8 research outputs found

    DNA sequence and expression of the B95-8 Epstein - Barr virus genome

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    The complete (172,282 base pairs) nucleotide sequence of the B95-8 strain of Epstein-Barr virus has been established using the dideoxynucleotide/M13 sequencing procedure. Many RNA polymerase II promoters have been mapped and the mRNAs from these promoters have been assigned to the latent or early/late productive virus cycles. Likely protein-coding regions have been identified and three of these have been shown to encode a ribonucleotide reductase, a DNA polymerase and two surface glycoproteins. © 1984 Nature Publishing Group

    THE NODULE-SPECIFIC VFENOD-GRP3 GENE ENCODING A GLYCINE-RICH EARLY NODULIN IS LOCATED ON CHROMOSOME-I OF VICIA-FABA L AND IS PREDOMINANTLY EXPRESSED IN THE INTERZONE II-III OF ROOT-NODULES

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    Küster H, SCHRODER G, FRUHLING M, et al. THE NODULE-SPECIFIC VFENOD-GRP3 GENE ENCODING A GLYCINE-RICH EARLY NODULIN IS LOCATED ON CHROMOSOME-I OF VICIA-FABA L AND IS PREDOMINANTLY EXPRESSED IN THE INTERZONE II-III OF ROOT-NODULES. PLANT MOLECULAR BIOLOGY. 1995;28(3):405-421.A nodule-specific cDNA was isolated from a Vicia faba L. nodule cDNA library. Since time course experiments revealed an early expression of this transcript in the nodule, this cDNA coded for an early nodulin and was designated VfENOD-GRP3. Based on tissue print hybridizations, we found a predominant expression of VfENOD-GRP3 transcripts in the interzone II-III region of broad bean root nodules. The encoded early nodulin ENOD-GRP3 was characterized by an N-terminal signal peptide and a C-terminal domain displaying a glycine content of 31%. Sequence analysis of a genomic VfENOD-GRP3 clone revealed that the signal peptide and the glycine-rich domain were specified by two separate exons. Primer extension experiments identified two adjacent transcription start sites for VfENOD-GRP3 transcripts. The common nodulin sequences 'AAAGAT' and 'CTCTT' were present five and three times on both DNA strands of the putative VfENOD-GRP3 promoter, respectively. Additionally, three sequence motifs resembling organ-specific elements of the soybean lbc3 gene promoter and a sequence similar to the binding site 1 for the nodule trans-acting factor Nat2 were identified. From Southern blot data and from sequence analysis of genomic PCR fragments, the presence of a VfENOD-GRP3 gene family was inferred. By PCR experiments using sequence-specific primers and DNA of microisolated chromosomes as a template, this family was located on the long arm of chromosome I
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