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 inBritish journal of haematology Vol. 115; no. 2; pp. 341 - 346
Main Authors Chan, Vivian, Yip, Ben, Lam, Y. H., Tse, H. Y., Wong, H. S., Chan, T. K.
Format Journal Article
LanguageEnglish
Published Oxford, UK Blackwell Science Ltd 01.11.2001
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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.
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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  surname: Wong
  fullname: Wong, H. S.
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  givenname: T. K.
  surname: Chan
  fullname: Chan, T. K.
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Issue 2
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
Language English
License CC BY 4.0
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Blackwell
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Snippet A quantitative polymerase chain reaction (Q‐PCR) method based on the TaqMan technology has been devised for the prenatal diagnosis of homozygous...
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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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