Defective DNA Ligation during Short-Patch Single-Strand Break Repair in Ataxia Oculomotor Apraxia 1

Ataxia oculomotor apraxia 1 (AOA1) results from mutations inaprataxin, a component of DNA strand break repair that removesAMP from 5' termini. Despite this, global rates of chromosomalstrand break repair are normal in a variety of AOA1 and otheraprataxin-defective cells. Here we show that short-patch single-strandbreak repair (SSBR) in AOA1 cell extracts bypasses the pointof aprataxin action at oxidative breaks and stalls at the finalstep of DNA ligation, resulting in the accumulation of adenylatedDNA nicks. Strikingly, this defect results from insufficientlevels of nonadenylated DNA ligase, and short-patch SSBR canbe restored in AOA1 extracts, independently of aprataxin, bythe addition of recombinant DNA ligase. Since adenylated nicksare substrates for long-patch SSBR, we reasoned that this pathwaymight in part explain the apparent absence of a chromosomalSSBR defect in aprataxin-defective cells. Indeed, whereas chemicalinhibition of long-patch repair did not affect SSBR rates inwild-type mouse neural astrocytes, it uncovered a significantdefect in Aptx^–^/^– neural astrocytes. These datademonstrate that aprataxin participates in chromosomal SSBRin vivo and suggest that short-patch SSBR arrests in AOA1 becauseof insufficient nonadenylated DNA ligase.

INTRODUCTION

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INTRODUCTION

Oxidative stress is an etiological factor in many neurologicaldiseases, including Alzheimer's disease, Parkinson's disease,and Huntington's disease. One type of macromolecule damagedby reactive oxygen species is DNA, and oxidative damage to DNAhas been suggested to be a significant factor in these and otherneurological conditions (2). In particular, a number of rarehereditary neurodegenerative disorders have provided directsupport for the notion that unrepaired DNA damage causes neuraldysfunction. Not least of these are the recessive spinocerebellarataxias, a number of which are associated with mutations inDNA damage response proteins (17). The archetypal DNA damage-associatedspinocerebellar ataxia is ataxia-telangiectasia (A-T), in whichmutations in ATM protein result in defects in the detectionand signaling of DNA double-strand breaks (DSBs) (3). A-T-likedisorder is a related disease that exhibits neurological featuressimilar to those of A-T, resulting from mutation of Mre11, acomponent of the MRN complex that operates in conjunction withATM during DSB detection and signaling (28).

Two additional spinocerebellar ataxias are spinocerebellar ataxiawith axonal neuropathy 1 (SCAN1) and ataxia oculomotor apraxia1 (AOA1), in which the TDP1 and aprataxin proteins are mutated,respectively (9, 19, 27). Both TDP1 and aprataxin are componentsof the DNA strand break repair machinery (recently reviewedin references 6 and 24). Whereas SCAN1 is currently limitedto nine individuals from a single family, AOA1 is one of thecommonest recessive spinocerebellar ataxias. Aprataxin is amember of the histidine triad superfamily of nucleotide hydrolases/transferasesand has been reported to remove phosphate and phosphoglycolatemoieties from the 3' termini of DNA strand breaks (26). Aprataxincan also remove AMP from a variety of ligands in vitro, includingadenosine polyphosphates, AMP-lysine, AMP-NH₂ (adenine monophosphoramidate),and adenylated DNA in which AMP is covalently attached to the5' terminus of a DNA single-strand break (SSB) or DSB (1, 16,23, 25). To date, aprataxin activity is greatest on AMP-DNA,suggesting that this may be the physiological substrate of thisenzyme.

In vitro, DNA strand breaks with 5'-AMP termini can arise frompremature DNA ligase activity. DNA ligases adenylate 5' terminiat DNA breaks to enable nucleophilic attack of the resultingpyrophosphate bonds by 3'-hydroxyl termini, thereby resealingthe breaks. However, DNA adenylation by DNA ligases can occurprematurely, before a 3'-hydroxyl terminus is available. Aprataxinreverses these premature DNA adenylation events, in vitro atleast, effectively "resetting" the DNA ligation reaction tothe beginning (1). Whether or not 5'-AMP arises in DNA in vivoor is a physiological substrate of aprataxin, however, is unknown.Moreover, attempts to measure DNA strand break repair ratesin vivo are conflicting and have failed to identify a consistentdefect in DNA SSB repair (SSBR) or DSB repair (DSBR) in AOA1cells (14, 15, 20). It is thus not clear whether or not defectsin DNA strand break repair can account for this neurodegenerativedisease.

Here we have resolved the discrepancy between the requirementsfor aprataxin in vitro and in vivo by identifying the stageat which SSBR reactions fail in vitro and by carefully analyzingchromosomal SSBR rates in vivo. We show that short-patch SSBRreactions are defective in AOA1 cell extracts at the final stepof DNA ligation, resulting in the accumulation of adenylatedDNA nicks, and that this defect can be rescued in AOA1 extractsindependently of aprataxin by addition of recombinant DNA ligase.We also find that treatment with aphidicolin, an inhibitor ofDNA polymerase ${delta}$ (Pol ${delta}$ ) and Pol ${varepsilon}$ , unveils a measurable defectin chromosomal SSBR in Aptx^–^/^– primary neural astrocytes,suggesting that the adenylated nicks that arise from the short-patchrepair defect can be channeled into long-patch repair in vivo.These data demonstrate that aprataxin participates in chromosomalSSBR and suggest that this process arrests in AOA1, at oxidativeSSBs, due to insufficient levels of nonadenylated DNA ligase.

MATERIALS AND METHODS

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MATERIALS AND METHODS

Preparation of adenylated DNA substrates. Oligonucleotide duplexes containing an SSB with a 5'-AMP terminusand either a 1-bp gap with a 3'-phosphate terminus or a nickwith a 3'-hydroxyl terminus were prepared as follows. A 25-mer(5'-GACATACTAACTTGAGCGAAACGGT) was labeled by phosphorylationwith T4 PNK and [ ${gamma}$ -³²P]ATP and was annealed with a 43-mer (5'-CCGTTTCGCTCAAGTTAGTATGTCAAAGCAGGCTTCAACGGAT)and a 17-mer with a 3'-phosphate terminus (17-mer-P) (5'-TCCGTTGAAGCCTGCTT-P).The labeled 25-mer in this duplex was then either adenylatedat the 5' terminus by incubation with 1 U T4 DNA ligase at 30°Cfor 1 h in ligation buffer (50 mM Tris-HCl [pH 7.5], 10 mM MgCl₂,5 mM dithiothreitol [DTT], 25 µg/µl bovine serumalbumin, 1 mM ATP) or mock adenylated in the absence of T4 DNAligase. The labeled adenylated 25-mer was then separated fromthe labeled nonadenylated 25-mer (and from the 17-mer and 43-mer)on a 15% denaturing polyacrylamide gel electrophoresis (PAGE)gel, excised, and eluted from the crushed gel in elution buffer(0.5 M ammonium acetate, 10 mM magnesium acetate, 1 mM EDTA[pH 8.0]) overnight at room temperature. The eluted DNA wasthen ethanol precipitated. The labeled mock-adenylated 25-merwas purified in parallel. The labeled adenylated 25-mer wasthen reannealed with the 43-mer and either the 17-mer-P (containinga 3' phosphate) or an 18-mer (5'-TCCGTTGAAGCCTGCTTT) to produceoligonucleotide duplexes harboring an adenylated SSB with eithera 1-bp gap and a 3'-phosphate terminus or a nick with a 3'-hydroxylterminus, respectively. To measure the repair of 3' terminiby PNK or gap filling by Pol β, the 17-mer-P or a 17-meroligonucleotide lacking a 3' phosphate, respectively, was labeledwith T4 PNK (phosphatase dead) and [ ${gamma}$ -³²P]ATP and was annealedto the 25-mer and 43-mer. The substrate was either mock adenylatedor adenylated as described above and was purified on a 15% nativePAGE gel. The final substrate contained a 1-bp gap with a 5'AMP and either a 3' P or a 3' OH.

Purification of recombinant human SSBR proteins. Pol β was expressed in Escherichia coli and purified byanion and cation exchange as previously described (29), usinga 1.6-ml Poros column on a Biocad Sprint chromatography system(Applied Biosystems, United Kingdom). His-tagged PNK and His-taggedDNA ligase III ${alpha}$ (Lig3 ${alpha}$ ) were expressed in the E. coli strain BL21(DE3)for 90 min at 20°C following addition of 1 mM isopropyl-β-D-thiogalactopyranoside(IPTG). PNK was purified by cation-exchange chromatography followedby immobilized metal chelate affinity chromatography (IMAC)as previously described (30). Lig3 ${alpha}$ was purified by IMAC as describedpreviously (7), followed by cation exchange as described previouslyfor PNK. His-tagged aprataxin was expressed from pB352 (8) inBL21(DE3) by addition of 1 mM IPTG and incubation at 30°Cfor 3 h. Aprataxin was purified by IMAC followed by cation exchangeas described above for PNK and Lig3 ${alpha}$ .

Preparation of human lymphoblastoid cell extracts. Total-cell extracts were prepared from 5 x 10⁶ ConR2 (wild type[WT]) or Ap5 (AOA1) lymphoblastoid cells or from Aptx^+/+ andAptx^–^/^– primary quiescent mouse astrocytes by lysisin 0.2 ml 20 mM Tris-HCl (pH 7.5), 10 mM EDTA, 1 mM EGTA, 100mM NaCl, 1% Triton X-100, and 1/100 dilution of protease inhibitorcocktail (Sigma). The extracts were clarified by centrifugation,quantified with a Bio-Rad DC protein assay kit using bovineserum albumin as a standard, and then aliquoted and snap-frozen.

In vitro repair of adenylated SSB substrates by recombinant proteins. For reactions employing recombinant human proteins, a 25 nMconcentration of the indicated ³²P-labeled substrate was incubatedwith the indicated concentrations of recombinant protein for1 h at 30°C in 25 mM HEPES (pH. 8.0), 130 mM KCl, 1 mM DTT,10 mM MgCl₂, 100 µM deoxynucleoside triphosphates (dNTPs),and 1 mM ATP unless otherwise indicated. Reactions were stoppedby addition of 1/3 volume of formamide gel loading buffer, andreaction products were fractionated on 15% denaturing PAGE gelsand analyzed by a phosphorimager.

For reactions employing cell extracts, 5 µg of extractfrom WT lymphoblastoid cells (ConR2) or AOA1 lymphoblastoidcells (Ap5) or from Aptx^+/+ and Aptx^–^/^– primaryquiescent mouse astrocytes was incubated with a 100 nM concentrationof the indicated ³²P-labeled substrate for 1 h at 30°C in25 mM HEPES (pH 8.0), 130 mM KCl, 1 mM DTT, and, unless otherwiseindicated, 10 mM MgCl₂, 100 µM dNTPs, and 1 mM ATP. A1,000-fold excess of a competitor oligonucleotide with an unrelatedsequence and a 5' phosphate (5'-P-TCTGCTAGCATCGATCCATG-3') wasadded to reduce degradation of the labeled substrate by nonspecificnucleases. Reactions were stopped and products analyzed as describedabove.

Cell culture. (i) Human cells. 1BR3 cells are primary human fibroblasts, and ConR and ConR2cells are lymphoblastoid cells, all from unrelated normal individuals.fAp1 and fAp4 cells are AOA1 primary fibroblasts, and Ap3 andAp5 cells are AOA1 lymphoblasts. ConR, Con R2, fAp1, fAp4, Ap3,and Ap5 cells were kindly provided by Malcolm Taylor and, exceptfor Ap5 and ConR2, have been described previously (8). Ap1,Ap3, and Ap4 cells harbor the homozygous APTX mutation W279X,which results in little or no aprataxin protein or activity(1, 8), and Ap5 cells harbor a genomic deletion of APTX (M.Taylor, unpublished data). Cells were cultured as describedpreviously (8).

(ii) Primary mouse astrocytes. Aptx^–^/^– mice have been described previously (1).The generation and characterization of nestin-Cre conditionalXrcc1^–^/^– mice will be described elsewhere. All animalswere housed in individually ventilated cabinets and were maintainedin accordance with the guidelines of the institutional animalcare and ethical committee at the University of Sussex. Mouseastrocytes were prepared from postnatal day 3 (P3) to P4 brains.Cortices were dissociated by passage through a 5-ml pipette,and cells were resuspended in Dulbecco's modified Eagle's mediumand Ham's F-12 nutrient mixture (1:1; Gibco-BRL) supplementedwith 10% fetal bovine serum, 1x Glutamax, 100 U/ml penicillin,100 µg/ml streptomycin, and 20 ng/ml epidermal growthfactor (Sigma). Primary astrocytes were established in PrimeriaT-25 tissue culture flasks (Falcon) at 37°C in a humidifiedoxygen-regulated (9%) incubator. The culture medium was changedafter 3 days, and astrocyte monolayers reached confluence 3days later. The purity of the astrocyte cultures was confirmedby immunofluorescence using an anti-GFAP antibody (Sigma).

Alkaline comet assays. Cells ( $~$ 3 x 10⁵/sample) were incubated with 75 µM (mouseastrocytes), 50 µM (human lymphoblastoid cells), or 75µM (primary human fibroblasts) H₂O₂ for 10 min on iceor with the indicated doses of methyl methanesulfonate (MMS)for 10 min at 37°C. Where indicated, cells were then incubatedin complete medium for the indicated repair periods at 37°C.To inhibit long-patch DNA polymerases, cells were incubatedwith 50 µM aphidicolin (Sigma) in complete medium for30 min at 37°C. Cells were then either mock treated or treatedwith H₂O₂ or MMS as described above in the continued presenceor absence of aphidicolin, as appropriate. Chromosomal DNA strandbreaks were then measured using alkaline comet assays as previouslydescribed (5). Statistical analyses were performed using SPSSsoftware.

RESULTS

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RESULTS

Aprataxin interacts with the SSBR scaffold protein XRCC1, raisingthe possibility that a defect in chromosomal SSBR underliesthe neuropathology of this disease. However, evidence for adefect in SSBR in aprataxin-defective AOA1 cells is conflicting(14, 15, 20). To resolve this issue, we employed alkaline cometassays to compare chromosomal SSBR rates in a variety of differentaprataxin-defective cell types. It should be noted that whilealkaline comet assays measure both SSBs and DSBs, these assaysprimarily measure SSBs following short periods of treatmentwith H₂O₂ or MMS, because these agents induce several ordersof magnitude more SSBs than DSBs (4, 18). In contrast to thefindings of a previous report (15), we failed to observe a significantdifference in chromosomal SSBR rates between either lymphoblastoidcells (Fig. 1A) or primary fibroblasts (Fig. 1B) from AOA1 patientsand those from normal individuals following H₂O₂-induced oxidativestress. Because individual genetic variability might mask differencesin SSBR rates, we also compared chromosomal SSBR in quiescentprimary astrocytes from Aptx^–^/^– mice and isogenicAptx^+/+ littermate controls. Astrocytes were chosen becausethey are neural in origin and thus better reflect the type ofcells affected in AOA1. However, SSBR rates were similar inAptx^+/+ and Aptx^–^/^– astrocytes following treatmentwith H₂O₂ (Fig. 1C). Aptx^+/+ and Aptx^–^/^– astrocytesalso accumulated SSBs at similar rates during incubation withthe alkyating agent MMS, suggesting that the rate of SSB rejoiningduring DNA base excision repair is also normal in Aptx^–^/^–cells (Fig. 1D). In contrast, astrocytes lacking the core SSBRfactor Xrcc1 exhibited greatly reduced SSBR rates followingtreatment with either H₂O₂ or MMS (Fig. 1C and D). It shouldbe noted that we also observed normal SSBR kinetics in Aptx^–^/^–postmitotic cerebellar granule neurons (data not shown). Weconclude from these experiments that AOA1 and other aprataxin-defectivecells lack a measurable defect in the global rate of chromosomalSSBR.

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FIG. 1. Normal rates of chromosomal SSBR in cells lacking aprataxin. (A) AOA1 lymphoblastoid cells were incubated in the absence (–) or presence (+) of 50 µM H₂O₂ (15 min on ice), followed by incubation in a drug-free medium for the indicated repair period at 37°C. Chromosomal DNA strand breaks were then measured by alkaline comet assays. (B) AOA1 primary fibroblasts were treated in the absence (–) or presence (+) of 75 µM H₂O₂ (15 min on ice) and processed as described for panel A. Insets in panels A and B contain the same data as in the main panels but plotted as percent damage remaining. (C) WT, Aptx^–^/^–, and Xrcc1^–^/^– primary quiescent astrocytes were incubated in the absence (–) or presence (+) of 75 µM H₂O₂ (10 min on ice), followed by incubation in a drug-free medium for the indicated repair period at 37°C. Chromosomal DNA strand breaks were then measured by alkaline comet assays. (D) WT, Aptx^–^/^–, and Xrcc1^–^/^– primary quiescent astrocytes were incubated in the absence (–) or presence of the indicated concentration of MMS (10 min at 37°C). Chromosomal DNA strand breaks were then measured by alkaline comet assays.

In contrast to the findings of cellular SSBR assays, proteinextracts from Aptx^–^/^– astrocytes and Aptx^–chicken DT40 cells are unable to support short-patch repairof adenylated oxidative SSBs in vitro (1). To resolve this discrepancy,we examined whether this was also true in AOA1 lymphoblastoidcell extracts. To measure short-patch SSBR, we employed an oligonucleotideduplex harboring a 1-bp gap with 3'-phosphate termini, a substratethat mimics one of the commonest types of oxidative SSB arisingin cells (Fig. 2A, top). The SSB also possesses a 5' AMP andis therefore a substrate for aprataxin. In agreement with previousexperiments with neural extracts (1), WT extracts efficientlyremoved AMP from 5' termini and repaired the SSBs, as indicatedby the respective appearance of the ³²P-labeled 25-mer and the³²P-labeled 43-mer (Fig. 2A, lanes 6 to 8). In contrast, AOA1extracts did not (Fig. 2A, lanes 3 to 5). Importantly, SSBRwas proficient in AOA1 extracts if the initial SSB lacked 5'AMP (Fig. 2B). A number of truncated oligonucleotide fragmentswere generated by nonspecific nucleolytic activity in theseexperiments, which represented degradation of the 3' terminusof the ³²P-labeled 25-mer. However, this activity did not accountfor the short-patch repair defect in AOA1 cell extracts, whichwas fully complemented by the addition of recombinant aprataxin(Fig. 2A, lanes 9 to 11). The appearance of ligated productin these experiments was dependent on the presence of dNTPs,confirming that these experiments measured gap repair ratherthan ligation across the 1-bp gap (data not shown).

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FIG. 2. Aprataxin-dependent short-patch SSBR of 5'-AMP SSBs in AOA1 lymphoblastoid extracts. (A) Defective short-patch SSBR in AOA1 extracts and its complementation by recombinant aprataxin. (Top) Cartoon of the oligonucleotide duplex employed for these experiments, containing a 1-bp gap, a 3'-phosphate terminus, and a 5'-AMP terminus. The 5' phosphate to which AMP is covalently linked is labeled with ³²P. The position of this label restricts the assay to measurements of short-patch repair events only. Nucleotide lengths are shown. (Bottom) Portions (0.1 µg, 1.0 µg, or 5.0 µg) of either WT (ConR2) or AOA1 (Ap5) cell extracts were incubated for 60 min at 30°C with a ³²P-labeled 5'-AMP SSB substrate (25 nM) in the absence (left) or presence (right) of recombinant human aprataxin (APTX) (100 nM). Reaction products were fractionated and detected as described in Materials and Methods. The ³²P-labeled 25-mer containing (AMP-³²P-25) or lacking (³²P-25) 5' AMP was fractionated in parallel for size markers (Mks). The position of the repaired ³²P-labeled 43-mer is also indicated. Asterisks indicate nonspecific nucleolytic products. (B) Normal short-patch repair of SSBs lacking 5' AMP in AOA1 cell extracts. (Top) Cartoon of the oligonucleotide duplex employed for these experiments, containing a 1-bp gap, a 3'-phosphate terminus, and a normal ³²P-labeled 5'-phosphate terminus. WT (ConR2) or AOA1 (Ap5) cell extracts (5 µg) were incubated for 60 min at 30°C with a ³²P-labeled SSB substrate lacking 5' AMP (100 nM). Reaction products were fractionated and detected as described in Materials and Methods.

The predicted pathway for short-patch repair of SSBs harboring5' AMP in WT cells is depicted in Fig. 3A. It was consideredlikely that this pathway arrests in AOA1 extracts at the verybeginning, prior to 3'-DNA end processing by PNK and/or DNAgap filling by Pol β, because the presence of AMP at the5' terminus might occlude access to the 3' terminus. Surprisingly,however, the 3'-phosphatase activity of PNK was similar irrespectiveof whether the SSB possessed 5' AMP or not, under conditionsin which PNK was limiting (Fig. 3B). Similar results were observedfor DNA gap filling by Pol β, with similar amounts of the³²P-labeled 17-mer converted into a ³²P-labeled 18-mer irrespectiveof the presence or absence of 5' AMP (Fig. 3C). These experimentssuggested that neither PNK nor Pol β activity is affectedby the presence of 5' AMP at these time points, and thus short-patchSSBR might fail in AOA1 extracts at the final step of DNA ligation,resulting in the accumulation of adenylated DNA nicks (Fig.3D).

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FIG. 3. Removal of 5' AMP by aprataxin is not required for end processing by PNK or gap filling by Pol β. (A) Cartoon of aprataxin-dependent short-patch repair of adenylated SSBs in WT cells. (B) 5' AMP does not affect processing of 3'-phosphate termini by PNK. An SSB substrate (25 nM) lacking or containing 5' AMP as indicated (top) was incubated either with 25 nM, 50 nM, 125 nM, or 250 nM recombinant human PNK or without PNK (–) for 1 h at 30°C. Reaction products were fractionated by denaturing PAGE and detected by phosphorimaging. Note that the 5' terminus of the 17-mer is labeled with ³²P in these experiments to allow detection of 3' end processing. The position of the 17-mer harboring 3' phosphate (17-P) or 3' hydroxyl (3'-OH) is indicated. (C) 5' AMP does not affect gap filling by Pol β. An SSB substrate (25 nM) lacking or containing 5' AMP as indicated (top) was incubated either with 5 nM, 15 nM, 30 nM, or 100 nM purified recombinant human Pol β or without Pol β (–) for 1 h at 30°C. Reaction products were fractionated by denaturing PAGE and detected by phosphorimaging. The positions of the 17-mer and 18-mer are indicated as markers. (D) Cartoon depicting APTX-independent repair of adenylated SSBs in AOA1. Note the hypothetical blockage of this process at the final step of DNA ligation.

To confirm this hypothesis, we compared WT and AOA1 extractsfor their abilities to ligate adenylated nicks. Indeed, whereasadenylated nicks were efficiently ligated by extracts from WTcells, they remained largely unligated in reaction mixturescontaining AOA1 cell extracts (Fig. 4A). The finding that short-patchrepair in AOA1 arrests during DNA ligation is surprising, becauseadenylated nicks are normal intermediates of DNA ligation andare normally rapidly resealed by nonadenylated DNA ligase (11).Normally, the nonadenylated DNA ligase required for this purposeis created during, and tightly coupled with, adenylation ofthe 5' terminus of the break by an adenylated DNA ligase (Fig.4B). However, in the absence of aprataxin, DNA nicks may accumulatein a preadenylated state and therefore require preexisting poolsof nonadenylated DNA ligase. While both nonadenylated and adenylatedDNA ligases exist in cells, the former may be very limited becausethe readenylation of DNA ligases by cellular ATP is very rapid.Consequently, we reasoned that the DNA ligation defect in AOA1may reflect insufficient cellular levels of nonadenylated DNAligase. To test this hypothesis, we examined the impact of supplementingshort-patch SSBR reaction mixtures in AOA1 cell extracts andAptx^–^/^– mouse neural astrocyte extracts with recombinantDNA ligase. Strikingly, addition of T4 ligase restored short-patchSSBR efficiency in both AOA1 cell extracts and Aptx^–^/^–neural cell extracts to a level similar to that observed inWT extracts (Fig. 4C and D, compare lanes 6 and 10). Importantly,complementation was more efficient in the absence of ATP thanin its presence, supporting the notion that it was the nonadenylatedsubfraction of T4 ligase that was responsible for complementation(Fig. 4C and D, compare lanes 8 and 10). Similar results wereobserved for AOA1 cell extracts if T4 ligase was replaced withhuman DNA ligase 3 ${alpha}$ , albeit to a lesser extent (Fig. 5A).

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FIG. 4. Short-patch SSBR fails in AOA1 due to insufficient levels of nonadenylated DNA ligase. (A) AOA1 cell extracts cannot efficiently ligate adenylated DNA nicks. Total WT (ConR2) or AOA1 (Ap5) lymphoblastoid cell extracts (6.25 µg) were incubated with a ³²P-labeled adenylated nicked substrate (25 nM) (top) for the indicated times at 30°C. Reaction products were fractionated by denaturing PAGE and detected by phosphorimaging. A ³²P-labeled 25-mer containing 5' AMP (AMP-25) and one lacking 5' AMP were fractionated for size markers (Mks). The position of the 43-mer ligated product is indicated. (B) Cartoon depicting ligation of a nonadenylated DNA nick by DNA ligase. (i) An adenylated DNA ligase molecule transfers AMP to the 5'-phosphate terminus of a DNA nick, resulting in an adenylated nick and a nonadenylated ligase molecule. (ii) The nonadenylated DNA ligase molecule rapidly catalyzes a nucleophilic attack of the pyrophosphate bond linking AMP to DNA, resulting in nick ligation and the release of AMP. The nonadenylated DNA ligase molecule is readenylated (dashed arrow) in readiness for the next ligation event. (C) Complementation of the SSBR defect in AOA1 lymphoblastoid extracts by recombinant T4 DNA ligase. Total WT (ConR2) or AOA1 (Ap5) lymphoblastoid cell extracts (5 µg) were incubated with a ³²P-labeled 5'-AMP SSB substrate (25 nM) for 1 h at 30°C in the presence or absence of 1 mM ATP and/or 2 U of T4 DNA ligase, as indicated. Reaction products were fractionated by denaturing PAGE and detected by phosphorimaging. The positions of the ³²P-labeled 43-mer reaction product and the ³²P-labeled 25-mer containing or lacking 5' AMP are indicated. M'rkers, markers. (D) Complementation of the SSBR defect in Aptx^–^/^– primary astrocyte extracts by recombinant T4 DNA ligase. Aptx^+/+ (+/+) or Aptx^–/– (–/–) mouse astrocyte extracts (5 µg) were incubated with a ³²P-labeled 5'-AMP SSB substrate (25 nM) for 1 h at 30°C in the presence or absence of 1 mM ATP and/or 2 U of T4 DNA ligase, as indicated. Reaction products were fractionated by denaturing PAGE and detected by phosphorimaging. The positions of the ³²P-labeled 43-mer reaction product and the ³²P-labeled 25-mer containing or lacking 5' AMP are indicated.

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FIG. 5. Complementation of the SSBR defect in AOA1 lymphoblastoid cell extracts by recombinant human Lig3 ${alpha}$ and reconstitution of aprataxin-independent SSBR with recombinant human proteins. (A) Complementation of the SSBR defect in AOA1 lymphoblastoid cell extracts by recombinant DNA ligase III ${alpha}$ (Lig3 ${alpha}$ ). Total WT or AOA1 lymphoblastoid cell extracts (5 µg) were incubated with a ³²P-labeled 5'-AMP SSB (100 nM) substrate for 1 h at 30°C in the presence or absence of 1 mM ATP and/or 8 nM, 24 nM, or 72 nM Lig3 ${alpha}$ , as indicated. (B) Reconstitution of aprataxin-independent SSBR with recombinant human proteins. A 5'-AMP SSB substrate (60 nM) was incubated with 250 nM recombinant PNK, 100 nM Pol β, and 80 nM Lig3 ${alpha}$ in the presence or absence of 100 nM aprataxin (APTX) and 1 mM ATP, as indicated, for 1 h at 30°C. Reaction products were fractionated by denaturing PAGE and detected by phosphorimager.

The data described above suggest that short-patch repair ofsome adenylated SSBs can occur independently of aprataxin ifsufficient nonadenylated DNA ligase is available. To confirmthis idea, we attempted to reconstitute this aprataxin-independentSSBR pathway using recombinant proteins. As expected, the repairof adenylated gaps by PNK, Pol β, and Lig3 ${alpha}$ was dependenton aprataxin in the presence of ATP, conditions under whichLig3 ${alpha}$ is largely adenylated (Fig. 5B). However, in the absenceof ATP, short-patch repair of 5'-AMP SSBs occurred independentlyof aprataxin. Taken together, these experiments indicate thatshort-patch repair arrests in AOA1 cell extracts at the finalstep of DNA ligation, due to insufficient levels of nonadenylatedDNA ligase.

Importantly, the finding that short-patch repair failed duringDNA ligation provides a possible explanation for the absenceof a measurable defect in chromosomal SSBR in AOA1, followingoxidative stress. This is because adenylated DNA nicks mightbe channeled into long-patch SSBR reactions, during which theadenylated 5' terminus is displaced by extended DNA gap fillingand then clipped off nucleolytically, avoiding the requirementfor either aprataxin or preexisting pools of nonadenylated DNAligase. While our in vitro assay was not capable of measuringlong-patch repair reactions, this process might operate efficientlyat adenylated nicks within a chromosomal context. To examinethis possibility, we compared chromosomal SSBR rates in WT andAptx^–^/^– quiescent mouse neural astrocytes in thepresence and absence of aphidicolin, an inhibitor of the DNApolymerases Pol ${delta}$ and Pol ${varepsilon}$ , which are implicated in long-patchrepair reactions (10, 13, 22). Strikingly, whereas aphidicolindid not measurably reduce SSBR rates in WT astrocytes followingH₂O₂ treatment, it significantly slowed SSBR in Aptx^–^/^–astrocytes (Fig. 6A). Aphidicolin also selectively slowed short-patchbase excision repair in AOA1 cells, as indicated by the accumulationof higher steady-state levels of chromosomal DNA strand breaksin Aptx^–^/^– astrocytes than in WT astrocytes duringshort incubations with the DNA-alkylating agent MMS (Fig. 6B).The fact that SSBR in Aptx^–^/^– cells was slowed ratherthan prevented by aphidicolin most likely reflects the factthat only a subset of H₂O₂- and MMS-induced SSBs possess adenylated5' termini. Nevertheless, the presence of a measurable defectin chromosomal SSBR in Aptx^–^/^– cells indicates thata significant fraction of endogenous SSBs arising from oxidativestress and DNA base damage are substrates for aprataxin.

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FIG. 6. Defective short-patch SSBR in quiescent primary Aptx^–^/^– mouse neural cells. (A) Quiescent WT and Aptx^–^/^– mouse astrocytes were either left untreated (–) or treated with 75 µM H₂O₂ for 10 min on ice (+) and, where indicated, then incubated in drug-free medium for 30 or 60 min. Where indicated (+Aph), cells were preincubated with 50 µM aphidicolin for 30 min at 37°C, and repair was conducted in the continued presence of aphidicolin. Chromosomal DNA strand breaks were then quantified by alkaline comet assays. Each bar represents the average mean tail moment from three independent experiments (error bars, ±1 standard deviation). Asterisks indicate statistically significant differences (*, P $≤$ 0.05; **, P $≤$ 0.01). (B) Quiescent WT and Aptx^–/– mouse astrocytes were either left untreated (–) or treated with 25, 50, or 100 µM MMS for 10 min at 37°C with (+Aph) or without preincubation with 50 µM aphidicolin. Chromosomal DNA strand breaks were then quantified by alkaline comet assays. Each bar represents the average mean tail moment from three independent experiments (error bars, ±1 standard deviation). Asterisks indicate statistically significant differences (*, P $≤$ 0.05; **, P $≤$ 0.01).

In summary, we demonstrate here that aprataxin is required forSSBR in vivo and suggest that short-patch SSBR is defectivein AOA1 cells, at oxidative SSBs, due to insufficient levelsof nonadenylated DNA ligase.

DISCUSSION

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DISCUSSION

AOA1 is one of the commonest recessive hereditary spinocerebellarataxias identified to date. This disease results from mutationsin aprataxin, a component of the DNA strand break repair machinerythat removes AMP from 5' termini during short-patch SSBR reactionsin vitro (1, 9, 19). However, whether or not aprataxin is requiredfor chromosomal DNA strand break repair in vivo is unclear.This is because the occurrence of DNA strand breaks with 5'AMP has not yet been demonstrated. Moreover, attempts to detecta chromosomal DNA repair defect in AOA1 cells have proved conflictingand unclear (14, 15, 20). To resolve the latter issue, we carefullymeasured chromosomal SSBR rates in a variety of aprataxin-defectivecell lines, including genetically matched WT and Aptx^–^/^–quiescent neural cells. These experiments revealed that theoverall rate of SSBR is normal in aprataxin-defective cells.Notably, we also failed to detect reduced rates of DSBR in AOA1(unpublished observations).

To resolve the discrepancy between the requirement for aprataxinfor SSBR in vitro versus that in vivo, we identified the stageat which short-patch SSBR fails in AOA1 in vitro. Notably, 3'-DNAend processing and DNA gap filling occurred normally duringSSBR in the absence of aprataxin, despite the persistence ofAMP on the 5' terminus. However, SSBR reactions subsequentlystalled at the final step of DNA ligation, resulting in theaccumulation of adenylated DNA nicks. This was surprising, becauseadenylated DNA nicks are normal, indeed prerequisite, intermediatesof DNA ligation reactions, requiring only nonadenylated DNAligase to reseal the breaks. We therefore reasoned that DNAligation might fail in AOA1 cell extracts because of insufficientlevels of nonadenylated DNA ligase. This would be consistentwith the notion that while DNA ligases exist in both adenylatedand nonadenylated states, the former predominates in cells becauseof the cellular ATP concentration. This would not pose a problemin WT cells, in which aprataxin activity ensures that DNA nicksarising during SSBR are not preadenylated and thus are substratesfor adenylated DNA ligase. However, in AOA1 cells, DNA nickscan arise in a preadenylated state during SSBR which thus requirenonadenylated DNA ligase. In short, we propose that while allcells possess low levels of nonadenylated ligase, due to therapid adenylation of free ligase molecules by cellular ATP,only in aprataxin-defective cells do preadenylated nicks ariseat a level that exceeds the availability of nonadenylated ligase.

Confirmation that short-patch SSBR fails in AOA1 due to insufficientlevels of nonadenylated DNA ligase emerged from our findingthat addition of recombinant T4 DNA ligase or human Lig3 ${alpha}$ restoredshort-patch SSBR in AOA1 extracts and Aptx^–^/^– quiescentastrocyte extracts in the absence of aprataxin. Importantly,complementation was more efficient if ATP was omitted from thereaction mixtures, supporting the notion that the complementingfactor was nonadenylated DNA ligase. This may also explain theapparent difference between the abilities of T4 DNA ligase andLig3 ${alpha}$ to complement the defect (compare Fig. 4C and 5A), sinceit is likely that the relative amounts of nonadenylated ligasepresent in the two DNA ligase preparations were different.

The finding that adenylated nicks accumulate during short-patchSSBR in AOA1 provides a possible explanation for the normalrate of chromosomal SSBR observed in this disease. This is becauseadenylated nicks can be channeled into long-patch SSBR. In thispathway, damaged 5' termini are displaced as a single-strandedflap during gap filling from the 3' terminus and cleaved offby Flap endonuclease 1 (FEN1) (reviewed in reference 12). Thisprocess would not be detected by the short-patch repair assaysemployed in the current work, because oligonucleotide duplexesof the type employed here are not good substrates for long-patchrepair reactions and because cleavage of the single-strand flapwould remove the ³²P label in our substrates. However, to determinewhether long-patch repair might compensate for the loss of short-patchrepair in aprataxin-defective cells, we exploited the observationthat long-patch SSBR employs the aphidicolin-sensitive DNA polymerasesPol ${delta}$ and/or Pol ${varepsilon}$ (10, 13, 22). Because inhibition of Pol ${delta}$ and/orPol ${varepsilon}$ also prevents DNA replication during S phase and can thusimpact DNA metabolism independently of long-patch SSBR, we employedquiescent primary astrocytes for these experiments. Strikingly,whereas preincubation with aphidicolin did not affect SSBR ratesin WT cells, it revealed a significant chromosomal SSBR defectin Aptx^–^/^– primary quiescent astrocytes followingtreatment with either H₂O₂ or MMS. SSBR was slowed rather thanprevented by aphidicolin, perhaps reflecting the fact that onlya subset of DNA strand breaks induced by these agents possess5'-AMP termini. Alternatively, it is possible that Aptx^–^/^–quiescent astrocytes possess additional, partially overlappingSSBR pathways. Nevertheless, these data demonstrate, for thefirst time, the involvement of aprataxin in chromosomal SSBRin vivo.

It remains to be determined whether long-patch repair can alsocompensate for defective short-patch repair in AOA1 cells, asappears to be the case in Aptx^–^/^– mouse neural cells.However, if this is the case, why do aprataxin mutations resultin disease? One possibility is that a subset of SSBs arise atwhich long-patch repair cannot operate. For example, it is possiblethat aprataxin is also required to repair specific types ofdamaged 3' termini (26). Long-patch repair would be unable tooperate at such breaks, because no 3'-hydroxyl primer terminusis available for DNA gap filling. Alternatively, since aprataxinis associated with the DSBR machinery (8), it is possible thatunrepaired DSBs might account for AOA1. It should be noted,however, that we have so far failed to detect a DSBR defectin AOA1 or Aptx^–^/^– cells (unpublished observations).Finally, it is possible that long-patch repair is not operativeor is attenuated in the specific cell types that are affectedin AOA1. For example, a number of replication-associated proteins,including several of those implicated in long-patch repair,are downregulated in certain differentiated cell types (21).Thus, it will now be of interest to expand the experiments describedin this study to other cell types, including those neural celltypes most likely affected in AOA1.

ACKNOWLEDGMENTS

We thank LiMei Ju and Poorvi Patel for technical assistanceand Malcolm Taylor for the provision of AOA1 lymphoblastoidcells.

This work was funded by MRC, BBSRC, and European Community (IntegratedProject DNA repair [LSHG-CT-2005-512113]) grants to K.W.C. P.J.M.is funded by grants from the NIH and ALSAC of SJCRH. S.F.E.-K.is funded by the Wellcome Trust (grant 085284).

FOOTNOTES

* Corresponding author. Mailing address: Genome Damage and Stability Centre, University of Sussex, Science Park Road, Falmer, Brighton BN1 9RQ, United Kingdom. Phone: 44 (0) 1273 877519. Fax: 44 (0) 1273 678121. E-mail: k.w.caldecott{at}sussex.ac.uk

Published ahead of print on 22 December 2008.

J.J.R. and S.F.E.-K. contributed equally to this work.

REFERENCES

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