Quantitative polmerase chain reaction for the rapid prenatal diagnosis of homozygous α‐thalassaemia (Hb Barts hydrops fetalis)
A quantitative polymerase chain reaction (Q‐PCR) method based on the TaqMan technology has been devised for the prenatal diagnosis of homozygous α°−thalassaemia (south‐east Asian type deletion). Primers and TaqMan probes were designed to specifically amplify an α°‐thal chromosomal fragment or a norm...
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Published in | British journal of haematology Vol. 115; no. 2; pp. 341 - 346 |
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Main Authors | , , , , , |
Format | Journal Article |
Language | English |
Published |
Oxford, UK
Blackwell Science Ltd
01.11.2001
Blackwell |
Subjects | |
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Abstract | A quantitative polymerase chain reaction (Q‐PCR) method based on the TaqMan technology has been devised for the prenatal diagnosis of homozygous α°−thalassaemia (south‐east Asian type deletion). Primers and TaqMan probes were designed to specifically amplify an α°‐thal chromosomal fragment or a normal α‐chromosomal fragment. Variations in input target DNA in individual sample wells were normalized by the simultaneous amplification of a β‐actin gene fragment and results expressed as a ratio to that of β‐actin. There was no overlap of the data between the homozygous α°‐thal, α°‐thal and normal subjects. Up to 5% maternal DNA (α°‐thal) contamination did not affect the specificity of the result. In 31 prenatal diagnoses, the result using Q‐PCR compared favourably with the gold standard of Southern hybridization of α‐genes. |
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AbstractList | A quantitative polymerase chain reaction (Q‐PCR) method based on the TaqMan technology has been devised for the prenatal diagnosis of homozygous α°−thalassaemia (south‐east Asian type deletion). Primers and TaqMan probes were designed to specifically amplify an α°‐thal chromosomal fragment or a normal α‐chromosomal fragment. Variations in input target DNA in individual sample wells were normalized by the simultaneous amplification of a β‐actin gene fragment and results expressed as a ratio to that of β‐actin. There was no overlap of the data between the homozygous α°‐thal, α°‐thal and normal subjects. Up to 5% maternal DNA (α°‐thal) contamination did not affect the specificity of the result. In 31 prenatal diagnoses, the result using Q‐PCR compared favourably with the gold standard of Southern hybridization of α‐genes. |
Author | Lam, Y. H. Chan, T. K. Wong, H. S. Tse, H. Y. Chan, Vivian Yip, Ben |
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Cites_doi | 10.1001/jama.241.15.1610 10.1111/j.1365-2141.1992.tb08180.x 10.1016/0092-8674(87)90289-3 10.1111/j.1471-0528.1985.tb01447.x 10.1016/0003-2697(90)90108-L 10.1002/(SICI)1097-0223(199706)17:6<505::AID-PD104>3.0.CO;2-R 10.1136/bmj.288.6427.1327 10.1111/j.1399-0004.1995.tb03972.x 10.1046/j.1365-2141.2000.01870.x 10.1126/science.121.3141.372 10.1128/aem.61.10.3724-3728.1995 10.1182/blood.V73.2.372.bloodjournal732372 10.1007/BF00197254 10.1101/gr.6.10.986 10.1182/blood.V78.3.853.853 |
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Keywords | Human Hemoglobinopathy Pregnancy disorders Hemopathy Genetic disease Prenatal Polymerase chain reaction Fetal diseases Hemolytic anemia Hydrops fetalis α-Thalassemia Diagnosis Technique Molecular biology Quantitative analysis |
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References | 1989; 73 1995; 61 1992; 81 1979; 241 1955; 121 1991; 78 1984; 288 1995; 47 2000; 108 1985; 92 1997; 17 1990; 189 1997; 3 1992; 88 1996; 6 1987; 49 e_1_2_6_10_1 Chang J.G. (e_1_2_6_7_1) 1991; 78 e_1_2_6_9_1 e_1_2_6_8_1 Bassler H.A. (e_1_2_6_2_1) 1995; 61 Cai S.P. (e_1_2_6_4_1) 1989; 73 Chan V. (e_1_2_6_5_1) 1997; 3 e_1_2_6_6_1 e_1_2_6_13_1 e_1_2_6_14_1 e_1_2_6_3_1 e_1_2_6_11_1 e_1_2_6_12_1 e_1_2_6_17_1 e_1_2_6_15_1 e_1_2_6_16_1 |
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SubjectTerms | Anemias. Hemoglobinopathies Biological and medical sciences Diseases of red blood cells Hematologic and hematopoietic diseases hydrops fetalis Medical sciences prenatal diagnosis Q‐PCR α°‐thalassaemia |
Title | Quantitative polmerase chain reaction for the rapid prenatal diagnosis of homozygous α‐thalassaemia (Hb Barts hydrops fetalis) |
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