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Sequence diversification and exon inactivation in the glycophorin A gene family from chimpanzee to human
Authors:Cheng-Han Huang  Shen-Si Xie  W Socha  Olga O Blumenfelde
Institution:(1) Lindsley F. Kimball Research Institute, New York Blood Center, 310 East 67th Street, 10021 New York, NY, USA;(2) Department of Biochemistry, Albert Einstein College of Medicine, 1300 Morris Park Avenue, 10461 Bronx, NY, USA;(3) Laboratory for Experimental Medicine and Surgery in Primates (LEMSIP), New York University School of Medicine, RR #1 Long Meadow Road, 10987 Tuxedo, NY, USA
Abstract:In humans, the allelic diversity of MNSs glycophorins (GP) occurs mainly through the recombinational modulation of silent exons (pseudoexons) in duplicated genes. To address the origin of such a mechanism, structures of GPA, GPB, and GPE were determined in chimpanzee, the only higher primate known to have achieved a three-gene framework as in humans. Pairwise comparison of the chimpanzee and human genes revealed a high degree of sequence identity and similar exon-intron organization. However, the chimpanzee GPA gene lacks a completely formed M- or N-defining sequence as well as a consensus sequence for the Asn-linked glycosylation. In the case of the GPB gene, exon III is expressed in the chimpanzee but silenced, as a pseudoexon, in the human. Therefore, the protein product in the chimpanzee bears a larger extracellular domain than in the human. For the GPE genes, exon III and exon IV have been inactivated by identical donor splice-site mutations in the two species. Nevertheless, the chimpanzee GPE-like mRNA appeared to be transcribed from a GPB/E composite gene containing no 24-bp insertion sequence in exon V for the transmembrane domain. These results suggest a divergent processing of exonic units from chimpanzee to human in which the inactivation of GPB exon III preserved a limited sequence repertoire for diversification of human glycophorins.Correspondence to: O.O. Blumenfeld
Keywords:Human  Chimpanzee  Glycophorins  MNSs blood-group system  Exon activation-inactivation
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