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Hemoglobin
international journal for hemoglobin research
Volume 41, 2017 - Issue 2
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Original Article

Design, Validation, and Clinical Implementation of a Gap-Polymerase Chain Reaction Method for α-Thalassemia Genotyping Using Capillary Electrophoresis

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Pages 124-130 | Received 06 Jan 2017, Accepted 12 Apr 2017, Published online: 09 Jun 2017
 

Abstract

α-Thalassemia (α-thal) is genetically heterogeneous with most cases caused by variably sized deletions of the HBA1 and/or HBA2 loci. In this report, we describe the development, validation, and implementation of a novel gap-polymerase chain reaction (gap-PCR)/capillary electrophoresis (CE). method. This assay utilizes two multiplex reactions and CE to detect the following deletions: –α3.7 (rightward), –α4.2 (leftward), –(α)20.5, – –SEA (Southeast Asian), – –MED, – –FIL and – –THAI. Validation studies using 36 previously characterized patient samples and plasmid controls demonstrated 100.0% accuracy. Following clinical implementation, 423 patients were analyzed over 24 months. Two hundred and twenty-seven cases (46.0%) showed abnormal results including heterozygous –α3.7 (n = 114, 27.0%), homozygous –α3.7 (n = 96, 23.0%), heterozygous – –SEA (n = 9, 2.0%), heterozygous –α 4.2 (n = 5, 1.0%), heterozygous – –MED (n = 1, <1.0%), and compound heterozygous –α3.7/–α4.2 (n = 2, <1.0%) deletions. Correlation with red blood cell (RBC) parameters showed that patients with a deletion of two or more genes were associated with significantly lower mean corpuscular volume (MCV) and mean corpuscular hemoglobin (Hb) (MCH) levels than patients with wild-type results. This novel multiplex gap-PCR protocol reliably detects the seven most common deletions giving rise to α-thal. Use of the fluorescently labeled CE method provides for a high throughput workflow suitable to a clinical diagnostic laboratory serving a multiethnic population.

Disclosure statement

No potential conflict of interest was reported by the authors.

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