β-Globin mutation detection by tagged single-base extension and hybridization to universal glass and flow-through microarrays

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Abstract

To test the feasibility of developing a diagnostic microarray for a specific disease, we selected all pathogenic changes of the β -globin gene occurring at a frequency ≥1% in the multi-ethnic Dutch population for analysis. A tagged single-base extension (SBE) approach was used to detect 19 different mutations causing β-thalassemia or abnormal hemoglobins. In the SBE reaction, the primers were elongated at the 3′ site with a fluorescently labeled dideoxyribonucleotide triphosphate (ddNTP) complementary to the mutation, following tag hybridization to a glass or flow-through microarray. We compared the performance of a generic glass array and a porous system, by testing each mutation separately using heterozygous carriers and by screening a cohort of 40 unknown β-thalassemia carriers and patients. The results were verified by direct sequencing. The microarray system was able to detect 17 β-globin mutations simultaneously with >95% accuracy in a single SBE reaction. The flow-through array performed slightly better (96%), but the main advantages of the system included real-time data recording and a considerable time saving achieved through a reduced hybridization time. © 2004 Nature Publishing Group All rights reserved.

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van Moorsel, C. H. M., van Wijngaarden, E. E., Fokkema, I. F. A. C., den Dunnen, J. T., Roos, D., van Zwieten, R., … Harteveld, C. L. (2004). β-Globin mutation detection by tagged single-base extension and hybridization to universal glass and flow-through microarrays. European Journal of Human Genetics, 12(7), 567–573. https://doi.org/10.1038/sj.ejhg.5201192

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