1997
DOI: 10.1046/j.1423-0410.1997.7230192.x
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Simultaneous Genotyping of Human Platelet Antigens by Hot Start Sequence‐Specific Polymerase Chain Reaction with DNA Polymerase AmpliTaq Gold

Abstract: Using our hot start PCR-SSP procedure with AmpliTaq Gold a simple, rapid and reproducible genotyping for HPA-1, 2, 3 and S systems could be achieved.

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Cited by 26 publications
(8 citation statements)
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“…To this end, we determined the phenotype and allele frequencies for those systems in 33 German patients with chronic refractory AITP, and compared them with the data obtained from 80 healthy German blood donors. Allele frequencies from the controls agreed with published data [14]. Further, the allele frequencies of the HPA–1, –3, and –5 systems in the chronic refractory AITP patients were similar to the allele frequencies in controls indicating lack of association between alleles of the HPA–1, –3, and –5 systems and the development of chronic refractory AITP.…”
Section: Discussionsupporting
confidence: 85%
“…To this end, we determined the phenotype and allele frequencies for those systems in 33 German patients with chronic refractory AITP, and compared them with the data obtained from 80 healthy German blood donors. Allele frequencies from the controls agreed with published data [14]. Further, the allele frequencies of the HPA–1, –3, and –5 systems in the chronic refractory AITP patients were similar to the allele frequencies in controls indicating lack of association between alleles of the HPA–1, –3, and –5 systems and the development of chronic refractory AITP.…”
Section: Discussionsupporting
confidence: 85%
“…In the past, HPA typing has been performed mostly by serological methods. Because of severe limitations of these methods, they have been replaced with rapid molecular methods such as polymerase chain reaction‐sequence specific primers (PCR‐SSP) (10–13) or PCR with restriction fragment length polymorphism (PCR‐RFLP) (14).…”
Section: Sequences Of Specific Primers Used For Human Platelet Antigementioning
confidence: 99%
“…Two primers which amplify a region of the C‐reactive protein (CRP) gene were used as an internal control in each amplification mixture. Genotyping of HPA systems was performed according to a previously published protocol with slight modifications in order to perform simultaneous determination of all HPA alleles (Chen et al , 1997). Briefly, the PCR mixture (20 μL) contained 1 × 10 × PCR buffer II, 0·5 U Amply Taq Gold, 0·2 mmol L −1 of each dNTP, 1·5 mmol L −1 MgCl 2 , 0·5 μmol L −1 of each specific primer, 0·05 μmol L −1 of the internal control primer (to amplify CRP) and 50 ng genomic DNA.…”
Section: Methodsmentioning
confidence: 99%