๐”– Bobbio Scriptorium
โœฆ   LIBER   โœฆ

A rapid and reliable PCR method for genotyping the ABO blood group

โœ Scribed by Denise S. O'Keefe; Alexander Dobrovic

Publisher
John Wiley and Sons
Year
1993
Tongue
English
Weight
310 KB
Volume
2
Category
Article
ISSN
1059-7794

No coin nor oath required. For personal study only.

โœฆ Synopsis

The ABO blood group has been used extensively as a marker in population studies, epidemiology, and forensic work. However, until the cloning of the gene, it was not possible to determine the genotype of group A and B individuals without recourse to family studies. We have developed a method to determine the ABO genotype directly from human DNA using multiplex PCR and restriction enzyme analysis. Two PCR fragments spanning positions 258 and 700 of the cDNA sequence are amplified.

The site at position 258 allows us to differentiate the 0 allele from the A and B alleles. The site at position 700 allows us to distinguish the B allele from the A and 0 alleles. Analysis at the two sites thus allows us to distinguish the three alleles. The multiplex PCR product is digested separately with four enzymes, two for each of the sites. The pair of enzymes for each site cut in a reciprocal fashion. Whereas one enzyme for each site is theoretically sufficient for genotyping, the use of complementary pairs of enzymes prevents the assignment of a false genotype as a result of false negative or partial digestion. This method is fast and reliable, does not rely on probing of blots, and should be widely applicable.

๐Ÿ“œ SIMILAR VOLUMES

A rapid and reliable PCR method for geno
A rapid and reliable PCR method for genotyping the ABO blood group. II: A2 and O2 alleles
โœ Denise S. O'Keefe; Alexander Dobrovic ๐Ÿ“‚ Article ๐Ÿ“… 1996 ๐Ÿ› John Wiley and Sons ๐ŸŒ English โš– 470 KB ๐Ÿ‘ 1 views

## Communicated by Henrik Dahl PCR permits direct genotyping of individuals at the ABO locus. Several methods have been reported for genotyping ABO that rely on differentiating the A, B, and 0 alleles at specific base substitutions. However, the 0 allele as defined by serology comprises at least t

Real-time PCR for single-cell genotyping
Real-time PCR for single-cell genotyping in sickle cell and thalassemia syndromes as a rapid, accurate, reliable, and widely applicable protocol for preimplantation genetic diagnosis
โœ Christina Vrettou; Joanne Traeger-Synodinos; Maria Tzetis; Giles Palmer; Christa ๐Ÿ“‚ Article ๐Ÿ“… 2004 ๐Ÿ› John Wiley and Sons ๐ŸŒ English โš– 213 KB ๐Ÿ‘ 1 views

## Communicated by Stylianos Antonarakis Sickle-cell and b-thalassemia syndromes are priority genetic diseases for prevention programs involving population screening with the option of prenatal diagnosis for carrier couples. Preimplantation genetic diagnosis (PGD) represents a specialized alternat

A rapid, reliable, and inexpensive metho
A rapid, reliable, and inexpensive method for detection of di- and trinucleotide repeat markers and disease loci from dried blood spots
โœ Holden, Jeanette J. A.; Chalifoux, Maryse; Wing, Maggie; Julien-Inalsingh, Colin ๐Ÿ“‚ Article ๐Ÿ“… 1996 ๐Ÿ› John Wiley and Sons ๐ŸŒ English โš– 564 KB

We used a rapid and inexpensive method for studying the FMRl CGG-repeat from dried blood spots, prepared from heel pricks, finger pricks, or an aliquot of blood from a venipuncture. The procedure includes a single tube for preparation of template DNA for PCR and minimal handling, avoiding opportunit