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Rapid ABO Genotyping Using Whole Blood without DNA Purification

Authors
Lee, Sung HoPark, GeonYang, Young GeunLee, Seung GwanKim, Suhng Wook
Issue Date
6월-2009
Publisher
KOREAN SOC LABORATORY MEDICINE
Keywords
ABO genotyping; Whole blood; Allele-specific polymerase chain reaction
Citation
KOREAN JOURNAL OF LABORATORY MEDICINE, v.29, no.3, pp.231 - 237
Indexed
SCIE
SCOPUS
KCI
Journal Title
KOREAN JOURNAL OF LABORATORY MEDICINE
Volume
29
Number
3
Start Page
231
End Page
237
URI
https://scholar.korea.ac.kr/handle/2021.sw.korea/119913
DOI
10.3343/kjlm.2009.29.3.231
ISSN
1598-6535
Abstract
Background: ABO genotyping is commonly used in cases of an ABO discrepancy between cell typing and serum typing, as well as in forensic practice for personal identification and paternity testing, We evaluated ABO genotyping via multiplex allele-specific PCR (ASPCR) amplification using whole blood samples without DNA purification. Methods: A four-reaction multiplex ASPCR genotyping assay was designed to detect specific nucleotide sequence differences between the six ABO alleles A101, A102, B101, O01, O02, and cis-AB01. The ABO genotypes of 127 randomly chosen samples were determined using the new multiplex ASPCR method. Results: The genotypes of the 127 samples were found to be A101/A102(n=1), A102/A102(n=9), A101/O01 (n=3), A102/O01 (n=12), A102/O02 (n=14), B101/B101 (n=5), B101/O01 (n=18), B101/O02 (n=15), O01/O01 (n=14), O02/O02 (n=8), O01/O02 (n=14) and A102/B101 (n=14), from which phenotypes were calculated to be A (n=39), B (n=38), O (n=36) and AB (n=14). The multiplex ASPCR assay results were compared with the serologically determined blood group phenotypes and genotypes determined by DNA sequencing, and there were no discrepancies. Conclusions : This convenient multiplex ASPCR assay, performed using whole blood samples, provides a supplement to routine serological ABO typing and might also be useful in other genotyping applications. (Korean J Lib Med 2009,29:231-7)
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보건과학대학 (보건환경융합과학부)
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