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Localization of sequences coding for histone messenger RNA in the chromosomes of Drosophila melanogaster
Authors:M L Pardue  L H Kedes  E S Weinberg  M L Birnstiel
Institution:(1) Department of Biology, Massachusetts Institute of Technology, 02139 Cambridge, Massachusetts, USA;(2) Department of Medicine, Stanford University School of Medicine and the Veterans Administration Hospital, 94305 Palo Alto, California, USA;(3) Department of Biology, The Johns Hopkins University, 21218 Baltimore, Maryland, USA;(4) Institut für Molekularbiologie II der Universität Zürich, Zürich, Switzerland
Abstract:In situ hybridization of sea urchin (Psammechinus miliaris, Lytechinus pictus and Strongylocentrotus purpuratus) histone messenger RNA has been used to map complementary sequences on polytene chromosomes from Drosophila melanogaster. The sea urchin RNA hybridizes to the polytene regions from 39D3 through 39E1-2, including both of these bands (39D2 may also be included). This region is identical to the one which hybridizes most heavily with non-polyadenylated cytoplasmic RNA from D. melanogaster tissues. Sea urchin mRNAs coding for several individual histones each hybridize across the entire region from 39D3 (or D2) through 39E1-2, as would be expected if the individual mRNA sequences are interspersed. In view of the apparently even distribution of sequences complementary to histone mRNA within the 39D3-39E1-2 region, the significance of the several polytene bands in this region remains an open question. Biochemical characterization of the hybrids between sea urchin histone mRNA and D. melanogaster DNA suggests that sea urchin mRNAs for several of the histone classes have some portions which retain enough sequence homology with the D. melanogaster sequences to form hybrids, although the hybrids have base pair mismatches. In situ hybridization of chromosomes in which region 39D-E is ectopically paired show no evidence of sequence homology in the chromosome region with which 39D-E is associated.
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