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Differential Killing of Mismatch Repair-Deficient and -Proficient Cells

Towards the Therapy of Tumors with Microsatellite Instability

Institute of Molecular Cancer Research, University of Zürich, Zurich, Switzerland

	ABSTRACT

Top ABSTRACT Introduction Materials and Methods Results and Discussion REFERENCES

 
DNA mismatch repair (MMR) defects bring about a strong mutator phenotype and microsatellite instability (MSI). In an attempt to exploit MSI in cancer therapy, we constructed expression vectors carrying a thymidine kinase/blasticidin deaminase fusion gene downstream from a (C)₁₂ or an (A)₂₆ microsatellite and stably transfected these constructs into human cells in which the MMR status could be regulated by doxycycline. We now show that ganciclovir-resistant clones arising through frameshifts in the (C)₁₂ microsatellite were 20 times more frequent in cells in which MMR was inactivated. This difference may be exploited in gene therapy of tumors with MSI, which represent a substantial proportion of cancers of many different tissues.

	Introduction

Top ABSTRACT Introduction Materials and Methods Results and Discussion REFERENCES

 
A substantial proportion of tumors of different organs displays MSI¹ , a phenotypic trait characterized by a large increase in the frequency of frameshift mutations within repeated sequence elements, the so-called microsatellites. This anomaly is caused by inactivation of the postreplicative MMR system, which normally corrects strand misalignments arising in these repeats during DNA replication (1) . In hereditary nonpolyposis colon cancer kindred, which represents 5% of colon cancer patients, the MMR defect and MSI are linked to inherited mutations in genes encoding MMR proteins. In 10% of sporadic colon cancers, MSI arises as a result of epigenetic silencing of the MMR gene hMLH1 (2 , 3) , and an ever-increasing number of reports describe MSI also in cancers of head and neck, lung, prostate, breast, bladder, and other tissues (reviewed in Ref. 4 ). Past attempts to identify agents able to selectively kill MSI⁺ cells largely failed. Upon treatment with a range of DNA damaging agents, substantial differences in the response of MMR-deficient and -proficient cells were observed only for cisplatin, which kills MMR-proficient cells 3-fold more efficiently than MMR-deficient ones (5) and for S_N1-type methylating agents, where the difference is 100-fold (6 , 7) . MMR-deficient cells were reported to be more sensitive to killing by CCNU than MMR-proficient controls (8) , but this difference appears to be limited to only a subset of MMR-deficient cell lines. Thus, in an attempt to identify a more general approach toward the therapy of MMR-deficient tumors, we set out to exploit the MSI phenotype. In cultured human cells established from these tumors, MSI was reported to be two to three orders of magnitude higher than in control lines. We plan to introduce into the cells a toxin-encoding gene, the ORF of which is preceded by a labile microsatellite sequence such that the gene is out-of-frame (Fig. 1A) . If the microsatellite undergoes insertion or deletion mutagenesis, the toxin ORF should in a given number of events be shifted into the correct reading frame; the construct should thus express the functional toxin polypeptide, and the transduced cell should be killed. This experimental strategy should result in an efficient elimination of MMR-deficient cells, whereas MMR proficient cells in which the microsatellite remains stable should be unaffected. However, before deploying the above strategy, we needed to establish an experimental system that would permit us to reliably test the relative stability of a variety of microsatellite repeats in MMR-proficient and -deficient cells. The critical characteristics of the ideal repeat should be its high stability in the former cells and substantial instability in the latter. The mutation frequencies of several microsatellites have been previously studied, using a variety of assays (9, 10, 11, 12) . However, in these studies, two major problems were encountered. First, it could not be excluded that the repeats acquired mutations already during the lengthy selection of the stable transfectants. Second, the studies did not use isogenic pairs of MMR-proficient and -deficient cell lines such that it was impossible to exclude the effects on the mutation frequency of other genetic defects present in these cells. Indeed, Hanford et al. (9) described extensive variation among microsatellite mutation rates of different clones of the same cell line. We now describe a system that successfully overcomes these drawbacks by making use of a strictly isogenic cell pair and a reporter system that allows for the elimination of mutated transfectants before the initiation of the experiment.

View larger version (21K): [in this window] [in a new window] [Download PPT slide]   Fig. 1. A, scheme of a gene therapy approach designed to target MSI+ cells. The microsatellite repeat puts the toxin out of the correct reading frame, and thus the vector produces no functional polypeptide. In a MMR- cell, the toxin gene may be reverted into its correct reading frame through MSI, and the cell will be killed. In contrast, the repeat should remain stable in cells with functional MMR. B, the constructs used in this study. The (C)12 and (A)26 microsatellites or a control DNA sequence without a repeat were inserted downstream from the start codon of the TKBSD fusion protein while keeping the ORF in its correct reading frame. C, scheme of the test assay (see also "Materials and Methods"). 293T L cells were transfected with constructs shown in B, and stable clones were isolated using blasticidin selection. The selected clones were then grown in two separate subcultures: in the MMR-proficient (L+, without DOX) and -deficient (L-, with DOX). After 4, 8, and 13 days (which corresponds to 4, 8, and 13 cell generations, respectively), the cells were treated with GANC and plated to select for TK- mutants.

	Materials and Methods

Top ABSTRACT Introduction Materials and Methods Results and Discussion REFERENCES

Vector Construction.
The pSBCTKBSD vector (13) containing the fusion gene encoding thymidine kinase and blasticidin deaminase was used as a template for a PCR reaction in an assay consisting of 1x Cloned PFU buffer, 1 µM forward primer, 1 µM reverse primer, 200 ng of template DNA, 0.2 mM deoxynucleoside triphosphates and 2.5units/50µl reaction Pfu turbo DNA polymerase (Stratagene, La Jolla, CA). The primers (Microsynth, Balgach, Switzerland) were as follows: forward no-repeat, TGG CCA GGA TCC ACC ATG ATT GAA GAA TTC ATT GAA CAA GAT GGA TTG CAC GCA GG; forward (C)₁₂, TGG CCA GGA TCC ACC ATG ATT GAA CCC CCC CCC CCC ATT GAA CAA GAT GGA TTG CAC GCA GG; forward (A)₂₆, TGG CCA GGA TCC ACC ATG ATT GTC AAA AAA AAA AAA AAA AAA AAA AAA ATT GAA CAA GAT GGA TTG CAC GCA GG; and reverse, TAC TCG CTC GAG TCA ATG TAT CTT ATC ATG TCT GGA TCG. The PCR cycle was as follows: 98°C for 3 min, (98°C for 1 min, 69°C for 1 min, and 72°C for 5 min)₃₀, 72°C for 10 min. The PCR products were digested with BamHI and XhoI (both New England Biolabs, Beverly, MA) and cloned into the corresponding sites of pcDNA3 (Invitrogen), creating pcDNA3-TKBSD, pcDNA3-(C)₁₂TKBSD, and pcDNA3-(A)₂₆TKBSD vectors.

Isolation of Stable Transfectants.
pcDNA3-TKBSD, pcDNA3-(C)₁₂TKBSD, and pcDNA3-(A)₂₆TKBSD vectors were digested with BglII and DraIII (both New England Biolabs) and subjected to preparative gel electrophoresis. The fragments containing the TKBSD fusion gene were isolated and used for transfection of 293T L cells using the FuGENE reagent (Roche, Basel, Switzerland). Selection was initiated 2 days after transfection with 10 µg/ml blasticidin S (Invitrogen). After 2–3 weeks, stable clones were isolated and additionally propagated with blasticidin (100 µg/ml).

Mutagenesis Assays.
The selected clone, carrying the microsatellite repeat/TKBSD fusion stably integrated in the genome, was grown without or with 50 ng/ml DOX in a 6-well plate in a medium containing 100 µg/ml blasticidin for 7 days. At this time point, the cells grown in the presence of DOX were completely free of hMLH1 and thus MMR-deficient, and cells grown without DOX remained MMR proficient. The high concentration of blasticidin in the medium ensured elimination of cells with frameshifted inserts. The blasticidin was then removed and the cells were additionally propagated without or with DOX in a 6-well plate. As the doubling time is 24 h, the cells were split every 2 days in a ratio 1:4 to maintain a constant cell number. In the absence of blasticidin, cells in which the TKBSD fusion gene was inactivated by frameshift mutagenesis (or otherwise) survived. Immediately upon blasticidin withdrawal and at the selected time points (4, 8, and 13 days, 4, 8, and 13 generations), 1 x 10⁵ or 5 x 10⁴ cells were plated into 10-cm dishes in 10 ml of medium containing 30 µM GANC (Sigma, St. Louis, MO) to score for mutant (GANC-resistant) cells. At the same time, 300 cells were plated in a medium without GANC to assess plating efficiency (control). After 2 weeks of incubation, the colonies were stained with Giemsa (Fluka, Buchs, Switzerland) and counted (see Fig. 1C for a schematic outline of the experiment).

MSI Analysis.
Chromosomal DNA from the GANC-resistant colonies was extracted using the TRI reagent (Molecular Research Center, Cincinnati, OH). The vector DNA sequence containing the repeat was amplified by PCR under the following conditions: 1x Taq buffer, 1 µM forward primer, 1 µM reverse primer, 300 ng of template DNA, 0.2 mM deoxynucleoside triphosphates, and 2 units/50 µl reaction TaqDNA polymerase (New England Biolabs). The following primers (Microsynth, Balgach, Switzerland) were used: forward (GCG GTA GGC GTG TAC GGT G), reverse (CCA GTC CTC CCG CCA CGA CC). The PCR procedure was as follows: 95°C for 2 min (95°C for 1 min, 60°C for 1 min, and 72°C for 1 min 20 s)₂₅, 72°C for 10 min. The PCR products were purified, and the DNA regions containing the repeats were sequenced using the primer GTA CGT AGA CGA TAT CGT CG on an ABI PRISM 310 Genetic Analyzer (Applied Biosystems, Foster City, CA).

	Results and Discussion

Top ABSTRACT Introduction Materials and Methods Results and Discussion REFERENCES

 
The experimental system intended for use in gene therapy of tumors with MSI is based on transduction of the tumor cells with a vector carrying a toxin gene that is out-of-frame because of the insertion of a microsatellite immediately downstream from its AUG start codon (Fig. 1A) . The inherent instability of the microsatellite in MMR^- cells should result in restoration of the correct reading frame in a given percentage of the transduced cells and thus in expression of the toxin and cell death. However, for the purposes of the present study, we decided to invert this strategy by making use of an in-frame reporter/toxin combination that allows for a more accurate estimation of mutation frequencies and is free of artifacts (Fig. 1, B and C) . The reporter gene construct was a fusion of BSD from Aspergillus terreus and TK from Herpes simplex virus (13) . This fusion gene was preceded by a microsatellite repeat, which was inserted immediately downstream from the start codon, but which maintained the correct reading frame of the fusion gene. For the initial experiments, we chose the (A)₂₆ and (C)₁₂ repeats, together with a control construct that carried no repeat (Fig. 1B) . The BSD protein confers resistance against blasticidin, which permits the selection of clones carrying the nonmutated construct stably integrated in the genome. Inducing MMR deficiency in one-half of the cells by adding DOX to the culture medium and propagating the cells independently in a MMR-deficient or -proficient mode for several generations without selection allows for mutations within the repeat to occur. Addition of GANC to the medium then eliminates cells in which no frameshifting occurred (Fig. 1C) . Thus, by counting the surviving TK^- (GANC-resistant) colonies, we can calculate the mutation frequency in a cell population that consisted initially exclusively of TK⁺ cells (i.e., without preexisting mutants), all carrying the vector integrated in the same genomic sequence context and in a strictly isogenic genetic background.

Before initiating this study, we had to check the integrity of the stable clones carrying the reporter constructs, more specifically, the integrity of the Tet-Off system that controls the inducible expression of hMLH1. As shown in Fig. 2A , the 293T L⁺ cells and the clone stably transfected with the pcDNA3-(C)₁₂TKBSD vector [denoted 293T L⁺(C)₁₂TKBSD] expressed both hPMS2 and hMLH1 in similar amounts. In the presence of DOX, the transcription of hMLH1 was shut off, which resulted in the depletion of the hMLH1/hPMS2 heterodimer (7) ; these cells are denoted 293T L^-(C)₁₂TKBSD. The selected clones carrying the pcDNA3-(A)₂₆TKBSD and pcDNA3-TKBSD vectors, 293T L(A)₂₆TKBSD and 293T L TKBSD, respectively, behaved similarly (data not shown).

View larger version (52K): [in this window] [in a new window] [Download PPT slide]   Fig. 2. Differences in repeat stability in isogenic 293T L cells. A, Western blot analysis of total cell extracts of 293T L (C)12TKBSD cells cultured in the absence (L+, expressing hMLH1/hPMS2) or presence (L-, not expressing hMLH1/hPMS2) of 50 ng/ml DOX. The extracts of 293T L+ cells are shown as the positive control. (See Ref. 7 for experimental details.) ß-Tubulin was used to ascertain equal gel loading. B and C, comparison of repeat stabilities in isogenic MMR-proficient (L+) and -deficient (L-) cells. B, example of a typical result of an assay described in Fig. 1C . Cells were grown for 8 days without blasticidin, treated with GANC, plated, and the GANC-resistant colonies (GANCr) were stained and counted after 2 weeks. Control, cells plated without GANC to estimate plating efficiency (see "Materials and Methods"). C, numbers of GANC-resistant colonies were adjusted, using plating efficiency, for 5 x 104 plated colony-forming cells, and plotted for each time point. Each data point represents the mean of five independent experiments; error bars show SD. D, MSI analysis. Left panel, original sequence without mutations; right panel, loss of one repeat unit.

Microsatellite mutation frequencies measured in our MMR-deficient cells (Fig. 2C and Table 2 ) roughly corresponded to those described by others (9 , 14 , 15) . However, the relative differences between MMR-proficient and -deficient cells were somewhat smaller: 20-fold in our system as compared with 16–340-fold as described by Hanford et al. (9) or 25–100-fold as described by Kahn et al. (12) . However, the latter studies compared mutation frequencies of MMR-deficient colon carcinoma cells either with those of unrelated MMR-proficient colon carcinoma cells or even with those of MMR-proficient cancer or normal cells of different type. It has been well documented that cells acquire a plethora of mutations during transformation. Some of these mutations might inactivate cell cycle checkpoint pathways, which might allow DNA replication in the presence of DNA damage, and thus permit the accumulation of additional mutations even in a MMR-proficient background. Indeed, Boyer and Farber (16) found a 75-fold difference in the mutation frequency of the same microsatellite in MMR-proficient normal human fibroblasts and fibrosarcoma cells. Clearly, genetic differences between cells of different origin make a direct comparison of mutation frequencies very difficult.

The 20-fold difference in the stability of the (C)₁₂ microsatellite between MMR-proficient and -deficient cells is lower than might have been anticipated from the results of earlier studies, however, given the extremely low mutation frequency in the MMR-proficient cells, it is likely to be therapeutically exploitable. Moreover, it is highly likely that analysis of a larger number of mononucleotide and dinucleotide repeats will identify a sequence with a substantially higher therapeutic index. Thus, exploitation of the MSI phenotype, which is currently estimated to segregate with 15% of colon cancers, may represent a valid approach toward combating these tumors and, more importantly, their metastases.

One of the major challenges of tumor therapy is acquired resistance to treatment. Because the MSI phenotype is linked with defective MMR, the only chance the transduced cell has to escape death is either to stop replicating, which would in itself lead to tumor regression, or to silence the transcription of the transgene. The latter scenario is unlikely because gene silencing requires as a rule many cell divisions and because the microsatellite repeat tested in our study was unstable after only four replication cycles. Even if this problem should arise, it could be overcome by repeated transductions. It is therefore likely that the problem of resistance will not pose a substantial threat to this approach.

The study described above represents but an initial step toward this goal. As the environment of cells in tumors differs dramatically from that in cell culture, it will be necessary to carry out in vivo experiments using, in the first instance, human tumor xenografts in nude mice. Should these experiments meet with success, the transducing vector will be remodeled to carry the suicide gene out-of-frame, which would be moved into the correct reading frame through selective frameshift mutagenesis in MSI cells, as shown in Fig. 1A . In a gene therapy setting, most cells in solid tumors are not transduced and it is likely that not each cell will mutate the microsatellite. But as tumor cells are in close contact, it is anticipated that the suicide gene will exert a bystander effect, which should bring about the death not only of the transduced cell that acquired the frameshift mutation but also of a number of surrounding cells (17) . A complete eradication of a tumor expressing TK has been reported, although only 10% of the tumor cells expressed the enzyme (17) . Cytosine deaminase, another suicide gene frequently used in gene therapy trials, has been reported to be effective even if only 2% of the tumor cells were transduced (18) , and strategies causing even more effective bystander effects are being developed (19) . The system described in this study should permit the identification of the most effective microsatellite/enzyme/prodrug combination that could then be further developed for therapeutic use.

	ACKNOWLEDGMENTS

 
We thank Dr. Niels de Wind for constructive discussions during the initial phases of this project. We also thank Dr. Christiaan Karreman for the generous gift of the pSBCTKBSD plasmid and Dr. Pavel Janscak for critical reading of the manuscript.

	FOOTNOTES

 
Grant support: UBS AG (to P. C.) and from the European Community Grant QLG1-CT-2000-001230 (to J. J., Z. S.).

The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore be hereby marked advertisement in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

Present address: Zuzana Storchova, Department of Pediatric Oncology, The Dana-Farber Cancer Institute, Boston, Massachusetts.

Requests for reprints: Josef Jiricny. Phone: 41-1-634-8910; Fax: 41-1-634-8904; E-mail: jiricny{at}imr.unizh.ch

¹ The abbreviations used are: MSI, microsatellite instability; BSD, blasticidin deaminase; DOX, doxycycline; GANC, ganciclovir; MMR, mismatch repair; ORF, open reading frame; TK, thymidine kinase; TKBSD, thymidine kinase/blasticidin deaminase fusion gene.

Received 8/14/03. Revised 10/ 2/03. Accepted 10/16/03.

	REFERENCES

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