Your search keyword '"Pfitzinger, H."' showing total 3 results

1. [DNA and paternity testing].

Author

de Mazancourt P and Pfitzinger H

Subjects

Adult, DNA Fingerprinting methods, Female, Humans, Male, DNA analysis, Paternity

Published

2005

2. French Caucasian population data for HUMTH01 and HUMFES/FPS short tandem repeat (STR) systems.

Author

Pfitzinger H, Ludes B, Kintz P, Tracqui A, and Mangin P

Subjects

Alleles, Base Sequence, Chromosome Mapping, France, Genotype, Humans, Molecular Sequence Data, Polymerase Chain Reaction, Polymorphism, Genetic, Random Allocation, Sensitivity and Specificity, DNA analysis, Forensic Medicine methods, Genetics, Population, Minisatellite Repeats genetics, White People genetics

Abstract

The recent technology of amplification of DNA sequences by the polymerase chain reaction (PCR) has already proved to be a very useful tool for the analysis of variable number of tandem repeat (VNTR) loci. Short tandem repeat (STR) loci appear as other promising PCR-based identification systems. In fact, DNA typing based on PCR amplification of STRs is very sensitive and allows to overcome major problems encountered when using the RFLP method, such as typing of very small amounts of DNA, highly degraded DNA or mixtures of DNA from more than one individual. Two STR systems, HUMTH01 (a tetranucleotide repeat (AATG) sequence located on chromosome 11) and HUMFES/FPS (a tetranucleotide repeat (ATTT) sequence located on chromosome 15) were investigated in order to determine allele and genotype frequencies for a French caucasian population sample. HUMTH01 and HUMFES/FPS alleles were amplified by the use of PCR and amplified STR sequences were analyzed on 6% Hydrolink Long Ranger gels and visualized by silver staining. The study was conducted on a sample of unrelated individuals (N approximately 190) randomly selected from the French caucasian population. The genotype distributions met Hardy-Weinberg expectations for both HUMTH01 and HUMFES/FPS STR systems. Furthermore, an additional allele, never reported before was observed at the HUMFES/FPS locus: it migrates as an allele containing 7 repeat units and corresponds to the smallest allele identified for this locus.

Published

1995

3. Sex determination of forensic samples: co-amplification and simultaneous detection of a Y-specific and an X-specific DNA sequence.

Author

Pfitzinger H, Ludes B, and Mangin P

Subjects

Base Sequence, Blood Stains, Female, Hair chemistry, Humans, Male, Repetitive Sequences, Nucleic Acid, Semen chemistry, Vaginal Smears, DNA genetics, Sex Determination Analysis methods, X Chromosome, Y Chromosome

Abstract

The detection of restriction fragment length polymorphisms (RFLP) (1) in DNA extracted from forensic samples remains impossible in a significant number of cases due to deterioration and contamination of the biological material and the extremely low quantities of DNA isolated. The polymerase chain reaction (PCR) is a recent and particularly convenient method for analysing and typing very small amounts (10-20 ng) of degraded human DNA. DNA analysis at the level of a few cells present in forensic samples such as bloodstains, semen stains, vaginal swabs and head hair bulbs now appears possible using DNA amplification. A PCR protocol was adapted to simultaneously amplify a Y-specific DNA repeat sequence from the DYZ1 locus and an X-specific DNA repeat sequence from the DXS424 locus. The co-amplified Y-specific DNA fragment (102 bp) and X-specific DNA fragments (181-199 bp) were visualized on an ethidium bromide-stained 4% agarose gel. The male or female type of the amplified DNA extracted from blood samples, bloodstains, semen stains, vaginal swabs, brain tissue and 1, 2, 5, or 10 head hair bulbs was determined.

Published

1993