10208647

Source:http://linkedlifedata.com/resource/pubmed/id/10208647

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Predicate	Object
rdf:type	pubmed:Citation
lifeskim:mentions	umls-concept:C0002085, umls-concept:C0032520, umls-concept:C0919534, umls-concept:C1511790
pubmed:issue	1
pubmed:dateCreated	1999-5-28
pubmed:abstractText	Approximately 50% of individuals in most human populations completely lack activity of the detoxifying enzyme glutathione S-transferase M1. The medical consequences of this deficiency have been extensively investigated in molecular epidemiological studies, but possible differences of the highly active homozygous genotype versus the moderately active heterozygous genotype could not be considered because many currently used polymerase chain reaction (PCR) assays cannot distinguish the homozygous genotypes GSTM1 A/A and GSTM1B/B from the heterozygous genotypes GSTM1A/0 and GSTM1B/0. Here, we describe that long PCR is suitable for this purpose by specifically producing a signal for the GSTM10 allele. Based on the published cluster of GSTM genes (GSTM1 to -M5), a 13-kb segment spanning the site of the GSTM1 deletion was amplified using a GSTM2-specific forward primer (5'-CATCGCTTATGATGTCCTTGAGAGAAACCAAG-3') and a reverse primer, which is specific for the upstream region of GSTMS (5'-GCGTTTCTGAGGACTGGACTGATGATCG-3'). Any failure in the amplification was controlled by co-amplification of a 15-kb human tissue plasminogen activator gene fragment. The GSTM10-specific 13-kb amplicon appears in all carriers of one or two null alleles, but in none of the 14 tested GST1A/B samples which served as controls since individuals with this genotype are known to lack any GSTM10 allele. While conventional PCR assays for detection of the GSTM1 deletion differentiated homozygously deficient from hetero- or homozygously active individuals, this long PCR assay differentiates homozygously active from hetero- or homozygously deficient individuals. Using both assays, an unambiguous differentiation into carriers of zero, one or two active alleles of GSTM1 is possible.
pubmed:language	eng
pubmed:journal	http://linkedlifedata.com/resource/pubmed/journal/9211735
pubmed:citationSubset	IM
pubmed:chemical	http://linkedlifedata.com/resource/pubmed/chemical/DNA Primers, http://linkedlifedata.com/resource/pubmed/chemical/Glutathione Transferase, http://linkedlifedata.com/resource/pubmed/chemical/glutathione S-transferase M1
pubmed:status	MEDLINE
pubmed:month	Feb
pubmed:issn	0960-314X
pubmed:author	pubmed-author:BrockmöllerJJ, pubmed-author:KerrBB, pubmed-author:RootsII, pubmed-author:SachseCC
pubmed:issnType	Print
pubmed:volume	9
pubmed:owner	NLM
pubmed:authorsComplete	Y
pubmed:pagination	89-94
pubmed:dateRevised	2006-11-15
pubmed:meshHeading	pubmed-meshheading:10208647-Alleles, pubmed-meshheading:10208647-Base Sequence, pubmed-meshheading:10208647-DNA Primers, pubmed-meshheading:10208647-Glutathione Transferase, pubmed-meshheading:10208647-Humans, pubmed-meshheading:10208647-Polymerase Chain Reaction
pubmed:year	1999
pubmed:articleTitle	Detection of the GSTM1*0 allele by long polymerase chain reaction.
pubmed:affiliation	Institute of Clinical Pharmacology, University Clinic Charité, Humboldt University of Berlin, Germany.
pubmed:publicationType	Journal Article, Research Support, Non-U.S. Gov't