Partial deletion of beta-globin gene DNA in certain patients with beta 0-thalassemia. | Zendy

Stuart H. Orkin | Zendy; Julie M. Old | Zendy; D. J. Weatherall | Zendy; David G. Nathan | Zendy

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Partial deletion of beta-globin gene DNA in certain patients with beta 0-thalassemia.

Author(s) -

Stuart H. Orkin,

Julie M. Old,

D. J. Weatherall,

David G. Nathan

Publication year - 1979

Publication title -

proceedings of the national academy of sciences

Language(s) - English

Resource type - Journals

SCImago Journal Rank - 5.011

H-Index - 771

eISSN - 1091-6490

pISSN - 0027-8424

DOI - 10.1073/pnas.76.5.2400

Subject(s) - bamhi , ecori , biology , microbiology and biotechnology , restriction enzyme , beta (programming language) , gene , genetics , globin , beta thalassemia , thalassemia , dna , computer science , programming language

We have used restriction endonuclease mapping of cell DNA to investigate the structure of the beta-globin gene in beta-thalassemias. Among 17 individuals with beta +- and beta 0-thalassemia, we observed three patients of Indian origin with beta 0-thalassemia whose DNA revealed a consistent mapping abnormality. In one beta allele in each diploid cell, 0.6 kilobase of DNA was deleted from beta-specific Pst I and Bgl II restriction fragments. This deletion involved 3' beta-globin gene sequences and eliminated the EcoRI site normally present at codons 121/122, but it did not extend to the BamHI site at codons 98--100 on the 5' side of the 0.90-kilobase intervening sequence normally present in beta-globin genes. Partial beta-globin gene deletion appears, therefore, to be a primary molecular defect seen in certain patients with beta 0-thalassemia.

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