treated cortical neurons couldnot be attributed to global differences in nuclear proteins, becauselevels of Oct-1 DNA binding were similar using 0.5 µg of thesetwo extracts (Fig. 1D).

Enhanced DNA-binding activity of Sp1 and Sp3 in response to oxidative stress results, in part, from increased levels of Sp1 and Sp3 protein

Previous studies have established that DNA binding of Sp family members to their cognate sequence can be enhanced by increasinglevels of Sp1 protein (Mortensen et al., 1997) or post-transcriptionalmodifications of the protein such as phosphorylation (Rohlff etal., 1997) or dephosphorylation (Leggett et al., 1995). To determinewhether HCA-induced oxidative stress induces changes in Sp1 andSp3 levels, we performed immunoblot analysis. We found that HCAleads to increases in both Sp1 and Sp3 protein levels (Fig. 1E).Five millimolar HCA leads to more rapid cystine deprivation andglutathione depletion after 5 hr than 1 mM HCA (Ratan et al.,1994a). As expected from these observations, treatment of corticalneurons with 5 mM HCA for 5 hr induced greater levels of Sp1 (Fig.1E) and Sp3 (Fig. 1F) proteins than did 1 mM HCA. A rabbit polyclonalSp1 antibody detected a dominant band at 95 kDa and a minor bandat 105 kDa. This slower-migrating band at 105 kDa likely reflectsphosphorylation of the 95 kDa Sp1 polypeptide, because the 95kDa band completely disappeared in the presence of the phosphataseinhibitor, calyculin A (Ryu et al.) (our unpublished observations).A rabbit polyclonal Sp3 antibody detected a dominant 115 kDa bandcorresponding to Sp3 previously identified by both immunochemicaland molecular genetic techniques (Kennett et al., 1997). A minor,faster-migrating band was observed at 78-80 kDa, a species ofSp3 that has been shown to result from internal translationalinitiation within Sp3 mRNA (Kennett et al., 1997). The increasesin Sp1 and Sp3 proteins were seen as early as 1 hr after HCA treatment,were maximum at 5 hr (Fig. 1G), and could be observed to be returningto baseline levels by 8 hr after HCA treatment (results notshown).

Glutathione depletion-induced oxidative stress induces Sp1 and Sp3 levels in the nucleus of cortical neurons

To verify that Sp1 and Sp3 proteins can be induced in the nuclei of neurons by HCA-induced glutathione depletion, we performedimmunocytochemical staining with antibodies to Sp1 (Fig. 2a,d),Sp2 (Fig. 2g,j), and Sp3 (Fig. 2m,p), using in all cases an FITC-labeledsecondary antibody that fluoresces green. In parallel, the samecultures were treated with the nuclear stain DAPI, which fluorescesblue (Molecular Probes, Eugene, OR) (Fig. 2b,e,h,i,n,o). Whenthe Sp1, Sp2, and Sp3 antibody fluorescence images were superimposedon the DAPI fluorescence images, most cells that were inducedto undergo oxidative stress by treatment with HCA and stainedwith an Sp1 or Sp3 antibody were found to have blue-green nuclei,indicative of an enhanced protein level in the nucleus (Fig. 2f,r).Moreover, staining with the Sp2 antibody revealed that levelsof this protein were not altered in the cytoplasm or nucleus byHCA-induced glutathione depletion and oxidative stress (Fig. 2g-l).Cells that stained positively for Sp1 and Sp3 were determinedto be neuronal by parallel immunostaining with a neurofilamentantibody (data not shown) as previously described (Zaman et al.,1999).

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Figure 2. HCA-induced glutathione depletion and oxidative stress induce Sp1 (A) and Sp3 (C), but not Sp2 (B), in the nucleus of embryonic cortical neurons. Immunocytochemical analysis of Sp1 (a, d), Sp2 (i), Sp3 (m, p), and the nuclear stain DAPI (b, e, h, k, n, q) in mock-treated (a, g, m, b, h, n) or HCA-treated (d, j, e, k, q) mixed cortical neuronal cultures. Cells were plated on eight-well chamber slides for 24 hr and treated with HCA (3 mM) for 3 hr. Cells were then fixed with 4% PFA for 15 min, and immunofluorescence staining was performed as described in Materials and Methods. Scale bar, 20 µm.

Antioxidants that prevent glutathione depletion-induced apoptotic death also prevent glutathione depletion-induced Sp1 and Sp3 DNA binding

Oxidative stress is defined as an imbalance between oxidants and antioxidants in favor of oxidants (Sies, 1997; for review,see Ratan, 1999). Thus, if oxidative stress is responsible forthe HCA-induced Sp1 and Sp3 DNA binding, then antioxidants thatcorrect the imbalance should diminish or suppress the induction.To address this question, we chose the iron chelator deferoxamine(DFO; 100 µM) and the non-iron-chelating lipid peroxidation inhibitorbutylated hydroxyanisole (BHA; 10 µM). We have demonstrated previouslythat these antioxidants completely abrogate HCA-induced apoptosisin cortical neurons (Ratan et al.,1994b, Zaman et al., 1999).In gel-shift assays, we found that DFO (Fig. 3A) and BHA (Fig.3B) suppress HCA-induced Sp1 and Sp3 DNA binding. These resultssuggest that HCA-induced oxidative stress mediates enhanced DNAbinding of Sp1 and Sp3 in cortical neurons. We demonstrated previouslythat DFO enhances the DNA binding of hypoxia-inducible factor-1and activating transcription factor-1/cAMP response element-bindingprotein to the hypoxia response element (Zaman et al., 1999),suggesting that its inhibition of Sp1 and Sp3 activation doesnot reflect nonspecific inhibition of the DNA binding of all transcriptionfactors.

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Figure 3. Increases in Sp1 and Sp3 DNA binding induced by the glutamate analog HCA are inhibited by antioxidants; Sp1 and Sp3 DNA binding in cortical neurons are activated by hydrogen peroxide. Induction of Sp1 and Sp3 DNA binding by HCA-induced glutathione depletion (4 hr) is decreased by the antioxidant iron chelator DFO (100 µM; A) and the lipid peroxidation inhibitor BHA (10 µM; B). C, Addition of exogenous peroxide, generated by the enzyme DAAO and its substrate D-ala (20 mM) for 4 hr increases Sp1 and Sp3 DNA binding in a concentration-dependent manner in cortical neurons. The induction is observed despite no morphological or biochemical evidence of cell death in cortical neurons. D, Addition of catalase abrogates Sp1 and Sp3 DNA binding induced by D-ala (20 mM) and DAAO (5 mU). Examples are representative of three to five independent experiments.

To determine whether the addition of the ROS hydrogen peroxide to cortical neurons is also capable of inducing Sp1 and Sp3DNA binding, we added increasing concentrations of the enzymeD-amino acid oxidase (DAAO; 1-5 mU) and its substrate D-alanine(D-ala; 20 mM) to the bathing medium of embryonic rat corticalneurons. DAAO catalyzes the stereoselective oxidative deaminationof D-amino acids to form hydrogen peroxide via the following reaction:D-amino acid + H₂O + O₂ $right-arrow$ $alpha$ -keto acid + NH₃ + H₂O₂ (Stegman etal., 1998). As expected, we found that hydrogen peroxide generatedfrom DAAO induces three complexes in cortical neurons in a concentration-dependentmanner (Fig. 3C). Supershift analysis confirmed that, like glutathionedepletion, the slowest migrating complex contains Sp1, and thetwo faster-migrating complexes contain Sp3 (data not shown). Inaddition, D-ala/DAAO-induced Sp1 and Sp3 DNA binding could becompletely suppressed by the coapplication of the peroxide-scavengingenzyme catalase (100 U/ml; Fig. 3D) or the nonenzymic peroxidescavenger pyruvate (2 mM; data notshown).

These results establish that Sp1 and Sp3 are oxidative stress-inducible transcription factors in vitro. To determine whetherSp1 and Sp3 protein levels can be similarly induced in vivo inrodent models in which neuronal loss has been attributed, in part,to oxidative stress, we examined Sp1 and Sp3 immunoreactivityin a transgenic mouse model or a chemical mouse model of HD (Fig.4). The R6/2 line is a transgenic mouse line expressing exon 1of the human HD gene with an expanded CAG repeat (Mangiarini etal., 1996). The mice develop loss of brain and body weight beginningat 6 weeks of age, and at 9-11 weeks, they develop a gait andmovement disorder as well as epilepsy. These clinical features,along with striatal atrophy and neuronal intranuclear inclusions,are similar to HD in humans. At 12 weeks of age, Sp1 and Sp3 levelsin the brains of R6/2 mice were found to be significantly increasedcompared with their littermate controls, as monitored by immunohistochemistry(Fig. 4A-F) or Western blot analysis (Fig. 4G). Sp1 and Sp3 weresimilarly induced in cells in the region adjacent to neuronalloss in response to the 3-NP. 3-NP is a mitochondrial toxin thatproduces striatal lesions that mimic HD and that are mediatedby excitotoxicity-induced oxidative stress mechanisms (Beal etal., 1993; Kim and Chan, 2002). Taken together, these resultsare consistent with the notion that Sp1 and Sp3 are induced bystimuli that lead to oxidative stress in vivo.

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Figure 4. Sp1 and Sp3 tissue immunoreactivity in R6/2 transgenic mice and 3-NP-lesioned-mice. Sp1 (A-C) and Sp3 (D-F) immunoreactivities in the neostriatum of 12-week-old wild-type littermate control mice (A, D) and R6/2 transgenic HD mice (B, E) and 3-NP-lesioned wild-type mice (C, F) are shown. Sp1 and Sp3 immunostaining of neurons in wild-type control mice (A, D) is shown. Markedly increased Sp1 and Sp3 immunoreactivity was observed in R6/2 mice compared with wild-type controls, with the greatest increases in Sp3 immunoreactivity. In 3-NP-lesioned mice, Sp1 (C) and Sp3 (F) immunoreactivities were both increased within neurons surrounding the lesion core (asterisk) within the penumbra or transition zone of neuronal injury. Scale bars: (in E) A, B, D, E, 100 µm; (in F), C, F, 200 µm. G, Sp1 and Sp3 protein levels in 12-week-old littermate controls and R6/2 transgenic mouse model of HD. $alpha$ -Tubulin was used as a loading control. H, Scatter plot of densitometric values (normalized to $alpha$ -tubulin) for Sp1 and Sp3 protein levels in seven littermate control and nine R6/2 HD mice.

Forced high-level expression of full-length Sp1 or full-length Sp3, but not its zinc finger DNA-binding domain alone, prevents cortical neuronal death attributable to oxidative stress or DNA damage

To determine whether the overexpression of Sp1 is sufficient to abrogate glutathione depletion-induced death in cortical neurons,we generated replication-deficient HSV-1-based vectors that carrythe wild-type Sp1 gene (HSV-Sp1-wt) or a truncated form of Sp1containing the DNA-binding domain alone (HSV-Sp1-ZnF). Sp1-ZnFcan bind DNA but does not possess regions of the Sp1 moleculerequired for activation of transcription (Chapman and Perkins,2000). As an additional control, we inserted the $beta$ -galactosidase(LacZ) gene into the HSV vector (HSV-LacZ). Infection of corticalneurons with HSV-Sp1-wt (Fig. 5A) but not HSV-Sp1-ZnF (Fig. 5A)or HSV-LacZ (Fig. 5D), resulted in the robust, MOI-dependent expressionof heterologous Sp1 in cortical neurons as monitored by an anti-Sp1antibody (Fig. 5A,D) or by an anti-Flag antibody (Fig. 5D) 6-12hr after infection. An MOI of 2 was used for the HSV viabilityexperiments, because this MOI resulted in infection of ~15-25%of the neurons in the dish (Fig. 5C) with no toxicity up to 48hr after infection. The overexpression of Sp1 by HSV led to athreefold induction of Sp1-dependent luciferase activity comparedwith HSV-LacZ.

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Figure 5. HSV can be used to achieve expression of heterologous Sp1 in cortical neurons. A, Immunoblot demonstrating expression of heterologous Sp1 in cortical neurons 24 hr after infection with HSV vectors. HSV has an MOI of 2. B, HSV-LacZ leads to MOI-dependent $beta$ -galactosidase expression in cortical neurons. C, HSV-Sp1 infection of cortical neurons leads to induction of luciferase activity driven by Sp1 response elements compared with HSV-LacZ. Results are means ± SE for three separate experiments. D, Immunoblot analysis confirms MOI-dependent, HSV vector-driven expression of Sp1 (HSV-Sp1) or $beta$ -galactosidase. In parallel, immunoblotting with Flag antibody confirms that HSV-Sp1 results in heterologous rather than endogenous Sp1 expression.

To determine the effect of enhancing Sp1 activity using the HSV vector on oxidative stress-induced death in cortical neurons,we monitored the viability of cells infected with HSV-LacZ, HSV-Sp1-wt,and HSV-Sp1-ZnF 17-24 hr after infection. LacZ is expressed diffuselyin the cytoplasm (Fig. 6A) and the neurites of neurons, whereasthe Sp1-wt and the Sp1-ZnF are found primarily in the nuclearcompartment (Fig. 6A). Under control, nonoxidative stress conditions,the nuclei of cells infected with HSV-LacZ, HSV-Sp1-wt, or HSV-Sp1-ZnFand stained with the nuclear probe DAPI appeared oval in shapeand homogeneously stained with moderate intensity. These apparentlynormal nuclei were present in neurons with smooth cell bodiesand ramified neurites, as determined by Nomarski differentialinterference contrast microscopy. Parallel cultures were infectedwith HSV-LacZ, HSV-Sp1-wt, or HSV-Sp1-dominant negative (dn),exposed to the glutamate analog HCA for 16-18 hr, and stainedwith DAPI or visualized by Nomarski optics. Cells infected withHSV-Sp1-ZnF or HSV-LacZ and exposed to HCA showed massive changesin chromatin structure (condensation), indicated by greatly enhancedDAPI fluorescence. These changes in chromatin structure are consistentwith the apoptotic cell death observed previously in corticalneurons exposed to glutathione depletion (Ratan et al., 1994b).By contrast, cells infected with HSV-Sp1-wt that were exposedto oxidative stress generally retained the oval, moderately intensestaining of normal nuclei. Two independent observers who wereblinded to the treatment group quantitated the number of LacZ-,Sp1-wt-, and Sp1-ZnF-expressing cells that possessed normal nuclearmorphology under conditions of oxidative stress and confirmedthat cells expressing the heterologous Sp1-wt were significantlymore resistant to glutathione depletion-induced death than cellsexpressing heterologous LacZ or Sp1-ZnF (Fig. 6B). In addition,TUNEL (a marker of DNA damage resulting from HCA-induced oxidativestress) was performed along with immunfluorescence for Sp1, LacZ,or Sp1-ZnF (Fig. 6C). These experiments showed that after 18 hrof HCA (1 mM) treatment, only LacZ- or Sp1-ZnF-expressing neuronswere TUNEL-positive, whereas cells expressing Sp1 were not (Fig.6C).

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Figure 6. Overexpression of Sp1 (HSV-Flag-Sp1), but not the Sp1 Zn finger DNA binding domain alone (HSV-Flag-Sp1-ZnF) or HSV-LacZ, in cortical neurons inhibits oxidative stress-induced cell death in cortical neurons. A, DAPI staining of LacZ-positive, Flag-Sp1-positive, or Flag-Sp1-ZnF-positive cortical neurons. The FITC column reflects FITC secondary antibody that recognizes LacZ-, Flag-Sp1-wt-, or Flag-Sp1-ZnF-expressing cortical neurons. Note the presence of LacZ in cell bodies as well as neurites, which is typical of cortical neurons in culture. Also note the presence of Sp1-wt and Sp1-ZnF in the nucleus, the expected localization for these transcription factors. The DAPI column shows the DAPI staining of FITC-positive cells in the same row, along with a few surrounding FITC-negative cells. Note that HCA produces an increase in the percentage of cells with pyknotic nuclei that display stronger fluorescence, which is characteristic of apoptotic cells. However, the Flag-Sp1-wt-expressing neurons display dim, diffuse DAPI staining, which is characteristic of normal cells. Cortical neurons were infected with 2-5 MOI of HSV vectors. B, Quantitative analysis. Overexpression of Flag-Sp1-wt but not Flag-Sp1-ZnF or LacZ blocks the increase in apoptotic cells elicited by HCA (LacZ or Sp1-ZnF vs Sp1-wt, p < 0.01). At least 300 cells were counted in each group, and the results are means ± SE for three different slides. C, TUNEL was performed to measure HCA-induced DNA damage of LacZ-positive, Flag-Sp1-positive, and Flag-Sp1-ZnF-positive cortical neurons. Cy3 (red) column reflects Cy3 secondary antibody that recognizes LacZ, Flag-Sp1, Flag-Sp3, or Sp1-ZnF. The overlay column reflects green TUNEL-FITC fluorescence superimposed on red Cy3 secondary antibody fluorescence for $beta$ -galactosidase, Sp1, and Sp1-ZnF and blue fluorescence for the nucleus.

To determine whether the overexpression of Sp1 using herpes vectors can inhibit death induced by apoptotic stimuli distinctfrom glutathione depletion, we examined the effects of HSV-Sp1-wtinfection of cortical neurons on apoptosis induced by the DNA-damagingagent camptothecin. Camptothecin is a cytotoxic plant alkaloidthat induces cell injury by inhibiting the activity of DNA topoisomeraseI, which leads to double-stranded DNA damage (Ng et al., 2001).Previous studies have established that, like glutathione depletion,cortical neuronal death induced by camptothecin has characteristicmorphological features of apoptosis. Unlike the case with glutathionedepletion-induced apoptosis, camptothecin-induced apoptosis isnot associated with increased hydrogen peroxide production andis not blocked by the antioxidant N-acetylcysteine. Cell viability,as measured by MTT reduction, revealed that cortical neurons infectedwith HSV-Sp1-wt, but not HSV-LacZ or HSV-Sp1-dn, were more resistantto camptothecin-induced death over a range of camptothecin concentrations(Fig. 7A). In parallel cultures, TUNEL [a marker of DNA double-strandbreaks resulting from camptothecin-induced topoisomerase inhibition(Morris and Geller, 1996)] was performed along with immunfluorescencefor Sp1, LacZ, or Sp1-ZnF (Fig. 7B). These studies revealed thatafter 18 hr of camptothecin treatment, only LacZ- or Sp1-ZnF-expressingneurons were TUNEL-positive, whereas cells expressing Sp1 or Sp3were not. Taken together, these studies suggest that the overexpressionof Sp1 or Sp3 can abrogate neuronal damage and death attributableto oxidative stress or other established apoptosis inducers, includingthe topoisomerase inhibitor camptothecin (Fig. 7).

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Figure 7. Overexpression of Sp1-wt or Sp3-wt, but not the Sp1-ZnF or LacZ, inhibits neuronal death attributable to the DNA-damaging agent and topoisomerase inhibitor camptothecin. A, Quantitative analysis. Overexpression of Flag-Sp1 or Flag-Sp3 but not LacZ or Flag-Sp1-ZnF diminishes cell death induced by camptothecin (2-10 µM). Cortical neurons were infected with 2-5 MOI of HSV vectors. Cell viability was measured by incubating cortical neurons with MTT for 2 hr and measuring the amount of reduction to blue formazan. Results are means ± SE for three separate experiments. B, TUNEL, a marker of DNA double-strand breaks resulting from camptothecin-induced topoisomerase inhibition (Morris and Geller, 1996) of LacZ-positive, Flag-Sp1-positive, Flag-Sp3-positive, or Flag-Sp1-ZnF-positive cortical neurons. The Cy3 (red) column reflects Cy3 secondary antibody that recognizes LacZ, Flag-Sp1, Flag-Sp3, or Sp1-ZnF. The overlay column reflects green TUNEL-FITC fluorescence superimposed on red Cy3 secondary antibody fluorescence. Note that only cells expressing LacZ or Flag Sp1-ZnF are yellow, whereas Cy3-positive Flag-Sp1- and Flag-Sp3-expressing cells are not TUNEL labeled and are therefore red.

  Discussion

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Sp1 and Sp3 are redox-regulated transcription factors in neurons

There is abundant evidence linking oxidative stress to the initiation or propagation of neuronal loss in neurological disease(Beal, 2000). This evidence has stimulated a search for transcriptionalregulators that are induced by oxidative stress in neurons whosenet effect is to prevent neuronal death (Ratan, 1999). Herein,we demonstrate that basal Sp1 DNA-binding activities are unexpectedlylow in embryonic cortical neurons and are dramatically inducedby agents that induce oxidative stress in these cells (Figs. 1,2, 4A). Second, we used gel-shift assays to show that one of theSp1 DNA-binding complexes induced by oxidative stress in corticalneurons contains Sp1, and two slower-migrating complexes containinSp3 (Fig. 1B). Furthermore, we used immunoblot analysis (Fig.1E-G) and immunocytochemistry (Fig. 1H) to demonstrate that proteinlevels of these transcription factors are increased in the nucleiof oxidatively stressed cortical neurons and that antioxidantsshown previously to inhibit oxidative stress-induced death incortical neurons also abrogate glutathione depletion-induced Sp1and Sp3 DNA binding (Fig. 2A,B). Finally, we demonstrate thatoxidative stress can enhance the activity of an Sp1-dependentreporter gene (data not shown). These results establish Sp1 andSp3 as redox-regulated transcription factors in embryonic corticalneurons and add these factors to a small list of transcriptionalactivators and repressors (e.g., nuclear factor $kappa$ B, activatorprotein-1, and heat shock transcription factor-1) known to beinduced by oxidative stress in neurons (Lezoualc'h and Behl, 1998;Post et al., 1998; Bijur et al., 1999; Scortegagna et al., 1999).

Sp1 and Sp3 activation appear to be temporally related to the onset of oxidative stress in cortical neurons and not a lateevent that is a consequence of oxidative stress-induced cell death.Activation of Sp1 and Sp3 DNA binding occurs within the first2 hr of glutamate or HCA exposure and is maximal by 5 hr. Thekinetics of Sp1 and Sp3 activation demonstrate that inductionof these factors is an "early" response to cell stress, and theiractivation is initiated 8-10 hr before the point at which neuronsbecome irreversibly "committed" to the cell death pathway (Ratanet al., 1994b; Zaman et al., 1999; Chatterjee et al., 2001). Theclose temporal relationship between oxidative stress and Sp1 andSp3 activation is also supported by the observation that structurallydiverse antioxidants known to ameliorate oxidative stress andinhibit oxidative glutamate toxicity can block the activationof Sp1 and Sp3 by glutathione depletion, despite having no effecton glutathione depletion per se (Ratan et al., 1994a; Zaman etal., 1999).

Although classically thought to regulate the constitutive expression of numerous housekeeping genes, Sp1 transcriptional activitieshave been found to change in association with differentiation(Leggett et al., 1995; Yan and Ziff, 1997; Krainc et al., 1998)and proliferation (Black et al., 1999) and to regulate gene expressionin association with these as well as other cellular functions.In agreement with the data presented herein, one of these studiesdemonstrated nearly absent basal DNA binding of Sp1 and Sp3 inorgans such as brain and muscle, in which most cells are postmitotic(Leggett et al., 1995). Two-dimensional electrophoresis revealedthat the decreased DNA binding of Sp1 and Sp3 in postmitotic tissuesis associated with the phosphorylation of Sp1 and Sp3. Accordingly,in vitro treatment of nuclear extracts from adult brain with aphosphatase abolished Sp1 and Sp3 phosphorylation and increasedthe affinity of these factors for a canonical Sp1 DNA-bindingsite by 10-fold. These results are consistent with a model inwhich the post-translational modification of Sp1 by activationof a phosphatase (dephosphorylation) or inhibition of a histonedeacetylase (acetylation) (Ryu et al., 2003) could account forthe dramatic increase in DNA binding we observe in response tooxidative stress. Our ability to observe oxidative stress-inducedchanges in Sp1 and Sp3 DNA binding is likely also enhanced, becausewe have been careful to verify that the concentration of the nuclearextract we use is in the dynamic range of DNA binding for Sp1and Sp3 (Fig. 1A).

Sp1 and Sp3 can act as antideath transcription factors

The data herein support the conclusion that Sp1 and Sp3 are sufficient components of the protective, homeostatic responseto oxidative stress (Fig. 6) and one potential consequence ofoxidative stress, DNA damage (Fig. 7), in neurons. Indeed, recentstudies suggest that Sp1 motifs are responsible for the regulationof the IAP protein survivin (Li and Altieri, 1999). Members ofthe IAP protein family have been shown to suppress apoptosis inducedby oxidative stress by directly suppressing the activity of terminalcaspase-3 and caspase-7 (Tamm et al., 1998; Suzuki et al., 2000).Interestingly, survivin is expressed not only in common humancancers but also in some types of embryonic neurons (Adida etal., 1998), suggesting that this protein is poised to act as aninhibitor of apoptosis in the cortical neurons used in the presentstudy. Bcl-2 and Bcl-x, two other general inhibitors of apoptosis,also have essential Sp1 sites in their promoters (Grillot et al.,1997; Dong et al., 1999), and p53 has been shown to repress theexpression of the antiapoptotic factor telomerase by binding tocognate Sp1 motifs in the telomerase promoter (Kanaya et al.,2000). Finally, Sp1 is cleaved by caspases in IgM-induced apoptosisin B cells (Rickers et al., 1999) and in retinoid-induced apoptosisin T-cells (Piedrafita and Pfahl, 1997). Taken together, theseobservations support an antiapoptotic role forSp1.

Inhibition of Sp1 activation in polyglutamine disorders such as HD may account for increased vulnerability to oxidative stress

The data herein are consistent with a model in which Sp1 is a part of a compensatory genetic program to oxidative stress inneurons. A prediction of this model is that neurons with acquiredor inherited defects in Sp1 signaling will be more vulnerableto oxidants. Indeed, autopsy tissue from HD patients shows prominentdefects in Sp1 DNA binding (despite increased Sp1 levels; Dunahet al., 2002) (Fig. 3) and increased markers of oxidative damage(Browne et al., 1999). Furthermore, toxicity of cultured neuronsinduced by the forced expression of mutant huntingtin with pathologicalnumbers of polyglutamine repeats can be abrogated by the coexpressionof Sp1 and its coactivator TAFII130 (Dunah et al., 2002; Li etal., 2002) or by the exogenous addition of small-molecule antioxidants(Wyttenbach et al., 2002). Future studies will define the preciseorder of oxidative stress and disrupted Sp1 signaling in HD. Nevertheless,these findings suggest that small-molecule activators of Sp1-dependentgene expression may be propitious therapeutic targets for a hostof neurodegenerative conditions, including HD, Parkinson's disease,amyotrophic lateral sclerosis, and stroke, which in some caseshave been associated with expanded polyglutamine repeats and inall cases have been associated with oxidativestress.

  FOOTNOTES

Received Jan. 2, 2003; revised Feb. 6, 2003; accepted Feb. 21, 2003.

This work was supported by National Institutes of Health Grants R29 NS34943 and R01 NS39170 to R.R.R. The cDNA for the zincfinger domain of Sp1 was a gift from Dr. Neil Perkins (Departmentof Biochemistry, University of Dundee, Dundee, UK) and the full-lengthSp1 and Sp3 were gifts from Dr. Guntram Suske (Institute of MolecularBiology and Tumor Research, Philipps-University Marburg, Marburg,Germany). We thank Rini Ratan and Donald DeFranco for carefulreview of thismanuscript.

Correspondence should be addressed to Dr. Rajiv R. Ratan, Neurology Laboratories at Beth Israel Deaconess Medical Center,Harvard Institutes of Medicine, Room 857, 77 Avenue Louis Pasteur,Boston, MA 02115. E-mail: rratan{at}caregroup.harvard.edu.

Dr. Ryu's present address: Department of Neurology, University of Massachusetts Medical School and Memorial Medical Center,Worcester, MA 06105

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