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Journal of the Medical Association of Thailand = Chotmaihet thangphaet 2010-Nov

Analysis of real-time PCR cycle threshold of alpha-thalassemia-1 Southeast Asian type deletion using fetal cell-free DNA in maternal plasma for noninvasive prenatal diagnosis of Bart's hydrops fetalis.

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Sakorn Pornprasert
Kanyakan Sukunthamala
Naowarat Kunyanone
Sririchai Sittiprasert
Khanungnit Thungkham
Sumeth Junorse
Khachonsilp Pongsawatkul
Wisut Pattanaporn
Chantip Jitwong
Torpong Sanguansermsri

Palabras clave

Abstracto

BACKGROUND

Noninvasive prenatal diagnosis based on detection of fetal cell-free DNA is hampered when mother and father are both carriers for the same autosomal recessive mutation.

OBJECTIVE

To compare the diagnosis of Bart's hydrops fetalis using conventional Gap-PCR analysis of fetal cells/tissues with the measurement of quantitative difference (deltaCp) between alpha-thalassemia-1 SEA type deletion gene (C(T-mutant)) and wild type alpha-globin gene (C(T-wild type)) in plasma of pregnancies by using the Taqman real-time quantitative PCR.

METHODS

Plasma DNA samples were collected from three groups of pregnancies whose fetuses have known thalasemia status (7 normal, 11 heterozygote alpha-thalassemia-1 SEA type deletion, and 7 Bart's hydrops fetalis). The alpha-thalassemia-1 SEA type deletion gene and wild type alpha-globin gene were quantified by using Taqman real-time quantitative PCR and then the delta C(T) was analyzed by subtracting the C(T-mutant) from C(T-wild type).

RESULTS

Mean deltaC(T) values were not significantly different among the three groups. However, women whose fetuses were diagnosed as Bart's hydrops fetalis had a higher proportion (43%) of plasma DNA samples that had negative deltaC(T) value than women whose fetuses were diagnosed as normal or heterozygote alpha-thalassemia-1 SEA type deletion (0 and 27%, respectively).

CONCLUSIONS

Further investigations are needed to improve the diagnosis of Bart's hydrops fetalis using fetal cell-free DNA.

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