Noninvasive prenatal testing of beta-thalassemia for common Pakistani mutations: a comparative study using cell-free fetal DNA from maternal plasma and chorionic villus sampling

Muhammad Afzal; Muhammad Abdul Naeem; Suhaib Ahmed; Nayyar Amin; Amena Rahim; Manazza Munawar; Mansoor Ishaq; Ali Rathore; K Maria

doi:10.1080/16078454.2022.2045052

Noninvasive prenatal testing of beta-thalassemia for common Pakistani mutations: a comparative study using cell-free fetal DNA from maternal plasma and chorionic villus sampling

Hematology. 2022 Dec;27(1):353-359. doi: 10.1080/16078454.2022.2045052.

Authors

Muhammad Afzal¹, Muhammad Abdul Naeem², Suhaib Ahmed¹, Nayyar Amin², Amena Rahim¹, Manazza Munawar¹, Mansoor Ishaq², Ali Rathore², K Maria²

Affiliations

¹ Biochemistry, Riphah International University Islamabad, Rawalpindi, Pakistan.
² Hematology, Armed Forces Institute of Transfusion, Rawalpindi, Pakistan.

PMID: 35287566
DOI: 10.1080/16078454.2022.2045052

Abstract

Background: The discovery of circulating cell-free fetal DNA (cff-DNA) in maternal plasma has inspired the noninvasive prenatal testing (NIPT) approaches for various genetic fetal screening including rhesus D typing, sex determination, aneuploidies, and single-gene disorders.

Objective: Noninvasive determination of paternally inherited beta-thalassemia mutations in maternal total cell-free DNA (cf-DNA) by using allele-specific amplification refractory mutation system (ARMS) real-time PCR (RT-PCR) in concordance with the conventional invasive method.

Methods: An observational study was conducted at the Armed Forces Institute of Blood Transfusion in collaboration with the genetics resource center from March 2021 to August 2021. A total number of 26 couples were selected having a history of previously affected children with beta-thalassemia. A routine chorionic villus sampling (CVS) invasive procedure was carried out, and the mutation analysis was done using conventional PCR. To assess NIPT, a total cf-DNA was also extracted from maternal plasma and analyzed using allele-specific ARMS RT-PCR.

Results: Based on conventional PCR testing, 13 of 26 couples were found having beta-thalassemia carriers with homozygous mutation, and 13 couples were carriers with heterozygous mutations. Further to assess NIPT, the cf-DNA of 13 pregnant females among the couples with different mutational patterns was analyzed by allele-specific ARMS RT-PCR to detect paternally inherited mutations. In comparison with conventional PCR, 11 cases (84.6%) were matched successfully, while two cases (15.4%) had no concordance with conventional invasive prenatal testing (IPT).

Conclusion: NIPT using maternal cf-DNA by allele-specific ARMS RT-PCR can be feasible to screen paternal inherited mutant alleles to rule out pregnant women from invasive procedures where the test would be negative for paternal inheritance. However, a low amount of fetal DNA in maternal plasma is a limiting factor and required further improvement to enrich fetal cf-DNA for complete concordance with conventional IPT.

Keywords: NIPT; beta-thalassemia; cff-DNA; maternal plasma; paternal inheritance.

Publication types

Observational Study

MeSH terms

Cell-Free Nucleic Acids* / genetics
Chorionic Villi Sampling
DNA
Female
Humans
Mutation
Noninvasive Prenatal Testing*
Pakistan
Pregnancy
Real-Time Polymerase Chain Reaction
beta-Thalassemia* / diagnosis
beta-Thalassemia* / genetics

Substances

Cell-Free Nucleic Acids
DNA