Dihydropyrimidine dehydrogenase (DPD) is the initial and rate-limiting enzyme in the catabolism of 5-fluorouracil (5FU), and it is suggested that patients with a partial deficiency of this enzyme are at risk from developing a severe 5FU-associated toxicity. In this study, we demonstrated that a lethal toxicity after a treatment with 5FU was attributable to a complete deficiency of DPD. Analysis of the DPD gene for the presence of mutations showed that the patient was homozygous for a G→A mutation in the invariant GT splice donor site flanking exon 14 (IVS14+1G>A). As a consequence, no significant residual activity of DPD was detected in peripheral blood mononuclear cells. To determine the frequency of the IVS14+1G>A mutation in the Dutch population, we developed a novel PCR-based method allowing the rapid analysis of the IVS14+1G>A mutation by RFLP. Screening for the presence of this mutation in 1357 Caucasians showed an allele frequency of 0.91%. In our view, the apparently high prevalence of the IVS14+1G>A mutation in the normal population, with 1.8% heterozygotes, warrants genetic screening for the presence of this mutation in cancer patients before the administration of 5FU.

5FU3 remains one of the most widely used chemotherapeutic agents for the systemic treatment of cancers of the gastrointestinal tract, breast, and head and neck. As a single drug, 5FU has only limited efficacy. To improve the clinical response of 5FU, optimal administration schedules as well as the combination of 5FU with other drugs, which should increase its antitumor activity or decrease the host toxicity, have been investigated. It has been shown that long-term continuous i.v. infusion of 5FU is superior to bolus injections of 5FU in terms of response rate, however, only a small increase in median survival was observed (1), and high inter- and intrapatient variations in the plasma concentrations of 5FU have been observed during prolonged infusion of the drug (2). In addition, a relationship between the 5FU dose intensity and the therapeutic response, as well as toxicity, has been noted (3, 4).

An important determinant in predicting the toxicity as well as the efficacy of 5FU might be the activity of DPD. DPD is the initial and rate-limiting enzyme in the catabolism of the pyrimidine bases uracil and thymine, but also of the pyrimidine analogue 5FU. It has been reported that >80% of the administered 5FU is catabolized by DPD (5). Furthermore, a correlation has been observed between the pretreatment activity of DPD in PBM cells and the systemic clearance of 5FU in cancer patients (6). The pivotal role of DPD in chemotherapy using 5FU has been shown in cancer patients with a complete or near-complete deficiency of this enzyme. These patients suffered from severe toxicity, including death, after the administration of 5FU (7, 8, 9, 10, 11). It was shown that a number of these patients were genotypically heterozygous for a mutant DPD allele (9, 10, 11, 12). To date, 17 variant DPYD alleles have been identified in pediatric patients suffering from a complete or near-complete DPD deficiency, or in tumor patients with decreased DPD activity (12, 13, 14, 15). Analysis of the prevalence of the various mutations among DPD patients has shown that the splice-site mutation, IVS14+1G>A, was by far the most common one (52%; Ref. 13).

To date, the frequency of the splice site mutation IVS14+1G>A in the normal population is not known. On the basis of population analysis of the DPD activity, the frequency of heterozygotes has been estimated to be as high as 3% (6). Such individuals might be at risk of developing severe toxicity after the administration of 5FU. Furthermore, only a small number of cases have been reported regarding lethal toxicity after the administration of 5FU. In none of these cases have the molecular mechanisms underlying the 5FU-induced death been resolved. In this paper, we describe a simple genotyping procedure to test for the presence of the IVS14+1G>A mutation. Furthermore, we describe the first patient with lethal toxicity, after the administration of 5FU, who proved to be homozygous for the IVS14+1G>A mutation.

Chemicals.

[4-14C]-thymine (1.85–2.22 GBq/mmol) was obtained from Moravek Biochemicals (Brea, CA). Lymphoprep (specific gravity, 1.077 g/ml; 280 mOsm) was obtained from Nycomed Pharma AS (Oslo, Norway). LeucoSep tubes were supplied by Greiner (Frickenhausen, Germany). FCS was obtained from BioWhittaker (Walkersville, MD). HAM-F10 medium with 20 mm HEPES was obtained from Life Technologies, Inc. (Breda, the Netherlands). AmpliTaq Taq polymerase BigDye-Terminator-Cycle-Sequencing-Ready Reaction kits were supplied by Perkin-Elmer Corp. (Foster City, CA). Restriction endonuclease NdeI was obtained from Roche Diagnostics Nederlands B.V. (Almere, the Netherlands). A Qiaquick Gel Extraction kit was obtained from Qiagen (Hilden, Germany). All other chemicals used were of analytical grade.

Analysis of Pyrimidine Bases.

The concentrations of the pyrimidine bases, uracil and thymine in plasma, were determined using reversed-phase HPLC combined with diode-array detection, as described before (16).

Culture Conditions of Human Fibroblasts.

Fibroblasts were cultured from skin biopsies obtained from controls and the index patient. Biopsies were incubated at 37°C in HAM-F10 medium, supplemented with 20 mm HEPES and 15% (v/v) FCS in 25-cm2 cell-culture flasks until an adequate number of proliferating cells was obtained. Subsequently, cells were cultured in HAM-F10 medium supplemented with 20 mm HEPES and 10% (v/v) FCS. Fibroblasts were harvested with 0.25% (w/v) trypsin, and after washing the cells once with PBS and twice with 0.9% (w/v) NaCl, the cells were collected by centrifugation (175 × g at 7°C for 5 min), and the supernatant was discarded. The pellets were stored at −80°C.

Isolation of Human PBM Cells and Granulocytes.

PBM cells were isolated from 15 ml EDTA-anticoagulated blood by centrifugation over Lymphoprep, and the cells from the interface were collected and treated with ice-cold NH4Cl to lyse the contaminating erythrocytes, as described before (17). The pellet of the centrifugation step over Lymphoprep containing the granulocytes and erythrocytes was diluted with 7 ml of supplemented PBS [9.2 mm Na2HPO4, 1.3 mm NaH2PO4, 140 mm NaCl, 0.2% (w/v) BSA, 13 mm sodium citrate, and 5 mm glucose (pH 7.4)] and centrifuged at 800 × g at room temperature for 10 min. To lyse the erythrocytes, the pellet was resuspended in 7 ml of ice-cold ammonium chloride solution (155 mm NH4Cl, 10 mm KHCO3, and 0.1 mm EDTA) and kept on ice for 5 min. After the addition of 10 ml of ice-cold supplemented PBS, the solution was centrifuged at 250 × g at 4°C for 10 min. The pellet was collected and subjected to another lysis step as described above. The pellet containing the granulocytes was washed once more with supplemented PBS, and the final cell pellet was frozen in liquid nitrogen and stored at −80°C until further analysis.

Determination of the DPD Activity.

The activity of DPD was determined in a reaction mixture containing 35 mm potassium phosphate (pH 7.4), 2.5 mm MgCl2, 1 mm DTT, 250 μm NADPH, and 25 μm [4-14C]-thymine (17). Separation of radiolabeled thymine from radiolabeled dihydrothymine was performed isocratically [50 mm NaH2PO4 (pH 4.5) at a flow rate of 2 ml/min] by high-performance liquid chromatography on a reversed-phase column (Alltima C18; 250 × 4.6 mm; 5-μm particle size; Alltech Associates Inc., Deerfield, IL) and protected by a guard column (Supelguard LC-18-S; 5-μm particle size; 20 × 4.6 mm; Supelco, Bellefonte, PA) with online detection of the radioactivity, as described before (17). Protein concentrations were determined with a copper-reduction method using bicinchoninic acid, essentially as described by Smith et al.(18).

PCR Amplification of Exon 14.

DNA was isolated from purified granulocytes by standard procedures. PCR amplification of exon 14 and its flanking intronic regions was carried out using the primer sets DPD14f and DPD14r as specified in Table 1. Amplification of exon 14 was carried out in a 50-μl reaction mixture containing 10 mm Tris-HCl (pH 8.3), 50 mm KCl, 2 mm MgCl2, 10 pmol each primer, 200 μm each deoxynucleotide triphosphate, and 2 units of Taq polymerase. After initial denaturation for 5 min at 95°C, amplification was carried out for 35 cycles (1 min 95°C, 1 min 55°C, 1 min 72°C). The PCR product was separated on 1% agarose gels, visualized with ethidium bromide, and purified using a Qiaquick Gel Extraction kit or used for direct sequencing.

RFLP of Exon 14.

PCR amplification of exon 14 and its flanking 5′ donor intronic region was carried out using the primer sets NDEf and NDEr as specified in Table 1. Amplification of exon 14 was carried out in a 25-μl reaction mixture containing 10 mm Tris-HCl (pH 8.3), 50 mm KCl, 3 mm MgCl2, 5 pmol each primer, 200 μm each deoxynucleotide triphosphate and 2 units of Taq polymerase. After initial denaturation for 5 min at 96°C, amplification was carried out for 35 cycles (0.5 min 96°C, 0.5 min 60°C, and 1 min 72°C). Restriction analysis of the PCR products was performed in a 20-μl reaction mixture containing 50 mm Tris-HCl (pH 7.5), 100 mm NaCl, 10 mm MgCl2, 1 mm dithioerythitol, 1 μl of PCR product, and 10 units of restriction endonuclease NdeI. The mixture was incubated overnight at 37°C. The DNA fragments were subsequently separated on a 3% agarose gel and visualized with ethidium bromide.

Sequence Analysis.

Sequence analysis of genomic fragments amplified by PCR was carried out on an Applied Biosystems model 377 automated DNA sequencer using the dye-terminator method.

Clinical Evaluation.

The patient was a female 44 years of age. At the age of 40, she underwent a curative resection of a Dukes B2 moderately differentiated rectum carcinoma and subsequent adjuvant radiotherapy. Three years later, the patient presented with an ileus caused by an intra-abdominal recurrence of the tumor at the right hypochondrium. Debulking of the tumor was performed as well as a partial ileal resection and extirpation of the uterus including the adnexes. No measurable lesions were present after the operation. After a period of 11 months, a palpable mass was present in the right lower abdomen and palliative chemotherapy was started with 5FU (900 mg) and leucovorin (200 mg), which was administered i.v. on a weekly basis. Five days after the first treatment, the patient developed stomatitis. Five days after the second injection with 5FU, the patient suffered from fever, severe stomatis, leucopenia (WBCs, 1.6 × 109/l) and thrombocytopenia (42 × 109/l). The next day, the patient developed a severe pancytopenia for which she received a transfusion with erythrocytes and thrombocytes. Physical examination revealed that the palpable mass in her abdomen had greatly decreased. Despite intensive medical care, the patient died 8 days later because of infectious complications.

Uracil and Thymine Levels in Plasma.

To investigate whether the lethal toxicity after the administration of 5FU might have been caused by a partial or complete deficiency of DPD, plasma was collected for determination of the levels of uracil and thymine. Strongly elevated concentrations of uracil (80 μm; controls, <0.2 μm; n = 20) and thymine (17.5 μm; controls, <0.2 μm; n = 20) were detected in plasma which is indicative of a complete deficiency of DPD.

DPD Activity in PBM Cells and Fibroblasts.

DPD activity was determined in PBM cells isolated from a blood sample obtained during pancytopenia. Morphological examination of the isolated PBM cells on a cytospin preparation showed the presence of only lymphocytes and some residual thrombocytes. Hardly any activity of DPD (0.09 nmol/mg/h) was detected in the PBM cells of the patient when compared with that observed in controls (10.0 ± 3.4 nmol/mg/h; n = 22). Surprisingly, a low but significant activity of DPD (0.56 nmol/mg/h) was detected in thrombocytes when compared with controls (1.7 ± 0.6 nmol/mg/h; n = 22). Because the patient received thrombocyte transfusions, we feel that the very low DPD activity detected in PBM cells of the patient is most likely attributable to contamination of the PBM cell fraction by thrombocytes of the donor. No activity of DPD (<0.009 nmol/mg/h; controls, 0.89 ± 0.56 nmol/mg/h; n = 21) could be detected in cultured fibroblasts established from a skin biopsy of the patient.

Sequence Analysis of the DPD Gene.

To investigate whether or not the common IVS14+1G>A mutation in the DPYD gene might underlie the complete DPD deficiency in the tumor patient, two intron-specific primers were used for amplification of exon 14 and its flanking intron sequences (19). Sequence analysis showed that the tumor patient was homozygous for the IVS14+1G>A mutation, which changes the invariant splice donor site from GT to AT.

RFLP Analysis of the IVS14+1G>A Mutation.

A PCR primer with a single-base mismatch was used, which introduced a NdeI restriction site in case a G→A point mutation is present in the invariant splice donor site of exon 14, to rapidly screen for the IVS14+1G>A mutation by RFLP (Fig. 1). As a positive control for the digestion efficiency of NdeI, an additional NdeI restriction site was introduced in the 5′ region of the PCR fragment using a forward PCR primer containing an A→T mismatch (Table 1). Under these conditions, the undigested PCR fragment has a length of 198 bp. After digestion with NdeI, the wild-type allele will produce two fragments of 181 bp and 17 bp. In contrast, the PCR fragment containing the G→A point mutation in the invariant splice donor site of exon 14 will produce three fragments of 17 bp, 154 bp, and 27 bp after digestion with NdeI. A diagrammatic representation of the PCR amplification of exon 14 and the subsequent analysis of the IVS14+1G>A mutation by RFLP is shown in Fig. 1. The validity of the concept is demonstrated by analysis of the DPYD gene of a patient homozygous for the IVS14+1G>A mutation, an individual who is obligate heterozygous for the IVS14+1G>A mutation and the wild-type DPYD gene from a control (Fig. 2).

Through analysis of 1357 Dutch Caucasians for the presence of the IVS14+1G>A mutation, we identified 24 individuals who were heterozygous for this mutation. Thus, the frequency of hetero zygotes in the Dutch population is 1.8%. No individuals were detected who were homozygous for the IVS14+1G>A mutation, resulting in an allele frequency of 0.91%.

Because 5FU has a relatively narrow therapeutic index, toxicity increases as the dose is increased, resulting in escalated plasma levels of the drug (3, 4). Although the cytotoxic effects of 5FU are probably directly mediated via the anabolic pathways, the catabolic route plays a significant role because >80% of the administered 5FU is catabolized by DPD (5). Thus, the activity of DPD appears to be of critical importance, not only in determining the efficacy of the therapy with 5FU, but also of toxicity (8, 20, 21). On the basis of previous experiences, it has been suggested that patients with a DPD activity <70% of that observed in the normal population might be prone to develop severe 5FU-associated side effects. In addition, the toxicity encountered in patients with a severe deficiency of DPD was significantly higher compared with patients with a moderate DPD deficiency (8). Patients heterozygous for a mutant DPYD allele, and especially patients with a complete deficiency of DPD, are, therefore, at risk. Although a number of tumor patients have been described as suffering from a partial deficiency of DPD (9, 10, 11, 12), the data regarding tumor patients with complete DPD deficiency is scarce (7, 22).

In the present study we have provided unambiguous evidence at the molecular level for homozygosity of a mutated allele of the gene encoding DPD in a tumor patient experiencing lethal toxicity after the administration of 5FU. Analysis of the DPYD gene for the presence of mutations showed that the patient was homozygous for the G→A mutation in the invariant GT splice donor site [IVS14+1G>A]. This mutation leads to the skipping of exon 14 immediately upstream of the mutated splice donor site in the process of DPD pre-mRNA splicing. As a result, the mature DPD mRNA lacks a 165-nt segment encoding the amino acids 581–635 (19). Apparently, the mutant DPD protein lacking the amino acids 581–635 bears no residual activity, because no significant activity of DPD could be measured in PBM cells and fibroblasts of the patient. Persistently increased levels of thymine and uracil in plasma are observed only in cases where the DPD enzyme has been inactivated for >97% of its normal activity (23). Thus, the strongly increased levels of thymine and uracil in the plasma of the patient are in line with the presence of a complete deficiency of DPD.

Recently, we showed that the G→A point mutation in the invariant splice donor site is by far the most common one (52%) among patients with a complete deficiency of DPD (13). Furthermore, there appears to be some kind of homogeneity for the IVS14+1G>A mutation in Northern Europe (13). To date, the frequency of this mutation in the population has not been thoroughly investigated. Screening for the presence of the G→A splice site mutation in only a very limited number of individuals has revealed heterozygosity for this mutation in 1% of the Finnish population (180 alleles analyzed) and none in the British (60 alleles), Japanese (100 alleles), African-American (210 alleles), or Dutch (100 alleles) populations (19, 24). These analyses of the presence of the G→A splice site mutation were performed using RFLP, based on the fact that the G→A point mutation destroys a unique MaeII restriction site, present in the amplified genomic fragment encompassing the skipped exon and its flanking sequences (9, 19). Unfortunately, the restriction enzyme MaeII is rather expensive and thus not suitable for use in screening large numbers of individuals on a routine basis. Recently, a RFLP procedure has been developed for the detection of the IVS14+1G>A mutation using a SnaBI restriction site, which was introduced using PCR-mediated site-directed mutagenesis (25). A serious drawback of this method, however, is the fact that the SnaBI site will not be present in the homozygous-deficient type, whereas no positive control for the cutting efficiency of the restriction enzyme was present. For these reasons, we have developed a novel genotyping test for the IVS14+1G>A mutation. In our test, a NdeI restriction site would be introduced, with PCR-mediated site-directed mutagenesis, in the invariant GT splice donor site in the intron downstream of exon 14, in the event that a G→A point mutation is present. As a positive control for the restriction efficiency of NdeI, a second NdeI restriction site was introduced in the 5′ region of the amplified genomic fragment.

Using this genotyping test for the G→A mutation, we demonstrated that there is a relatively high frequency of the mutated allele in the normal Dutch population, with an allele frequency of 0.91%. Using the Hardy-Weinberg equilibrium and a frequency of heterozygotes of 1.8%, one can estimate the number of individuals homozygous for the G→A mutation to be 1.2 in 10,000. Compared with other frequently occurring inborn errors of metabolism, such as phenylketonuria (1:20,000), the expected prevalence of a DPD deficiency is high. Considering the common use of 5FU in the treatment of cancer patients and the increasing percentage of patients receiving high doses of 5FU in adjuvant therapy, the apparently high prevalence of the IVS14+1G>A mutation in the normal population warrants genetic screening for the presence of this mutation in cancer patients before the administration of 5FU. In this way, the serious and sometimes lethal 5FU-related toxicities encountered in patients heterozygous or homozygous for the IVS14+1G>A mutation might be prevented.

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.

        
1

This work was supported by the “Stichting Kinder Oncologisch Centrum Amsterdam.”

                
3

The abbreviations used are: 5FU, 5-fluorouracil; DPD, dihydropyrimidine dehydrogenase; PBM, peripheral blood mononuclear.

We thank Fiona Ward for critical reading of the manuscript.

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