Terminally Differentiated Human Neurons Repair Transcribed Genes but Display Attenuated Global DNA Repair and Modulation of Repair Gene Expression

doi:10.1128/MCB.20.5.1562-1570.2000

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Molecular and Cellular Biology, March 2000, p. 1562-1570, Vol. 20, No. 5
0270-7306/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Terminally Differentiated Human Neurons Repair Transcribed Genes but Display Attenuated Global DNA Repair and Modulation of Repair Gene Expression

Thierry Nouspikel and Philip C. Hanawalt^*

Department of Biological Sciences, Stanford University, Stanford, California 94305-5020

Received 22 September 1999/Returned for modification 22 October 1999/Accepted 22 November 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Repair of UV-induced DNA lesions in terminally differentiated human hNT neurons was compared to that in their repair-proficientprecursor NT2 cells. Global genome repair of (6-4)pyrimidine-pyrimidonephotoproducts was significantly slower in hNT neurons than inthe precursor cells, and repair of cyclobutane pyrimidine dimers(CPDs) was not detected in the hNT neurons. This deficiency inglobal genome repair did not appear to be due to denser chromatinstructure in hNT neurons. By contrast, CPDs were removed efficientlyfrom both strands of transcribed genes in hNT neurons, with thenontranscribed strand being repaired unexpectedly well. Correlatedwith these changes in repair during neuronal differentiation weremodifications in the expression of several repair genes, in particularan up-regulation of the two structure-specific nucleases XPG andXPF/ERCC1. These results have implications for neuronal dysfunctionandaging.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The human genome is the target of DNA damage from multiple sources, both environmental, such as radiation or chemicals, andintracellular, such as the reactive products of cellular oxidativemetabolism. DNA lesions are a threat to the organism for severalreasons. First, they may arrest transcription, thereby preventingappropriate gene expression and potentially disturbing the cellularmetabolism. Second, lesions encountered during DNA replicationcan result in the introduction of mutations, the accumulationof which may lead to cancer. Finally, DNA damage can prevent cellproliferation and kill cells, which can result in various growthand developmental defects (7).

Eucaryotic cells have evolved several systems, including nucleotide excision repair (NER), base excision repair, and mismatchrepair, to repair inappropriate DNA alterations. Some are ableto target transcribed genes specifically and repair them morerapidly than they can repair the global genome (10). Other mechanisms,involving the genes ATM and p53, can arrest the cell cycle untildamage is repaired, and if this does not occur rapidly, they cantrigger apoptosis (4). Finally, cells can tolerate some DNAlesions through translesion DNA synthesis and/orrecombination.

However, cells that have undergone terminal differentiation, such as myotubes, adipocytes, or neurons, represent a specialsituation. (i) Since they no longer divide, apoptosis would resultin an uncompensated cell loss for the organism, which would probablybe a harmful situation. One would then expect that such cellswould rely heavily on their repair systems to deal with lesionsin their genomes. (ii) Recombinational repair most probably doesnot occur in cells that remain in interphase. (iii) Since thesecells do not replicate their DNA, the risk of accumulating carcinogenicmutations is extremely low, as documented by the rarity of neuronalcancer in adults. Neurons and other postmitotic cells could thus,in principle, afford to repair only the portion of their genomethat is really needed for their specialized functions, i.e., transcribedgenes.

For these reasons, neurons constitute a particularly interesting system in which to study DNA repair, especially in conjunctionwith transcription. However, surprisingly little is known aboutthe repair capabilities of neurons. It has been shown that mouseneuroblastoma cells become extremely UV sensitive after terminaldifferentiation (21) and that human neuroblastoma cells aredeficient in removal of bulky adducts and exhibit low levels ofunscheduled DNA synthesis, an indication of repair activity (15).Preliminary studies in our laboratory with rat pheochromocytomaPC12 cells differentiating into neuron-like cells have indicateda marked decrease in global genome repair but not in the repairof expressed genes (summarized in reference 11).

The present work makes use of the NT2-hNT system, a well-characterized human precursor/neuron cell system. It was undertakento examine in detail the repair phenotype of human neurons andto try to understand how terminal differentiation might modulateDNANER.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Cell culture and treatments. NT2 cells (Stratagene) were grown and differentiated as recommended by the supplier. Due to the poor quality of the commerciallyavailable cells, another batch was obtained directly from PeterAndrews (18). The cells were irradiated with 254-nm UV lightusing a Westinghouse SB-30 germicidal lamp at 1 W/m². They were harvested by trypsinization, and DNA was preparedas described previously (25). In some cases, 6 h before irradiation,the cells were fed medium containing trichostatin A (ICN) dissolvedat 1 mg/ml inethanol.

T4 endo V sensitive-site assay. DNA (200 ng) was digested with 0.07 µl of T4 endonuclease V (endo V) (activity, 2 × 10¹³ nicks/min/µl) (a kind gift from Stephen Lloyd) in TEV buffer(100 mM NaCl, 10 mM Tris [pH 7.5], 10 mM EDTA, 1 mg of bovineserum albumin per ml). The reaction mixture was loaded on 5 to20% sucrose gradients containing 0.1 M NaOH and 10 mM EDTA, andcentrifuged for 2 h at 30,000 rpm at 20°C in an SW-50.1 rotor(Beckman). Fractions (22 to 24 per gradient) were collected fromthe bottom, and 100 µl of each, mixed with 100 µl of 20× SSPE(1× SSPE is 0.18 M NaCl, 10 mM NaH₂PO₄, and 1 mM EDTA [pH 7.7]),was slot blotted under vacuum on a Hybond N+ membrane (Amersham)and fixed for 20 min on 3MM paper (Whatman) soaked in 0.4 N NaOH.A ³²P-labeled DNA probe was prepared from genomic DNA by using a nicktranslation labeling kit (Gibco). The membrane was prehybridizedfor 2 h at 42°C in 6× SSPE-5× Denhardt's solution-0.5% sodiumdodecyl sulfate (SDS)-50% formamide-200 µg of denatured salmonsperm DNA per ml, hybridized overnight with the ³²P-labeled probe at 42°C in 6× SSPE-0.5% SDS-50% formamide-100mg of denatured salmon sperm DNA per ml, and washed for 5 minat 20°C in 2× SSC (1× SSC is 0.15 M NaCl plus 0.015 M sodium citrate)-0.5%SDS, 15 min at 20°C in 2× SSC-0.1% SDS, 30 min at 37°C in 0.1×SSC-0.5% SDS, and 30 min at 65°C in 0.1× SSC-0.5% SDS, and rinsedin 0.1× SSC, and the ³²P was quantified with a Bio-Rad GS-363phosphorimager.

T4 endo V accessibility assay. The T4 endo V accessibility assay was conducted as previously described (29). Briefly, cells were resuspended in a low-saltbuffer (100 mM Tris [pH 8], 100 mM NaCl, 10 mM EDTA, 1 mg of bovineserum albumin per ml) and permeabilized by three cycles of freezing-thawing.Some samples were incubated in high-salt buffer (as above butwith 2 M NaCl) for 15 minutes at room temperature before beingdiluted back to 100 mM NaCl. Samples containing 20,000 cells weredigested for 20 min at 37°C with 0.1 µl of T4 endo V. The cellswere then lysed in a layer of 1 N NaOH at the top of high-saltalkaline sucrose gradients (5 to 20% sucrose in 2 M NaCl-0.3 NNaOH-10 mM EDTA). The gradients were processed and DNA was detectedin the fractions as describedabove.

Antibody assay. Cellular DNA in Tris-EDTA (TE) was denatured by boiling. One volume of 2× SSPE was added, and samples were slot blotted intriplicate on a Hybond N+ membrane, using 60 ng of DNA for theCPD assay and 1 µg of DNA for the (6-4)PPs assay. The DNA wasfixed as above, and the membranes were blocked overnight in phosphate-bufferedsaline (PBS)-0.2% Tween 20 (PBS-T) containing 5% (wt/vol) skimmilk, washed in PBS-T, and incubated for 2 h at room temperaturewith monoclonal antibodies specific for cyclobutane pyrimidinedimer (CPD) or (6-4)pyrimidine-pyrimidone photoproducts [(6-4)PPs](a kind gift from Toshio Mori [22]) diluted 1/2,000 in PBS.The membrane was washed as above and incubated for 1 h at roomtemperature with a peroxidase-labeled anti-mouse monoclonal antibody(Amersham) diluted 1/4,000 in PBS. After extensive washes withPBS-T, the membrane was assayed with an ECL chemiluminescencekit (Amersham). The signal was quantified using a Bio-Rad GS-363phosphorimager.

TCR assay. The transcription-coupled repair (TCR) assay was conducted essentially as described previously (25) except that the DNAcould not be ³H labeled (since neurons do not replicate DNA). The CsCl gradientstep was thus omitted, and after restriction, DNA was ethanolprecipitated with 0.8 M LiCl, resuspended in TE, and subjectedto T4 endo V digestion. The restriction enzymes were KpnI forthe dihydrofolate reductase (DHFR) gene, SphI and HincII for theglucagon gene, EcoRI and BamHI for the NF-L gene, BclI and XhoIfor the CK8 gene, and HindIII for the CK18gene.

Quantitative RT-PCR. RNA was prepared by resuspending trypsinized cells in 8 ml of GT buffer (4 M guanidinium thiocyanate, 0.1 M Tris [pH 7.5],1% $beta$ -mercaptoethanol, 0.5% sodium lauroyl sarcosinate) and passingthe lysate 10 times through a 20-gauge needle. It was then laidon a cushion of 1 ml of 40% (wt/vol) CsCl on top of 3 ml of 5.7M CsCl in TE (pH 7.6) and centrifuged in an SW27 rotor for 22h at 34,000 rpm and 20°C. The RNA pellet was dissolved in TE (pH7.6), extracted with 1 volume of chloroform-butanol (1:1), ethanol(2 volumes) precipitated with 0.3 M sodium acetate (pH 5.2), anddissolved in nuclease-free water. RNA (3 µg) was reverse transcribedwith 50 ng of random hexamers (Gibco) using a Superscript II kit(Gibco). PCR was performed using a touchdown method; 5 min at94°C; then 10 cycles of 15 s at 94°C, 30 s at the calculated annealingtemperature (T_a) plus 10°C, subtracting 1°C at each cycle, and1 min at 72°C; then 18 to 25 cycles of 15 s at 94°C, 30 s at T_a,and 1 min at 72°C; followed by a final 5 min at 72°C. The reactionmixtures were assembled in a volume of 50 µl, using 400 nM eachdATP, dGTP, and dTTP, 120 nM dCTP, 10 µCi of [ $alpha$ -³²P]dCTP (Amersham), 1.5 mM MgCl₂, and 1.25 U of Taq polymerase(Gibco). Three different dilutions of reverse transcription (RT)reaction mixture (up to 1/70 of the RT reaction mixture) wereroutinely used to verify that the band intensity was linearlydependent on the amount of template. The number of cycles andthe respective amounts of primers for target and reference geneswere adjusted in preliminary experiments to avoid saturation andto obtain bands of comparable intensity for both genes. A 5-µlsample of each reaction mixture was run on a 1.8% agarose gel,and the gels were dried and quantified with a Bio-Rad GS-363 phosphorimager.The intensity of each band was normalized to the number of cytidinesin a givenfragment.

Strand-specific RT-PCR. Total cellular RNA was reverse transcribed as above, except that 50-ng portions of oligonucleotides specific for the senseor antisense strand were used instead of random hexamers as primers.In the case of the DHFR gene, RT was detected in the absence ofany primer, probably due to self-priming of the mRNA. To overcomethis problem, RT was first performed for 20 min in the absenceof any primer, with 0.6 µl of the ddA mix from a sequencing kit(Promega), in a volume of 18 µl. Regular deoxynucleoside triphosphates(final concentration, 5 mM) and 50-ng portions of strand-specificprimers were then added, and the reaction was continued as abovefor an additional 40min.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Global genome repair is greatly attenuated upon neuronal differentiation. The system used for our studies consisted of NT2 human neuroteratoma cells, which upon appropriate stimulation differentiateinto neuron-like cells termed hNT neurons (18). This well-characterizedsystem has the advantage that repair can be studied in the identicalgenetic background, with the two cell types differing only bythe fact that the hNT neurons have attained terminal differentiation.We have used it to study the repair of UV-induced DNA damage.Short-wavelength UV radiation induces covalent bonds between adjacentpyrimidines on the same DNA strand. There are two main types ofsuch dimers, depending upon where the bonds form: CPDs and (6-4)PPs.CPDs are induced to a higher level upon irradiation with 254-nmlight (8), but (6-4)PPs are more rapidly repaired (31).

We first evaluated the status of the NER system at the global genome level in the two cell types by measuring the repair ofCPDs. Cells were irradiated with UV light or not irradiated, andtheir DNA was extracted and digested with T4 endo V, an enzymethat nicks the DNA backbone wherever it contains a CPD. The DNAwas then analyzed by sedimentation on alkaline sucrose gradients(Fig. 1). The nicked DNA sedimented more slowly than undamagedDNA did. When NT2 cells were allowed 24 h after irradiation torepair their DNA, the resulting peak shifted back toward the positionof undamaged DNA, indicating that these cells repaired a significantfraction of the CPD lesions induced by UV irradiation. In strikingcontrast, no such shift was observed when the same experimentwas carried out with hNT neurons. Calculations based upon theaverage size of the DNA fragments indicated that the average distancebetween CPDs was 25.6 kbp in NT2 cells immediately after irradiationand increased to 322.3 kbp within 24 h, which means that over90% of the lesions were repaired. By contrast, the average distancebetween CPDs in hNT neurons was 14.7 kbp upon irradiation and17.0 kbp after 24 h, which indicates that only 14% of the CPDswere removed.

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FIG. 1. Global genome repair of CPDs in NT2 precursor cells and hNT neurons. NT2 cells and hNT neurons were either not irradiated (open symbols) or irradiated with 254-nm UV light at 10 J/m² and harvested immediately (solid symbols) or 24 h after irradiation (crossed symbols). Total DNA was digested with T4 endo V, fractionated on alkaline sucrose gradients, slot blotted, and detected with a ³²P-labeled genomic probe. The arrowheads indicate the positions of the molecular size markers: bacteriophage T2 (166 kbp), bacteriophage $lambda$ (48 kbp), and the largest fragment of HindIII-digested phage $lambda$ (23 kbp).

To determine whether the repair of CPDs and (6-4)PPs was equally affected by differentiation, cells were harvested at varioustimes after irradiation with 254-nm UV light, and DNA was blottedon a nylon membrane and probed with monoclonal antibodies specificfor CPDs or (6-4)PPs (22). Figure 2 shows that NT2 cells removedmost of the (6-4)PPs from their DNA within a few hours whereasremoval of CPDs took somewhat longer. This result is consistentwith our previous observations on other cell types (5, 14),in that repair is somewhat underestimated with the anti-CPD antibody,probably due to the relatively weak specificity of this antibody.In this respect, the T4 endo V incision assay is more reliable,although it detects only CPDs. The antibody assay revealed thathNT neurons removed (6-4)PPs much more slowly than did NT2 cellsand did not seem to repair CPDs at all, consistent with the resultspresented in Fig. 1. Experiments in which hNT neurons were allowedlonger times for repair showed that (6-4)PPs were almost completelyremoved within 3 days whereas removal of CPDs was still not detectableby that time (data not shown). Thus, most domains of the genomedid not appear to be totally inaccessible to repair enzymes, eventhough the repair of CPDs was severely attenuated.

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FIG. 2. Global genome repair of CPDs and (6-4)PPs in NT2 and hNT cells. DNA from NT2 cells (circles) and hNT neurons (diamonds) that were irradiated (solid symbols) or not (open symbols) was slot blotted on a nylon membrane and assayed with monoclonal antibodies specific for CPDs or (6-4)PPs. The results are the means of two to four experiments; the error bars indicate standard error of the mean.

Transcribed genes are efficiently repaired in hNT neurons. Human cells generally repair transcribed genes with greater efficiency than the rest of their genome, a process known as TCR.The enhanced repair is confined to the transcribed strand of activegenes, with the nontranscribed strand being only marginally betterrepaired than inactive DNA (10, 28).

To determine whether TCR was impaired in hNT neurons, genomic DNA was isolated from NT2 and hNT cells at various times afterirradiation with UV light. The DNA was sequentially digested withappropriate restriction enzymes and with T4 endo V, run on a denaturinggel, subjected to Southern transfer, and hybridized with riboprobesspecific for the transcribed or nontranscribed strand of the geneof interest. The treatment with T4 endo V resulted in nickingof the restriction fragments that contained at least one CPD.The percentage of intact fragments was determined by quantifyingthe full-size band and comparing it with a lane in which the T4endo V treatment had been omitted. The Poisson expression wasthen used to derive the total number of CPDs present at varioustimes after irradiation and hence the percentage that was repaired(25).

This analysis was performed on five different genes. The DHFR gene is transcribed in both cell lines, although transcriptionis twofold higher in NT2 than in hNT (see Fig. 7). The glucagongene is not expressed in either cell type. The NF-L gene encodesthe large subunit of the neurofilament complex; it is silent inNT2 cells but vigorously induced by differentiation. Both cytokeratingenes CK8 and CK18 are expressed in both cell types and at essentiallysimilarlevels.

Figure 3 summarizes the results of our TCR analyses. It can be seen that although NT2 cells repaired both strands of activegenes efficiently, the transcribed strand was better repairedthan the nontranscribed one. This strand bias is typical of TCRand occurs because although both strands are subject to the globalgenome repair process, transcribed DNA strands are additionallyrepaired by the TCR machinery. This is illustrated by the twogenes that are silent in NT2 cells, glucagon and NF-L, in whichboth strands were repaired with the same efficiency.

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FIG. 3. TCR in NT2 and hNT cells. DNA from UV-irradiated NT2 cells and hNT neurons was prepared at various times after irradiation, digested with restriction enzymes and then with T4 endo V, and subjected to a Southern analysis with riboprobes specific for the transcribed or nontranscribed strand of the gene of interest. Quantification of the fragment resistant to T4 endo V is an indication of the number of CPDs present at that time, from which the percentage of repair can be calculated. DNA from nonirradiated cells is included as a control; the corresponding points are reported on the y axis.

The situation was somewhat different for hNT neurons, which do not exhibit significant repair at the global genome level.As expected, for the silent glucagon gene, both strands were repairedpoorly compared with NT2 cells: only about 25% of the lesionswere eventually removed, which is consistent with the residualrepair we observed at the global genome level (14% in Fig. 1).By contrast, in the four other genes that are transcribed in hNTneurons, the transcribed strand was repaired as well as in NT2cells, indicating that TCR is proficient in these cells. The surprisingfinding was that the nontranscribed strand was also proficientlyrepaired in hNT neurons, at least to the same extent as in NT2cells, and in some cases (i.e., DHFR and NF-L genes) was repairedas well as the transcribed strand. This lack of strand bias shouldnot be mistaken for deficient TCR, however; in such a situation,both strands would be poorly repaired, as was the case for thesilent glucagon gene. We observed the opposite for the expressedgenes: both strands were repaired as efficiently as or even betterthan in NT2 cells. It is difficult to determine whether the gene-to-genevariations shown in Fig. 3 are due to heterogeneity in repairat the gene level or to experimental error, since the limitedavailability of hNT neurons did not allow us to accumulate enoughdata to run statistical tests. The data presented only allow usto conclude that the nontranscribed strand is proficiently repairedin active genes in hNT neurons and thus does not reflect the overallpoor repair at the global genomelevel.

The nontranscribed strand does not become transcribed in hNT neurons. One main concern, in view of our above results, is that there could be another transcription unit, in the opposite direction,downstream from the genes we studied. A tissue-specific activationof that unit in neurons would result in transcription of the previouslynontranscribed strand, which could then account for the unusuallyefficient repair weobserved.

To examine this possibility, we reverse transcribed RNA from NT2 or hNT cells, using primers specific for the DHFR or CK18mRNA or for a putative antisense RNA that could result from thetranscription of the nontranscribed strand in these genes. SemiquantitativePCR was then performed, with primers nested within the one usedfor RT. To our surprise, even in the absence of any primer, theRT yielded a detectable level of cDNA. This could have been dueto secondary structures in the mRNA that would serve as self-primersor to impurities (e.g., oligonucleotides) in the preparation ofreverse transcriptase. The first explanation seems more likely,since this phenomenon was much more marked with the DHFR genethan with the CK18gene.

We were able to partially solve the problem by using a two-step approach. First, RT was performed in the absence of any primer,with a small amount of dideoxy-ATP. This was meant to quicklyterminate the elongation of any nonspecific RT product. Then thedideoxy-ATP was diluted with an excess of normal deoxynucleotides,and RT was continued with the strand-specific primer of interest.Under these conditions, the background signal was reduced to manageablelevels, and we detected no transcription products that could haveoriginated from the nontranscribed strand of either the DHFR orthe CK18 gene (Fig. 4).

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FIG. 4. Search for transcription products from either strand of the DHFR and CK18 genes. Total RNA from NT2 or hNT cells was reverse transcribed with primers specific for the DHFR or CK18 mRNA or for putative antisense RNA generated by transcription of the nontranscribed strand of these genes. As a control, RT reactions were performed with no primer. The resulting cDNA was then measured by semiquantitative PCR.

The defect in global genome repair is not due to a more compact chromatin structure. To determine whether a more compact chromatin structure in hNT neurons could prevent repair enzymes from reaching the lesions,cells were UV irradiated, permeabilized, treated (or not) with2 M NaCl to disrupt chromatin, and then digested with T4 endoV. The cells were then lysed directly at the top of alkaline sucrosegradients containing 2 M NaCl. After centrifugation, DNA was quantifiedin the fractions collected from the gradients. The sedimentationprofiles obtained in this way reflect the number of UV-inducedlesions that were incised by T4 endo V. As expected, the high-salttreatment unmasked a few lesions that were not previously accessibleto the T4 endo V (Fig. 5). However, this unmasking effect wasnot any stronger in hNT neurons than in NT2 cells, indicatingthat chromatin was not more of an obstacle for T4 endo V accessibilityto CPDs in hNT neurons than in the precursor cells.

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FIG. 5. Detection of CPDs by T4 endo V in NT2 and hNT cells. NT2 cells and hNT neurons were either not irradiated (open symbols) or irradiated (solid symbols) with 254-nm UV light at 10 J/m², permeabilized, treated with T4 endo V, and lysed at the top of alkaline sucrose gradients. The DNA in gradient fractions was blotted and assayed with a ³²P-labeled genomic probe. In some cases (crossed symbols), chromatin was disrupted by treating the cells with high salt prior to T4 endo V digestion.

Since it is conceivable that a small enzyme such as T4 endo V would not be impaired by chromatin structures that would bean obstacle for a huge "repairosome," we cross-checked these resultsusing a different approach. We made use of trichostatin A, a specificinhibitor of histone deacetylases, to destabilize chromatin andhopefully make neuronal DNA more accessible for repair enzymes.Preliminary experiments (results not shown) were conducted todetermine the sublethal range of trichostatin A concentrations,and subsequent experiments were performed with trichostatin Aat 25 to 50 µg/ml. In another pilot experiment, cells were treatedwith trichostatin A before being UV irradiated and subjected tothe T4 endo V assay described in the previous paragraph. The resultingDNA profile (not shown) peaked in a position intermediate betweenthat of DNA from untreated cells and that of DNA from cells treatedwith high salt. We took this as an indication that trichostatinA facilitates the access of T4 endonuclease V to the DNA, althoughnot to the same extent as high saltdoes.

DNA from UV-irradiated cells pretreated with trichostatin A for 6 h or not pretreated was blotted onto a nylon membrane andassayed for the presence of CPDs and (6-4)PPs by using specificmonoclonal antibodies (Fig. 6). Treatment with trichostatin Adid not improve the repair of CPDs in either cell type. Therewas marginal improvement in the removal of (6-4)PPs after trichostatinA treatment, although one could argue whether this effect wassignificant. In any case, it was no more marked in hNT neuronsthan in NT2 precursor cells, a result that would not have beenexpected if chromatin structure changes had been responsible forthe poor repair in neurons. In other words, destabilizing chromatinin hNT neurons did not cause their global genome repair capabilityto revert to what it had been prior to differentiation.

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FIG. 6. Effect of trichostatin A on the repair of CPDs and (6-4)PPs. DNA from NT2 cells (circles) and hNT neurons (diamonds) harvested at various times after UV irradiation was blotted onto a nylon membrane and assayed with monoclonal antibodies specific for CPDs or (6-4)PPs. For 6 h prior to irradiation, the cells were treated (solid symbols) or not treated (open symbols) with trichostatin A at 25 µg/ml for (6-4)PPs and 50 µg/ml for CPDs. Results are taken from two experiments performed in triplicate; the error bars indicate standard deviation.

Effect of differentiation on gene expression. Quantitative RT-PCR experiments were performed to determine whether the changes in repair phenotype observed during differentiationmight be explained by modulation in the expression of repair genes.The mRNA for the relevant genes was reverse transcribed and coamplifiedwith a reference gene, either a glyceraldehyde phosphate dehydrogenase(GAPDH) or a $beta$ -actin gene, to allow precise comparisons betweenexpression in NT2 and hNT cells. Figure 7 summarizes the resultsof these analyses for genes associated with repair (top panel)and other genes (bottom panel). It can be seen that expressionof most repair genes remained unaffected by the differentiationprocess, with the main exceptions being the two NER incision factors,XPG (induced four- to sevenfold) and ERCC1/XPF (induced two- tofivefold). More modestly induced genes were CSB and MO15, althoughthere was some discrepancy between the results obtained with GAPDHand $beta$ -actin as a control. In fact, in most cases, the use of $beta$ -actinas a control provided higher induction values than did the useof GAPDH. This is probably because the expression of one or bothof these reference genes is affected by differentiation. Finally,because the XPC-hHR23B complex is necessary for the global genomerepair subpathway, it is worth noting that both XPC and hHR23Bwere repressed to about 70% of the control values.

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FIG. 7. Effect of differentiation on gene expression. Total RNA from NT2 precursor cells and hNT neurons was reverse transcribed, and quantitative PCRs were performed for repair genes (top panel) or nonrepair genes (bottom panel) (note the change in scale). Normalization was achieved by coamplifying a reference gene, either the GAPDH or $beta$ -actin gene. Bars show the means of one to six measurements, depending on the gene; the error bars indicate standard error of the mean. Data are expressed as the ratio of expression in hNT neurons to that in NT2 cells.

Among the genes not directly related to DNA repair, the neuron-specific neurofilament genes NF-L and NF-M were massively induced,as expected. The DHFR and p53 genes were repressed about twofold,whereas p21/WAF was induced two- tosevenfold.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The analysis of DNA metabolism in terminally differentiated cells poses quite a challenge to the experimenter since thesecells do not grow in vitro. Resorting to primary cells is noteasily done for human cells, particularly for neurons. The NT2-hNTcell system therefore represents a suitable compromise: the NT2precursor cells, although neoplastic, are likely to present areasonably normal phenotype, and the hNT neurons, resulting fromthe differentiation process, are very similar to normal neurons.In particular, hNT cells express neuron-specific genes (Fig. 7)and histological markers. They have been widely used for biochemical,cytological, and electrophysiological studies involving neurons(12, 18). The main drawback of this system is the low yieldof hNT neurons, which limits the number and feasibility of sometypes ofexperiments.

Using the NT2-hNT model system for differentiating human neurons, we showed that upon differentiation, global genomic repairof CPDs was markedly decreased in hNT neurons (Fig. 1). A moredetailed analysis, distinguishing CPDs from (6-4)PPs with specificmonoclonal antibodies (Fig. 2), allowed us to detect low levelsof repair for (6-4)PPs: nearly complete removal was achieved after3 days in hNT neurons, whereas it was substantially completedwithin hours in NT2 cells. Since it is well known that (6-4)PPsare repaired faster than CPDs (31), it is conceivable that CPDscould be completely removed after several weeks. Unfortunately,this was impossible to assay since hNT cultures are never completelyfree of precursor cells: initially the proportion of NT2 cellsis less than 5%, but because those cells replicate, they rapidlyoutnumber the hNT neurons. Another explanation for the residualrepair of (6-4)PPs in hNT neurons is that they could be more accessiblethan CPDs to the repair complex, since they are concentrated inthe linker regions between nucleosome cores (8).

Repair of transcribed genes, on the other hand, was fully functional in hNT neurons (Fig. 3). One could rationalize that sinceneurons do not need to replicate their DNA, they do not need torepair the bulk of their genome and therefore can concentrateon the genes that are expressed and essential for their function.In addition, it seems that hNT neurons display a peculiar transcription-coupledrepair phenotype, in that they repair the nontranscribed strandbetter than would be expected for cells that are deficient inCPD repair in the global genome overall. A possible explanationfor the latter observation is that a neuron-specific promotertriggers transcription of the opposite strand in hNT neurons.One can even envision that this could be a general strategy usedby terminally differentiated cells to increase the repair of thenontranscribed strand in critical genes. We thus made use of asensitive RT-PCR approach to try to detect such transcriptionproducts (Fig. 4). Under those conditions, we could not detectany transcription of the nontranscribed strand in hNTneurons.

By definition, TCR occurs only in the transcribed strand; the nontranscribed strand is supposedly dealt with by global genomerepair (10). However, in hNT neurons, the global genome repairis greatly impaired whereas the repair of the nontranscribed strandis proficient in active genes, which calls for a different explanation.This phenomenon, which we tentatively have termed differentiation-associatedrepair (DAR), seems to be confined to transcribed genes, as judgedby the poor repair of the silent glucagon gene in hNT neurons.Such a situation was previously encountered in two rodent modelsystems, rat myoblasts differentiating to myocytes (13) andrat PC12 pheochromocytoma cells that display a neuron-like phenotypeupon differentiation (reviewed in reference 11). Human HL60promyelocytic leukemia cells also showed an improved repair ofthe nontranscribed strand in the c-myc gene after differentiation(14). By contrast, different results were reported for Swissmouse 3T3 cells, which, when differentiating into adipocytes,exhibited reduced unscheduled DNA synthesis (a measure of repair)(27) but also lost the capacity to selectively repair transcribedgenes (2). However, strand-specific repair was not assayedin that study (2). To our knowledge, this is the first timeDAR has been described in humanneurons.

It is known that terminal differentiation in neurons is concomitant with important changes in the composition and structureof the chromatin, involving different histone variants and nucleosomerepositioning (17). Thus, a possible explanation for our observationsis that the chromatin structure in neurons is somewhat denser,which would make it more difficult for repair enzymes to accessthe lesions. By contrast, active genes would be exposed by thetranscription process and both their strands could benefit fromthe increased availability of repair enzymes, relieved from theiroverall global genome repair commitment. However, we have notbeen able to validate such a model, even using two different approaches.First, the enzyme T4 endo V accessed CPDs in hNT neurons justas well as in NT2 cells (Fig. 5). Furthermore, a chromatin-destabilizingcompound, trichostatin A, did not improve global genome repairin hNT neurons (Fig. 6). This suggests that the defect in globalgenome repair observed in hNT neurons is not due to a denser chromatinstructure.

Another possibility is that differentiation affects the expression of one or more repair genes. For instance, a massive decreasein XPC protein could explain the poor global genome repair, mimickingthe situation observed in XPC cells in which global genomic repairis defective but TCR is normal (30). It was not possible tomeasure protein levels directly for all the known repair enzymesbecause of the small amount of material that could be obtainedfrom hNT cultures and because antibodies are not available foreach enzyme. Therefore, we used a quantitative RT-PCR approach,keeping in mind the limitation that it would not detect any posttranscriptionalregulation. Our measurements (Fig. 7) revealed only a small decreasein the mRNA levels of XPC and of its partner hHR23B. Such a modestchange is not likely to be the cause of the massive impairmentin global genome repair we haveobserved.

On the other hand, several repair genes were found to be up-regulated by differentiation, mainly the two NER structure-specificnucleases, XPG and XPF/ERCC1. The current view of the molecularmechanism for NER is that a bulky lesion in the DNA, whether aUV-induced dimer or a chemical adduct, is recognized by a complexof proteins involving XPC, XPA, possibly XPE, and the single-strand-DNA-bindingprotein RPA. A denaturation bubble is created around the lesionwith the help of the helicases XPB and XPD, both of which areconstituents of the TFIIH general transcription factor. XPG thenincises the damaged strand 3' to the bubble, and the heterodimerXPF/ERCC1 cuts it on the 5' side, allowing the removal of a 27-to 29-nucleotide fragment containing the lesion. The resultinggap can now be sealed by DNA polymerase $delta$ or $varepsilon$ and DNA ligaseI. Although it is hard to imagine how an increase in the concentrationof the two incision enzymes would result in a decrease in globalgenome repair, it could well contribute to the better repair ofthe nontranscribed strand in transcriptionally active genes. Ifthis were true, it would imply that the limiting step for NERis not simply lesion recognition but, rather, incision of theDNA backbone. Indeed, it makes sense that lesion recognition wouldbe very sensitive but poorly specific whereas incision, the firstirreversible step, would occur only when the presence of a lesionhas beenverified.

It has been shown in this laboratory that p53-deficient cells exhibit an impairment in global genome repair of CPDs whileretaining their capabilities for TCR (5, 6). This phenotypeis similar to what we have observed in neurons, raising the possibilitythat p53 plays a role in DAR. Our RT-PCR quantification experimentswith hNT neurons indeed revealed a 50% decrease in the level p53mRNA but at the same time an increase in the level of p21/WAF,whose promoter is one of the targets of p53 (1). Since it isknown that marginal amounts of p53 generally result in normalrepair of (6-4)PPs (5), a twofold decrease is not likely tobe responsible for the impaired global genome repair in hNT neurons.On the other hand, although p21/WAF can also be activated by ap53-independent pathway, its induction in hNT neurons stronglysuggests a posttranscriptional activation of p53 that would stimulatethe transcription of several target genes, including p21/WAF.A feedback mechanism, such as the known mdm2/p53 feedback loop(1), could be responsible for the subsequent transcriptionalrepression of p53. In fact, such a situation has been observedin several other terminally differentiated cell types such asmyocytes and keratinocytes (20, 26, 32), in which p53 mRNAand, sometimes, protein levels are lower but the p53 activityis higher than that in precursor cells. Thus, it appears thatp53 is generally activated posttranscriptionally upon differentiation.However, this activation is not expected to trigger the apoptosispathway, since this would be a disastrous option for cells thatdo not multiply and cannot be replaced. Indeed, we have observedby microscopic examination or trypan blue counting that hNT neuronsappear to be more resistant than NT2 cells to killing by UV radiation(data notshown).

We are currently investigating the possibility that this repair phenotype in differentiated neurons is not limited to NERand that other repair systems, such as base excision repair, arealso affected. This would provide an alternative explanation forthe spectacular increase in the level of XPG mRNA, which was evenmore striking than those of ERCC1 and XPF: coamplification ofXPG with XPF indicated that the XPG/XPF ratio increases abouttwofold upon differentiation (data not shown). It has been recentlyshown that XPG, unlike other NER enzymes, is also involved inthe removal of oxidative lesions that are traditionally thoughtto be repaired by base excision repair (although NER is also ableto remove this type of damage [24]). Furthermore, XPG has beenimplicated in the TCR of such lesions (3, 23) and stimulatesbase excision repair in vitro (16). Neurons have a high cellularmetabolism (9), and it is therefore likely that oxidative lesionsare more of a challenge for them than are UV-induced lesions orbulky adducts. Stimulating the transcription of XPG and possiblyother genes involved in base excision repair might be an importantstrategy to cope with a higher level of oxidative lesions. Inthis respect, the fact that about half the xeroderma pigmentosumgroup G patients also suffer from Cockayne syndrome, which includessevere neurological problems, emphasizes the important role ofXPG inneurons.

Similarly, turning off repair at the global genome level to concentrate on the repair of transcribed genes may be the beststrategy to deal with the continuing induction of damage in postmitoticcells. However, this strategy would result in poor repair of thenontranscribed strand in these genes, since this strand is repairedby the same mechanism as that for the bulk of the genome. Sincethe nontranscribed strand will be needed as a template for repairingthe transcribed strand, it should not be allowed to accumulatedamage for decades. If it were, there would be a significant probabilitythat a lesion in the nontranscribed strand could interfere withthe synthesis of a repair patch, within 29 nucleotides arounda lesion in the transcribed strand. The NER machinery would thenintroduce a mutation in the transcribed strand when repairingit, a potentially disastrous situation. It therefore makes sensethat a special mechanism, such as DAR, might ensure that the nontranscribedstrand will be equally well repaired in terminally differentiatedcells. It has often been suggested that neuron aging and someforms of dementia could be due to the accumulation of unrepairedDNA lesions, which would eventually interfere with neuronal function(9, 19). The mechanisms we suggest could be a way for normalneurons to delay, if not preclude, suchevents.

	ACKNOWLEDGMENTS

We are indebted to Peter Andrews for providing us with NT2 cells and useful advice on how to grow them. We gratefully thankToshio Mori for the gift of anti-CPD and anti-(6-4)PPs antibodiesand Stephen Lloyd for the gift of T4 endonuclease V. We thankC. A. Smith and A. K. Ganesan for advice and helpfuldiscussions.

This work was supported by grants from the Swiss National Science Foundation (823-046695) and from the Novartis Jubilaum Stiftungto T.N. and an Outstanding Investigator Grant, CA44349, from theNational Cancer Institute to P.C.H.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Biological Sciences, Stanford University, Stanford, CA 94305-5020. Phone:(650) 723-2424. Fax: (650) 725-1848. E-mail: hanawalt{at}leland.stanford.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Bates, S., and K. H. Vousden. 1996. p53 in signalling checkpoint arrest or apoptosis. Curr. Opin. Genet. Dev. 6:12-19[CrossRef][Medline].

2. Bill, C. A., B. M. Grochan, R. E. Meyn, V. A. Bohr, and P. J. Tofilon. 1991. Loss of intragenomic DNA repair heterogeneity with cellular differentiation. J. Biol. Chem. 266:21821-21826[Abstract/Free Full Text].

3. Cooper, P. K., T. Nouspikel, S. G. Clarkson, and S. A. Leadon. 1997. Defective transcription-coupled repair of oxidative base damage in Cockayne syndrome patients from xeroderma pigmentosum group G. Science 275:990-993[Abstract/Free Full Text].

4. Enoch, E., and C. Norbury. 1995. Cellular responses to DNA damage: cell-cycle checkpoints, apoptosis and the roles of p53 and ATM. Trends Biol. Sci. 20:426-430.

5. Ford, J., and P. C. Hanawalt. 1997. Expression of wild-type p53 is required for efficient global genomic nucleotide excision repair in UV-irradiated human fibroblasts. J. Biol. Chem. 272:28073-28080[Abstract/Free Full Text].

6. Ford, J. M., and P. C. Hanawalt. 1995. Li-Fraumeni syndrome fibroblasts homozygous for p53 mutations are deficient in global DNA repair but exhibit normal transcription-coupled repair and enhanced UV resistance. Proc. Natl. Acad. Sci. USA 92:8876-8880[Abstract/Free Full Text].

7. Friedberg, E. C., G. C. Walker, and W. Siede. 1995. DNA repair and mutagenesis. ASM Press, Washington, D.C.

8. Gale, J. M., and M. J. Smerdon. 1990. UV induced (6-4) photoproducts are distributed differently than cyclobutane dimers in nucleosomes. Photochemi. Photobiol. 51:411-417.

9. Gensler, H. L., and H. Bernstein. 1981. DNA damage as the primary cause of aging. Q. Rev. Biol. 56:279-303[CrossRef][Medline].

10. Hanawalt, P. C. 1994. Transcription-coupled repair and human disease. Science 266:1957-1958[Free Full Text].

11. Hanawalt, P. C., P. Gee, L. Ho, R. K. Hsu, and C. J. M. Kane. 1992. Genomic heterogeneity of DNA repair. Role in aging? Ann. N. Y. Acad. Sci. 663:17-25[Medline].

12. Hardy, M., D. Younkin, C.-M. Tang, J. Pleasure, Q.-Y. Shi, M. Williams, and D. Pleasure. 1994. Expression of non-NMDA glutamate receptor chanel genes by clonal human neurons. J. Neurochem. 63:482-489[Medline].

13. Ho, L., and P. C. Hanawalt. 1991. Gene-specific DNA repair in terminally differentiating rat myoblasts. Mutat. Res. DNA Repair 255:124-141.

14. Islas, A., and P. C. Hanawalt. 1995. DNA repair in the MYC and FMS proto-oncogenes in ultraviolet light-irradiated human HL60 promyelocytic cells during differentiation. Cancer Res. 55:336-341[Abstract/Free Full Text].

15. Jensen, L., and S. Linn. 1988. A reduced rate of bulky DNA adduct removal is coincident with differentiation of human neuroblastoma cells induced by nerve growth factor. Mol. Cell. Biol. 8:3964-3968[Abstract/Free Full Text].

16. Klungland, A., M. Höss, D. Gunz, A. Constantinou, S. G. Clarkson, P. W. Doetsch, P. H. Bolton, R. D. Wood, and T. Lindahl. 1999. Base excision repair of oxidative DNA damage activated by XPG protein. Mol. Cell 3:33-42[CrossRef][Medline].

17. Kuenzle, C. C., C. W. Heizmann, U. Hubscher, R. Hobi, G. C. Winkler, A. W. Jaeger, and G. Morgenegg. 1983. Chromatin changes accompanying neuronal differentiation. Cold Spring Harbor Symp. Quant. Biol. 48:493-499.

18. Lee, V. M. Y., and P. W. Andrews. 1986. Differentiation of NTERA-2 clonal human embryonal carcinoma cells into neurons involves the induction of all three neurofilament proteins. J. Neurosci. 6:514-521[Abstract].

19. Lindahl, T. 1993. Instability and decay of the primary structure of DNA. Nature 362:709-715[CrossRef][Medline].

20. Lutzker, S., and A. Levine. 1996. A functionally inactive p53 protein in teratocarcinoma cells is activated by either DNA damage or cellular differentiation. Nat. Med. 2:804-810[CrossRef][Medline].

21. McCombe, P., M. Lavin, and C. Kidson. 1976. Control of DNA repair linked to neuroblastoma differentiation. Int. J. Radiat. Biol. Relat. Stud. Phys. Chem. Med. 29:523-531[Medline].

22. Mori, T., M. Nakane, T. Hattori, T. Matsunaga, M. Ihara, and O. Nikaido. 1991. Simultaneous establishment of monoclonal antibodies specific for either cyclobutane pyrimidine dimer or (6-4) photoproduct from the same mouse immunized with ultraviolet-irradiated DNA. Photochem. Photobiol. 54:225-232[Medline].

23. Nouspikel, T., P. Lalle, S. A. Leadon, P. K. Cooper, and S. G. Clarkson. 1997. A common mutational pattern in Cockayne syndrome patients from xeroderma pigmentosum group G: implications for a second XPG function. Proc. Natl. Acad. Sci. USA 94:3116-3121[Abstract/Free Full Text].

24. Scott, A. D., M. Neishabury, D. H. Jones, S. H. Reed, S. Boiteux, and R. Waters. 1999. Spontaneous mutation, oxidative DNA damage, and the roles of base and nucleotide excision repair in the yeast Saccharomyces cerevisiae. Yeast 15:205-218[CrossRef][Medline].

25. Spivak, G., and P. C. Hanawalt. 1995. Determination of damage and repair in specific DNA sequences. Gene Methods Companion Methods Enzymol. 7:147-161.

26. Tamir, Y., and E. Bengal. 1998. p53 protein is activated during muscle differentiation and participates with MyoD in the transcription of muscle creatine kinase gene. Oncogene 17:347-356[CrossRef][Medline].

27. Tofilon, P. J., and R. E. Meyn. 1988. Influence of cellular differentiation on repair of ultraviolet-induced DNA damage in murine proadipocytes. Radiat. Res. 116:217-237[Medline].

28. van Hoffen, A., A. T. Natarajan, L. V. Mayne, A. A. van Zeeland, L. H. Mullenders, and J. Venema. 1993. Deficient repair of the transcribed strand of active genes in Cockayne's syndrome cells. Nucleic Acids Res. 21:5890-5895[Abstract/Free Full Text].

29. van Zeeland, A. A., C. A. Smith, and P. C. Hanawalt. 1981. Sensitive determination of pyrimidine dimers in DNA of UV-irradiated mammalian cells. Introduction of T4 endonuclease V into frozen and thawed cells. Mutat. Res. 82:173-189[Medline].

30. Venema, J., A. van Hoffen, V. Karcagi, A. T. Natarajan, A. A. van Zeeland, and L. H. F. Mullenders. 1991. Xeroderma pigmentosum complementation group C cells remove pyrimidine dimers selectively from the transcribed strand of active genes. Mol. Cell. Biol. 11:4128-4134[Abstract/Free Full Text].

31. Vreeswijk, M. P., A. van Hoffen, B. E. Westland, H. Vrieling, A. A. van Zeeland, and L. H. Mullenders. 1994. Analysis of repair of cyclobutane pyrimidine dimers and pyrimidine 6-4 pyrimidone photoproducts in transcriptionally active and inactive genes in Chinese hamster cells. J. Biol. Chem. 269:31858-31863[Abstract/Free Full Text].

32. Weinberg, W., C. Azzoli, K. Chapman, A. Levine, and S. Yuspa. 1995. p53-mediated transcriptional activity increases in differentiating epidermal keratinocytes in association with decreased p53 protein. Oncogene 10:2271-2279[Medline].

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1.	Bates, S., and K. H. Vousden. 1996. p53 in signalling checkpoint arrest or apoptosis. Curr. Opin. Genet. Dev. 6:12-19[CrossRef][Medline].
2.	Bill, C. A., B. M. Grochan, R. E. Meyn, V. A. Bohr, and P. J. Tofilon. 1991. Loss of intragenomic DNA repair heterogeneity with cellular differentiation. J. Biol. Chem. 266:21821-21826[Abstract/Free Full Text].
3.	Cooper, P. K., T. Nouspikel, S. G. Clarkson, and S. A. Leadon. 1997. Defective transcription-coupled repair of oxidative base damage in Cockayne syndrome patients from xeroderma pigmentosum group G. Science 275:990-993[Abstract/Free Full Text].
4.	Enoch, E., and C. Norbury. 1995. Cellular responses to DNA damage: cell-cycle checkpoints, apoptosis and the roles of p53 and ATM. Trends Biol. Sci. 20:426-430.
5.	Ford, J., and P. C. Hanawalt. 1997. Expression of wild-type p53 is required for efficient global genomic nucleotide excision repair in UV-irradiated human fibroblasts. J. Biol. Chem. 272:28073-28080[Abstract/Free Full Text].
6.	Ford, J. M., and P. C. Hanawalt. 1995. Li-Fraumeni syndrome fibroblasts homozygous for p53 mutations are deficient in global DNA repair but exhibit normal transcription-coupled repair and enhanced UV resistance. Proc. Natl. Acad. Sci. USA 92:8876-8880[Abstract/Free Full Text].
7.	Friedberg, E. C., G. C. Walker, and W. Siede. 1995. DNA repair and mutagenesis. ASM Press, Washington, D.C.
8.	Gale, J. M., and M. J. Smerdon. 1990. UV induced (6-4) photoproducts are distributed differently than cyclobutane dimers in nucleosomes. Photochemi. Photobiol. 51:411-417.
9.	Gensler, H. L., and H. Bernstein. 1981. DNA damage as the primary cause of aging. Q. Rev. Biol. 56:279-303[CrossRef][Medline].
10.	Hanawalt, P. C. 1994. Transcription-coupled repair and human disease. Science 266:1957-1958[Free Full Text].
11.	Hanawalt, P. C., P. Gee, L. Ho, R. K. Hsu, and C. J. M. Kane. 1992. Genomic heterogeneity of DNA repair. Role in aging? Ann. N. Y. Acad. Sci. 663:17-25[Medline].
12.	Hardy, M., D. Younkin, C.-M. Tang, J. Pleasure, Q.-Y. Shi, M. Williams, and D. Pleasure. 1994. Expression of non-NMDA glutamate receptor chanel genes by clonal human neurons. J. Neurochem. 63:482-489[Medline].
13.	Ho, L., and P. C. Hanawalt. 1991. Gene-specific DNA repair in terminally differentiating rat myoblasts. Mutat. Res. DNA Repair 255:124-141.
14.	Islas, A., and P. C. Hanawalt. 1995. DNA repair in the MYC and FMS proto-oncogenes in ultraviolet light-irradiated human HL60 promyelocytic cells during differentiation. Cancer Res. 55:336-341[Abstract/Free Full Text].
15.	Jensen, L., and S. Linn. 1988. A reduced rate of bulky DNA adduct removal is coincident with differentiation of human neuroblastoma cells induced by nerve growth factor. Mol. Cell. Biol. 8:3964-3968[Abstract/Free Full Text].
16.	Klungland, A., M. Höss, D. Gunz, A. Constantinou, S. G. Clarkson, P. W. Doetsch, P. H. Bolton, R. D. Wood, and T. Lindahl. 1999. Base excision repair of oxidative DNA damage activated by XPG protein. Mol. Cell 3:33-42[CrossRef][Medline].
17.	Kuenzle, C. C., C. W. Heizmann, U. Hubscher, R. Hobi, G. C. Winkler, A. W. Jaeger, and G. Morgenegg. 1983. Chromatin changes accompanying neuronal differentiation. Cold Spring Harbor Symp. Quant. Biol. 48:493-499.
18.	Lee, V. M. Y., and P. W. Andrews. 1986. Differentiation of NTERA-2 clonal human embryonal carcinoma cells into neurons involves the induction of all three neurofilament proteins. J. Neurosci. 6:514-521[Abstract].
19.	Lindahl, T. 1993. Instability and decay of the primary structure of DNA. Nature 362:709-715[CrossRef][Medline].
20.	Lutzker, S., and A. Levine. 1996. A functionally inactive p53 protein in teratocarcinoma cells is activated by either DNA damage or cellular differentiation. Nat. Med. 2:804-810[CrossRef][Medline].
21.	McCombe, P., M. Lavin, and C. Kidson. 1976. Control of DNA repair linked to neuroblastoma differentiation. Int. J. Radiat. Biol. Relat. Stud. Phys. Chem. Med. 29:523-531[Medline].
22.	Mori, T., M. Nakane, T. Hattori, T. Matsunaga, M. Ihara, and O. Nikaido. 1991. Simultaneous establishment of monoclonal antibodies specific for either cyclobutane pyrimidine dimer or (6-4) photoproduct from the same mouse immunized with ultraviolet-irradiated DNA. Photochem. Photobiol. 54:225-232[Medline].
23.	Nouspikel, T., P. Lalle, S. A. Leadon, P. K. Cooper, and S. G. Clarkson. 1997. A common mutational pattern in Cockayne syndrome patients from xeroderma pigmentosum group G: implications for a second XPG function. Proc. Natl. Acad. Sci. USA 94:3116-3121[Abstract/Free Full Text].
24.	Scott, A. D., M. Neishabury, D. H. Jones, S. H. Reed, S. Boiteux, and R. Waters. 1999. Spontaneous mutation, oxidative DNA damage, and the roles of base and nucleotide excision repair in the yeast Saccharomyces cerevisiae. Yeast 15:205-218[CrossRef][Medline].
25.	Spivak, G., and P. C. Hanawalt. 1995. Determination of damage and repair in specific DNA sequences. Gene Methods Companion Methods Enzymol. 7:147-161.
26.	Tamir, Y., and E. Bengal. 1998. p53 protein is activated during muscle differentiation and participates with MyoD in the transcription of muscle creatine kinase gene. Oncogene 17:347-356[CrossRef][Medline].
27.	Tofilon, P. J., and R. E. Meyn. 1988. Influence of cellular differentiation on repair of ultraviolet-induced DNA damage in murine proadipocytes. Radiat. Res. 116:217-237[Medline].
28.	van Hoffen, A., A. T. Natarajan, L. V. Mayne, A. A. van Zeeland, L. H. Mullenders, and J. Venema. 1993. Deficient repair of the transcribed strand of active genes in Cockayne's syndrome cells. Nucleic Acids Res. 21:5890-5895[Abstract/Free Full Text].
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