Your search keyword '"Chunming Ding"' showing total 3 results

1. Detection of the placental epigenetic signature of the maspin gene in maternal plasma.

Author

Chim, Stephen S. C., Tong, Yu K., Chiu, Rossa W. K., Lau, Tze K., Leung, Tse N., Chan, Lisa Y. S., Oudejans, Cees B. M., Chunming Ding, and Dennis Lo, Y. M.

Subjects

GENETIC polymorphisms, CORD blood, BLOOD cells, PREGNANT women, POLYMORPHISM (Zoology), GENETIC markers

Abstract

The discovery of fetal DNA in the plasma of pregnant women has opened up new approaches for noninvasive prenatal diagnosis and monitoring. Up to now, the lack of a fetal DNA marker that can be universally detected in maternal plasma has limited the clinical application of this technology. We hypothesized that epigenetic differences between the placenta and maternal blood cells could be used for developing such a marker. By using bisulfite DNA sequencing. the methylation status of the maspin gene promoter in placental tissues and paired maternal blood cells from pregnant women was analyzed. The maspin gene promoter was found to be hypomethylated in placental tissues and densely methylated in maternal blood cells. Genotyping of a single nucleotide polymorphism within the unmethylated maspin sequences in maternal plasma demonstrated that these sequences were derived from the fetus. By using real-time quantitative methylation-specific PCR, unmethylated maspin sequences were detected in maternal plasma in all three trimesters of pregnancy and were cleared within 24 h after delivery. The maternal plasma concentration of unmethylated maspin sequences was elevated by a median of 5.7 times in preeclamptic pregnancies compared with nonpreeclamptic pregnancies. 1-lypomethylated maspin DNA is the first universal marker for fetal DNA in maternal plasma, thus allowing the measurement of fetal DNA concentrations in pregnancy-associated disorders, irrespective of fetal gender and genetic polymorphisms. Differential DNA methylation between the placenta and maternal blood cells may be exploited to develop further markers for noninvasive prenatal assessment. [ABSTRACT FROM AUTHOR]

Published

2005

2. MS analysis of single-nucleotide differences in circulating nucleic acids: Application to noninvasive prenatal diagnosis.

Author

Chunming Ding, Chiu, Rossa W. K., Lau, Tze K., Leung, Tse N., Chan, Li C., Chan, Amy Y. Y., Charoenkwan, Pimlak, Ngi, Ivy S. L., Hai-yang Law, Ma, Edmond S. K., Xiangmin Xu, Chanane Wanapirak, Torpong Sanguansermsri, Can Liao, Mary Anne Tan Jin Ai, Chui, David H. K., Cantor, Charles R., and Dennis, Y. M.

Subjects

*PREGNANCY, *NUCLEOTIDES, *DNA, *NUCLEIC acids, *ONCOLOGY, *PROTEINS

Abstract

The analysis of circulating nucleic acids has revealed applications in the noninvasive diagnosis, monitoring, and prognostication of many clinical conditions. Circulating fetal-specific sequences have been detected and constitute a fraction of the total DNA in maternal plasma. The diagnostic reliability of circulating DNA analysis depends on the fractional concentration of the targeted sequence, the analytical sensitivity, and the specificity. The robust discrimination of single-nucleotide differences between circulating DNA species is technically challenging and demands the adoption of highly sensitive and specific analytical systems. We have developed a method based on single-allele base extension reaction and MS, which allows for the reliable detection of fetal-specific alleles, including point mutations and single-nucleotide polymorphisms, in maternal plasma. The approach was applied to exclude the fetal inheritance of the four most common Southeast Asian β-thalassemia mutations in at-risk pregnancies between weeks 7 and 21 of gestation. Fetal genotypes were correctly predicted in all cases studied. Fetal haplotype analysis based on a single-nucleotide polymorphism linked to the β-globin locus, HBB, in maternal plasma also was achieved. Consequently, noninvasive prenatal diagnosis in a mother and father carrying identical β-thalassemia mutations was accomplished. These advances will help in catalyzing the clinical applications of fetal nucleic acids in maternal plasma. This analytical approach also will have implications for many other applications of circulating nucleic acids in areas such as oncology and transplantation. [ABSTRACT FROM AUTHOR]

Published

2004

3. Direct molecular haplotyping of long-range genomic DNA with M1-PCR.

Author

Chunming Ding and Cantor, Charles R.

Subjects

*DNA, *GENETIC polymorphisms

Abstract

Haplotypes, combinations of several phase-determined polymorphic markers, are extremely valuable for studies of disease association and chromosome evolution. Here we describe a technique called M1-PCR (M for "multiplex" and 1 for "single-copy DNA molecules") that enables direct molecular haplotyping of several polymorphic markers separated by as many as 24 kb. A genomic DNA sample first is diluted to approximately single-copy. The haplotype is directly determined by simultaneously genotyping several polymorphic markers in the same reaction with a multiplex PCR and base extension reaction. This approach does not rely on pedigree data and does not require previous amplification of the entire genomic region containing the selected markers. [ABSTRACT FROM AUTHOR]

Published

2003