Your search keyword '"Blastomeres metabolism"' showing total 3 results

1. [Preimplantation genetic diagnosis of Duchenne muscular dystrophy by single cell triplex PCR].

Author

Wu YL, Wu LQ, Li YP, Liu DE, Zeng Q, Zhu HY, Pan Q, Liang DS, Hu H, Long ZG, Li J, Dai HP, Xia K, and Xia JH

Subjects

Blastomeres cytology, Blastomeres metabolism, Chromosomes, Human, X genetics, Chromosomes, Human, Y genetics, Cytogenetic Analysis methods, Exons genetics, Female, Gene Deletion, Humans, Lymphocytes cytology, Lymphocytes metabolism, Male, Muscular Dystrophy, Duchenne blood, Muscular Dystrophy, Duchenne genetics, Pregnancy, Amelogenin genetics, Muscular Dystrophy, Duchenne diagnosis, Polymerase Chain Reaction methods, Preimplantation Diagnosis methods

Abstract

Objective: To detect two exons of Duchenne muscular dystrophy (DMD) gene and a gender discrimination locus amelogenin gene by single cell triplex PCR, and to evaluate the possibility of this technique for preimplantation genetic diagnosis (PGD) in DMD family with DMD deletion mutation., Methods: Single lymphocytes from a normal male, a normal female, two DMD patients (exon 8 and 47 deleted, respectively) and single blastomeres from the couples treated by the in vitro fertilization pre-embryo transfer (IVF-ET) and without family history of DMD were obtained. Exons 8 and 47 of DMD gene were amplified by a triplex PCR assay, the amelogenin gene on X and Y chromosomes were co-amplified to analyze the correlation between embryo gender and deletion status., Results: In the normal single lymphocytes, the amplification rate of exons 8 and 47 of DMD and amelogenin gene were 93.8%, 93.8%, and 95.3% respectively. The false positive rate was 3.3%. In the exon 8 deleted DMD patient, the amplification rate of exon 47 of DMD and amelogenin gene was 95.8%, and the false positive rate was 3.3%. In the exon 47 deleted DMD patient, the amplification rate of exon 8 of DMD and amelogenin gene was 95.8%, and the false positive rate was 0. In the single blastomeres, the amplification rate of exons 8 and 47 of DMD and amelogenin gene was 82.5%, 80.0% and 77.5%, respectively, and the false positive rate was 0., Conclusion: The single cell triplex PCR protocol for the detection of DMD and amelogenin gene is highly sensitive, specific and reliable, and can be used for PGD in those DMD families with DMD deletion mutation.

Published

2007

2. [HLA-A site genotyping on single blastomeres is studied by nest-PCR-SSP method].

Author

Xu BS, Hu YW, Huang XF, Lin JJ, Zhou Y, Ye BL, Xu LX, Xu KP, and Yang HM

Subjects

Base Sequence, DNA analysis, DNA Fingerprinting methods, DNA Mutational Analysis, Female, HLA Antigens analysis, HLA-A Antigens analysis, Histocompatibility Antigens Class I analysis, Histocompatibility Antigens Class I genetics, Humans, Male, Single Person, Blastomeres metabolism, HLA-A Antigens genetics, Polymerase Chain Reaction methods

Abstract

Objective: To assess the accuracy and reliability of the nest-PCR-sequence specific primer(SSP) method in HLA-A site genotyping of single blastomeres retrieved from human pre-implantation embryos., Methods: By nest PCR on HLA-A exon 2, the success rate of first-round amplification was estimated for single blastomeres. Based on the first-round amplification, the HLA-A genotype of every single blastomeres was analyzed by commercially available PCR-SSP kits., Results: The amplification of HLA-A exon 2 were performed to 120 blasotmeres retrieved from in vitro fertilization(IVF) surplus embryos donated by 10 couples. The average success rate of family 1-5 and 6-10 was 78.2%(43/55) and 93.8%(61/65), respectively. And 86.7%(104/120) in total. Eighty blastomeres were further tested by nest-PCR-SSP, among which 11 blastomeres failed to HLA-A exon 2 amplification and then failed to genotyping while the other 69 blastomeres succeed in HLA-A exon 2 amplification and succeed in genotyping. Except for 6 blastomeres that were uncertain for allele lost because of parents' homozygosity, the left 63 blastomeres had accurate HLA genotyping. Among these 63 blastomeres, 59 blastomeres had genotypes confirmed from their parents(93.6%), 3 blastomeres lost one of parents' alleles(4.8%), and only one blastomere had two more than parents' alleles(1.6%)., Conclusion: The above research results indicated that based on the successful first round amplification of single blastomeres, nest-PCR-SSP strategy offers a convenient and reliable option for HLA genotyping on single blastomeres, which is a key process in pre-selecting HLA-identical sibling for allogeneic cord blood cell transplantation.

Published

2006

3. [Sex determination of human preimplantation embryo using nested polymerase chain reaction].

Author

Jiao ZX, Zhuang GL, Zhou CQ, Zhang MF, and Li LL

Subjects

Amelogenin, Blastocyst cytology, Blastomeres cytology, Blastomeres metabolism, DNA genetics, Dental Enamel Proteins genetics, Female, Genotype, Humans, Lymphocytes cytology, Lymphocytes metabolism, Male, Polymerase Chain Reaction methods, Blastocyst metabolism, Sex Determination Analysis methods

Abstract

Objective: Using nested polymerase chain reaction (PCR) to perform preimplantation gender diagnosis., Methods: One (or two) lymphocyte and blastomere (n=50/group) were collected and prepared under the following conditions: (1) water only (H(2)O); (2) freeze-thaw liquid nitrogen, then boiling; (3) potassium hydroxide/dithiotheriol, heated to 65 degree centigrade, followed by acid neutralization (KOH). Cells were analyzed by PCR using nested primers amplification with amelogenin gene., Results: The amplification rate and allele dropout (ADO) rate for male lymphocytes by the three methods were 83%, 94%, 95% and 24%, 12%, 4%, respectively. Using two cells per reaction did not increase the amplification rate for the KOH method., Conclusion: The KOH method for DNA preparation is superior to the other methods evaluated. Dual blastomere biopsy and independent blastomere analysis may improve preimplantation diagnostic reliability.

Published

2003