Your search keyword '"Dero B"' showing total 4 results

1. Gene activation and re‐expression of a Trypanosoma brucei variant surface glycoprotein.

Author

Michiels, F., Matthyssens, G., Kronenberger, P., Pays, E., Dero, B., Van Assel, S., Darville, M., Carvador, A., Steinert, M., and Hamers, R.

Abstract

The expression of the Trypanosoma brucei variant surface glycoprotein AnTat 1.1 proceeds by a mechanism that transfers a duplicated gene copy into a new genomic environment, the so‐called expression site, where it will be expressed. We have isolated a genomic fragment containing the region spanning the expression site‐transposon junction, and the 5′ half of the coding sequence. Comparing this DNA segment with its template copy (basic copy) allowed us to identify the exact breaking point and indicated a base sequence which could be involved in initiating the transposition event. Sequencing data also indicated that the co‐transposed segment 5′ to the coding sequence is 430 bp in length. The extreme 5′ end of the mRNA is derived from a region in the expression site not immediately adjacent to the transposed DNA segment. This particular sequence exists in multiple copies in the genome and is common to the mRNA of all variant surface glycoproteins so far analysed.

Published

1983

2. Structure and transcription of the actin gene of Trypanosoma brucei

Author

Ben Amar, M F, Pays, A, Tebabi, P, Dero, B, Seebeck, T, Steinert, M, and Pays, E

Abstract

In Trypanosoma brucei, the actin gene is present in a cluster of two, three, or four tandemly linked copies, depending on the strain. Each cluster seems to exist in two allelic versions, as suggested by the polymorphism of both gene number and restriction fragment length in the DNA from cloned trypanosomes. The amplification of the gene copy number probably occurs through unequal sister chromatid exchange. The chromosomes harboring the actin genes belong to the large size class. The coding sequence was 1,128 nucleotides long and showed 60 to 70% homology to other eucaryotic actin genes. Surprisingly, this homology seemed weaker with Trypanosoma congolense, Trypanosoma cruzi, Trypanosoma vivax, Trypanosoma mega, or Leishmania actin-specific sequences. The mRNA was around 1.6 kilobases long and was synthesized at the same level in bloodstream and procyclic forms of the parasite. Large RNA precursors, up to 7.7 kilobases, were found in a pattern identical in strains containing either two or three gene copies. Probing of the flanking regions of the gene with either steady-state or in vitro transcripts, as well as S1 nuclease protection and primer extension experiments, allowed mapping of the 3' splice site of the actin mRNA, 38 nucleotides upstream from the translation initiation codon. A variably sized poly(dT) tract was found about 30 base pairs ahead of the splice site. The largest detected actin mRNA precursor seemed to give rise to at least two additional stable mRNAs. The RNA polymerase transcribing the actin gene exhibited the same sensitivity to inhibition by alpha-amanitin as that transcribing both the spliced leader and the bulk of polyadenylated mRNAs.

Published

1988

3. The genome and the antigen gene repertoire of Trypanosoma brucei gambiense are smaller than those of T. b. brucei.

Author

Dero B, Zampetti-Bosseler F, Pays E, and Steinert M

Subjects

Animals, Base Sequence, Chromosome Mapping, Flow Cytometry, Molecular Sequence Data, Nucleic Acid Hybridization, Trypanosoma brucei brucei immunology, Trypanosoma brucei gambiense immunology, Antigens, Protozoan genetics, DNA genetics, Genes, Trypanosoma brucei brucei genetics, Trypanosoma brucei gambiense genetics

Abstract

The amount of nuclear DNA of Trypanosoma brucei gambiense is only 70% of that of T. b. brucei. The difference is partially due to depletion of 50-150 kb mini-chromosomes in T. b. gambiense, as well as a reduction in the content of some repetitive DNA families. Quantitation of 'barren' DNA regions characteristic of the 5' environment of telomeric antigen genes confirms that the T. b. gambiense genome contains fewer chromosome ends, and thus most probably fewer telomeric antigen genes, than T. b. brucei. The extent of the antigen gene repertoire of the two subspecies has been estimated by hybridization with probes specific for the conserved 3' region of antigen genes. It appears that the repertoire of the gambiense subspecies is only about 50% of that of T. b. brucei. These observations are discussed with regard to the stability of the T. b. gambiense repertoire.

Published

1987

4. At least two transposed sequences are associated in the expression site of a surface antigen gene in different trypanosome clones.

Author

Pays E, Van Assel S, Laurent M, Dero B, Michiels F, Kronenberger P, Matthyssens G, Van Meirvenne N, Le Ray D, and Steinert M

Subjects

Animals, Base Sequence, Transcription, Genetic, Trypanosoma immunology, Antigens, Surface genetics, Cloning, Molecular, DNA Transposable Elements, Trypanosoma genetics

Abstract

The expression of several trypanosome surface antigen genes proceeds by duplication of a basic copy (BC) of the gene and transposition of the expression-linked copy (ELC) into an expression site. This site, which seems to be the same for different genes of the same repertoire, is located near a chromosome end. In the AnTat 1.1 antigen gene expression site, the ELC is found associated with another sequence that we have called the "companion." We found that this companion is the transposed copy of another sequence also located in an unstable DNA terminus, and that it is conserved in the expression site of AnTat 1.10 and AnTat 1.1B, two clones successively derived from AnTat 1.1. The companion sequence is not part of the surface antigen gene, but we may infer from extensive homologies with another ELC sequence (IoTat 1.3, J. E. Donelson, personal communication) that it represents a 5' residual fragment of a former ELC. In three other AnTat 1.1-like clones, the companion sequence was not found associated with the ELC. It is concluded that the expression-linked duplicative transposition of variable antigen genes is a flexible mechanism, which can apply to variably sized stretches of the same BC.

Published

1983