Preimplantation genetic diagnosis for ornithine transcarbamylase deficiency by simultaneous analysis of duplex-nested PCR and fluorescence in situ hybridization: a case report.

Ornithine transcarbamylase (OTC) deficiency is an X-linked co-dominant disorder. A couple, with a previous history of a neonatal death and a therapeutical termination due to OTC deficiency, was referred to our center for preimplantation genetic diagnosis (PGD). The female partner has a nonsense mutation in the exon 9 of the OTC gene (R320X). We carried out nested polymerase chain reaction (PCR) for R320X mutation and fluorescence in situ hybridization (FISH) for aneuploidy screening. Among a total of 11 embryos, two blastomeres per embryo from 9 embryos were biopsied and analyzed by duplex-nested PCR and FISH, and one blastomere per embryo from 2 embryos by only duplex-nested PCR. As a result of PCR and restriction fragment length polymorphism analysis, four embryos were diagnosed as unaffected embryos having the normal OTC gene. Among these embryos, only one embryo was confirmed as euploidy for chromosome X, Y and 18 by FISH analysis. A single normal embryo was transferred to the mother, yielding an unaffected pregnancy and birth of a healthy boy. Based on our results, PCR for mutation loci and FISH for aneuploidy screening with two blastomeres from an embryo could provide higher accuracy for the selection of genetically and chromosomally normal embryos in the PGD for single gene defects.

INTRODUCTION

In the last decade, preimplantation genetic diagnosis (PGD) has become an important alternative to prenatal diagnosis for couples at high risk of transmitting inherited disorders to their children. Fluorescence in situ hybridization (FISH) has been offered for gender selection in X-linked diseases (1, 2), chromosomal translocations (3-5), aneuploidy, and recurrent implantation failure (6, 7). Procedures using polymerase chain reaction (PCR) has been applied for single gene defects including X-linked diseases (8-11).

Ornithine transcarbamylase (OTC; EC 2.1.3.3) is placed in the mitochondrial matrix where it contributes to the detoxification of nitrogenous wastes through the urea cycle, and catalyzes the synthesis of citruline from carbamyl phosphate and ornithine. The OTC gene is located on the short arm of the X chromosome within band Xp21.1 (12). It spans 73 kb, has an open reading frame of 1,062 nucleotides, and contains 10 exons and 9 introns (13, 14). OTC deficiency (MIM-#311250) is an X-linked and co-dominant metabolic disorder with partial penetrance in females (15). The phenotype of OTC deficiency is extremely heterogeneous, ranging from asymptomatic adult hemizygous males to acute neonatal hyperammonemic coma in the first week of affected male babies. Approximately 80% of heterozygous females are asymptomatic and remaining 20% show clinical severity similar to males with partial deficiencies (16, 17). There are more than 341 mutations known to cause OTC deficiency, all of which are specific for the individual families. Mutations have been found in all exons and introns with a relative paucity of mutations in the sequence encoding the leader peptide (exon 1 and a part of exon 2) and in exon 7 (17, 18).

To our knowledge, only two cases have been reported where specific PGD for OTC deficiency were carried out using multiplex or duplex-nested PCR assay and healthy babies devoid of the OTC mutation were born (19, 20). In this study, we describe the successful pregnancy and birth after PGD for OTC deficiency with simultaneous analyses of FISH and duplex-nested PCR in Korea. We have applied a duplex-nested PCR for the amplification of both the causative mutation and the Y chromosome specific Sry gene, and FISH for aneuploidy screening of chromosome X, Y and 18. A healthy boy was born by the transfer of only one unaffected normal embryo.

CASE REPORT

A couple was referred to our center after therapeutic termination of the second pregnancy following prenatal diagnosis for OTC deficiency. In the first pregnancy, a male baby was born but died at 10 days after birth due to liver dysfunction accompanying hyperammonemia. Molecular genetic analysis of the couple's OTC gene was performed by PCR and direct sequencing at Seoul Asan Hospital and revealed a single base substitution (R320X) in the exon 9 of the female partner. In the second pregnancy, the fetus was identified to be an affected boy by PCR and direct sequencing on a chorionic villus sample, and the pregnancy was therapeutically terminated. In order to avoid a pregnancy with an affected baby, the couple was counseled for PGD in Cheil General Hospital.

In order to determine the efficiency of single cell PCR and allele drop-out (ADO) rate, primers used for the detection of the causative mutation and Y chromosome specific Sry gene were tested using single lymphocytes (Table 1). Ovarian stimulation, in vitro fertilization, and blastomere biopsy were done as previously described (4, 5). After the blastomere biopsy procedure, the embryos were washed several times and transferred to the G2.2 medium (Vitrolife Sweden AB, Kungsbacka, Sweden). Each blastomere was washed twice through two drops of G2.2 medium and transferred into sterile 0.2 mL PCR tubes containing 5 µL of alkaline lysis buffer. For each embryo biopsied, blank negative controls were prepared from the wash drops. The nested-duplex PCR analysis was performed by previously described protocol (6). Mutation analysis by restriction fragment length polynorphism (RFLP) with BclI restriction enzyme was carried out only for positively amplified PCR products of blastomeres. Another blastomere from the same embryo was prepared for FISH. The FISH analysis for chromosome X, Y and 18 was done as previously described and the manufacture's protocol (4, 5). The embryos were cultured under standard culture condition until the diagnosis was established. The embryos with the normal genotype were selected and transferred on day 4 after fertilization. Amniocentesis was performed at 16 weeks of gestation to confirm the results of PGD. Postnatal genetic and physiological diagnosis was also conducted.

Table 1

Sequences of oligonucleotide primers and PCR conditions for duplex-nested PCR for OTC deficiency

PCR, polymerase chain reaction; OTC, ornithine transcarbamylase.

All 10 exons and exon-intron boundaries of the OTC gene were screened by PCR followed by direct DNA sequencing analysis. The heterozygous OTC gene with R320X nonsense mutation (CGA→TGA) and wild type was detected in the exon 9 of the female partner by RFLP (Fig. 1) and direct sequencing (data not shown). This R320X nonsense mutation was associated with acute neonatal hyperammonemia in their first pregnancy and reduced enzyme activity by 10-15% (21). Male partner has a normal OTC gene.

Fig. 1

Identification of the maternal mutation (heterozygote type) in exon 9 of the OTC gene. After digesting the PCR product with BclI, the 319 or 218 bp PCR products of the affected mother were digested into 223 and 96 bp (lane 1) and 178 and 40 bp products (lane 4), respectively. The 40 bp product was hardly seen on an agarose gel. Lane 1 and 4; the first and nested PCR products of the affected mother, respectively, lane 2 and 3; BclI-digested products from the first PCR products of the father. M: molecular weight marker.

The efficiency and accuracy of the duplex-nested PCR analysis were tested on single lymphocytes from the heterozygous female partner and normal male partner. PCR on single lymphocytes resulted in 90.6% (58/64) amplification rate, whereas none of the negative controls showed a positive band. ADO was detected in 4 out of 30 lymphocytes (13.3%).

After ovarian hyperstimulation, a total of 18 oocytes were retrieved and 17 oocytes were injected using intracytoplasmic sperm injection in order to prevent DNA contamination from inseminated sperm. Among a total of 11 embryos, two blastomeres per embryo from 9 embryos were biopsied and simultaneously analyzed by duplex-nested PCR and FISH, and one blastomere per embryo from 2 embryos by only duplex-nested PCR. As a result of duplex-nested PCR and RFLP analysis with the BclI restriction enzyme, ten showed successful amplification for the exon 9 of the OTC gene, and the amplification rate was 90.9%, almost same as that of the single lymphocyte test. There were two unaffected males, five affected males, two unaffected females, and one heterozygous female (Fig. 2 and Table 2). No amplification was detected in any of the negative controls. On the other hand, out of nine blastomeres analyzed by FISH, only six blastomeres were identified as chromosomally normal embryos (Fig. 3, Table 2). However, among total four unaffected embryos (embryo 1, 2, 3, and 8) diagnosed by PCR, only two embryos (embryo 3 and 8) were identified as chromosomally normal by FISH. The other two embryos (embryo 1 and 2) were shown to have trisomy 18 and monosomy 18, respectively. Only one male embryo (embryo 8) was transferred, and another female unaffected embryo (embryo 3) was cryopreserved at blastocyst stage on day 5 after fertilization. This PGD cycle resulted in a singleton pregnancy and the genotype of the fetus was confirmed to be a normal male by amniocentesis at 16 weeks of gestation. A healthy boy of 2.8 kg was delivered at 36 weeks. The genotype of the baby for the exon 9 of OTC gene and level of ammonia were confirmed as normal.

Fig. 2

Results of agarose gel electrophoresis of the restriction fragment length polymorphism (RFLP) analysis with BclI restriction enzyme in the preimplantation genetic diagnosis for ornithine transcarbamylase deficiency. In normal embryos (No. 1, 2, 3 and 8), the 218-bp PCR products were not digested with BclI.

Table 2

Summary of the results of the PGD for OTC deficiency with simultaneous analysis of duplex nested PCR and FISH

Plus (+) and minus (-) signs indicate whether a band was detected corresponding to the Sry gene. N.A. (not assayed) indicates that blastomere was not available for FISH. In the table, transferred embryo is presented with bold and italic characters.

PGD, preimplantation genetic diagnosis; OTC, ornithine transcarbamylase; PCR, polymerase chain reaction; FISH, fluorescence in situ hybridization.

Fig. 3

Results of the fluorescence in situ hybridization (FISH) analysis on the embryos diagnosed to be normal by PCR in the PGD for OTC deficiency. Panels A-D show the photographs for the results of FISH on the embryos No. 1, 2, 3, and 8 in Table II, respectively. Aqua, green and orange signals indicate the presence of the chromosome X, Y and 18 in the nucleus of the blastomeres, respectively.

PGD, preimplantation genetic diagnosis; OTC, ornithine transcarbamylase; PCR, polymerase chain reaction

DISCUSSION

Most PGD cycles for X-linked disorders such as Duchenne muscular dystrophy and fragile X syndrome involved the selection of female embryos which were diagnosed as normal or heterozygous. These gender selections were supported by couples at risk of X-linked recessive conditions. However, OTC deficiency is an X-linked and co-dominant disorder. Some heterozygous females represent severe phenotypic abnormalities such as nausea, vomiting and ataxia. ADO for affected allele could lead to yielding an affected heterozygous baby, even if the female embryo was diagnosed as normal by PGD for OTC deficiency. Gender selection with FISH for Y chromosome-specific loci is more reliable because amplification failure could occasionally occur in single cell PCR. Thus, our protocol with PCR and FISH in this study provides higher accuracy for the selection of genetically and chromosomally normal embryos in the PGD for X-linked co-dominant defects.

We applied duplex-nested PCR and FISH analysis in two blastomeres from each embryo, which were more than 6-cell stage. Biopsy of more than a quarter of blastomeres from each embryo could interfere with developmental potential of embryos. Thus, single blastomere biopsy was applied to less than 6-cell stage embryos in this study. Sequential PCR and FISH analysis in one blastomere (cell recycling) was reported and could be used to detect the aneuploidy, but the rate of ADO after PCR seems to be higher using this method (22, 23). Therefore, we carried out two methods separately on two blastomeres. A duplex-nested PCR analysis was developed for the simultaneous diagnosis of a R320X mutation and a gender selection, and FISH analysis was used to detect aneuploidy for chromosome X, Y and 18. As a result of duplex nested PCR and FISH analysis, concordant results have been obtained from two blastomeres at the sex locus, and the amplification efficiency was 100% (9/9 except two blastomeres, that were not analyzed by FISH analysis) for Sry. And the amplification rate was 90.9% (10/11) for exon 9 of the OTC gene.

Several strategies have been developed to decrease amplification failure and ADO in single cell analysis of PGD. These included the development of sequential first and second polar body analysis (24), improvement of the PCR condition by increasing the denaturation temperature and time (19), using a more powerful lysis method (25-28) and the use of fluorescent PCR for mutations or linked markers and multiplex PCR (29-32). As mentioned above, we have also endeavored to optimize single cell PCR conditions, which included longer initial denaturation time, higher denaturation temperature, and the selection of Taq polymerase, the concentration of MgCl2, and lysis methods. The incidence of ADO was 5-15% in many PGD laboratories (27, 28). At a preliminary experiment on single lymphocytes in this study, the ADO rate for exon 9 of the OTC gene was about 13.0% when using duplex-nested PCR. We could not absolutely exclude the possibility of ADO in the diagnosis of unaffected female embryo owing to the relatively higher ADO. Thus, FISH was simultaneously applied for the aneuploidy screening and sex selection to prevent the pregnancy of heterozygous female.

In this study, we report the successful PGD and delivery of a healthy boy in a couple at risk of transmitting the OTC deficiency. This was carried out by the simultaneous analysis of the duplex-nested PCR for a R320X mutation in the OTC gene underlying the OTC deficiency and Y chromosome-specific loci, and FISH for aneuploidy screening of chromosome X, Y and 18. This strategy could provide higher accuracy for the selection of genetically and chromosomally normal embryos in PGD for single gene defects.