Your search keyword '"Christian Tschudi"' showing total 113 results

101. Reverse transcription of trypanosome variable antigen mRNAs initiated by a specific oligonucleotide primer

Author

William H. Konigsberg, Stephen C. Merritt, Frank F. Richards, and Christian Tschudi

Subjects

Genetics, Multidisciplinary, Base Sequence, Oligonucleotide, Trypanosoma brucei brucei, Nucleic Acid Hybridization, Oligonucleotide Primer, RNA-Directed DNA Polymerase, DNA, Biology, Molecular biology, Reverse transcriptase, genomic DNA, Nucleic acid thermodynamics, Oligodeoxyribonucleotides, Transcription (biology), Complementary DNA, Antigens, Surface, parasitic diseases, Animals, Genomic library, Amino Acid Sequence, RNA, Messenger, Cloning, Molecular, Research Article

Abstract

African trypanosomes change their antigenicity by successively expressing different members of a group of related but highly diverse proteins, the variant surface glycoproteins (VSGs). We describe a synthetic oligonucleotide that can prime specifically reverse transcription of VSG mRNA out of total trypanosome poly(A)+ RNA. The specificity of this priming was verified by cDNA sequence analysis of the transcription products and by the demonstration of variant-specific hybridization of the individual cDNAs to cellular RNA. The oligonucleotide primer also was used as a probe for the conserved sequence found on these VSG mRNAs in trypanosome genomic DNA libraries. A large number of primer-positive clones were detected in a Trypanosoma gambiense genomic library, but very few positive signals were found in a library of Trypanosoma congolense genomic DNA.

Published

1983

102. The U2 RNA analogue of Trypanosoma brucei gambiense: implications for a splicing mechanism in trypanosomes

Author

Elisabetta Ullu, Christian Tschudi, and Frank F. Richards

Subjects

Genetics, Base Sequence, RNA Splicing, Trypanosoma brucei gambiense, Trypanosoma brucei brucei, Intron, RNA-dependent RNA polymerase, RNA, Nucleic Acid Hybridization, Biology, Non-coding RNA, Post-transcriptional modification, Genes, Species Specificity, RNA editing, RNA, Small Nuclear, RNA splicing, Animals, Nucleic Acid Conformation, Cloning, Molecular, Small nuclear RNA

Abstract

We have isolated the gene coding for the U2 analogue in trypanosomes. The 148 nucleotide long U2 RNA is capped and transcribed from a single copy gene. The 5' half of the molecule is highly homologous to mammalian U2 RNA, while the 3' half does not show any significant sequence homology with the mammalian counterpart. Nevertheless, the trypanosome U2 RNA can be folded into a secondary structure resembling the one proposed for U2 RNA. The presence of a U2 analogue and most likely other U RNAs in trypanosomes suggests that splicing is involved at some point in the maturation of mRNA. Possible interactions of the U2 RNA with the spliced leader RNA are considered.

Published

1986

103. The U6 small nuclear RNA from Trypanosoma brucei

Author

Adrian R. Krainer, Christian Tschudi, and Elisabetta Ullu

Subjects

biology, Base Sequence, Trypanosoma brucei gambiense, Saccharomyces cerevisiae, Molecular Sequence Data, Nucleic acid sequence, Molecular cloning, Trypanosoma brucei, biology.organism_classification, Molecular biology, Rats, chemistry.chemical_compound, chemistry, RNA, Small Nuclear, Sequence Homology, Nucleic Acid, Transfer RNA, Genetics, Protozoa, Animals, Small nuclear RNA, DNA

Published

1988

104. Polygene transcripts are precursors to calmodulin mRNAs in trypanosomes

Author

Christian Tschudi and E. Ullu

Subjects

Polyadenylation, Calmodulin, Transcription, Genetic, Trypanosoma brucei gambiense, Trypanosoma brucei brucei, DNA, Ribosomal, General Biochemistry, Genetics and Molecular Biology, Transcription (biology), Gene expression, Animals, Cloning, Molecular, Molecular Biology, Gene, Repetitive Sequences, Nucleic Acid, Messenger RNA, General Immunology and Microbiology, biology, General Neuroscience, RNA, Nucleic Acid Hybridization, Molecular biology, Genes, Polygene, biology.protein, Research Article

Abstract

In African trypanosomes, calmodulin is encoded by a small family of tandemly repeated genes consisting of three to four units. We show that all the members of the calmodulin cluster of Trypanosoma brucei gambiense are expressed. In addition to mature mRNAs, steady-state RNA contains a small percentage of polygene transcripts which comprise at least two and probably all calmodulin genes. The 5' ends of a portion of these molecules appear to be indistinguishable from those of mature calmodulin mRNAs. Polygene transcripts are not polyadenylated and have discrete ends which map in the intergenic regions downstream from the polyadenylation sites. Using biotinylated hybridization probes and selection of the hybrids on streptavidin-agarose, we further show that calmodulin polygene transcripts are the most abundant RNA species detected in pulse-labelled RNA of cultured procyclic trypanosomes. Our data strongly imply that polygene transcripts are authentic precursors to mature calmodulin mRNAs.

Published

1988

105. Calmodulin genes in trypanosomes are tandemly repeated and produce multiple mRNAs with a common 5' leader sequence

Author

Frank F. Richards, Curtis L. Patton, Christian Tschudi, Alexander S. Young, and Larry Ruben

Subjects

Calmodulin, Genetic Linkage, RNA Splicing, Trypanosoma brucei brucei, chemistry.chemical_compound, Transcription (biology), Animals, Amino Acid Sequence, RNA, Messenger, Cloning, Molecular, RNA Processing, Post-Transcriptional, Gene, Peptide sequence, Repetitive Sequences, Nucleic Acid, Genetics, Messenger RNA, Multidisciplinary, biology, Base Sequence, RNA, chemistry, Gene Expression Regulation, Genes, RNA splicing, biology.protein, Calcium, DNA, Research Article

Abstract

In Trypanosoma brucei gambiense, the Ca2+ binding protein calmodulin is encoded by three identical tandemly repeated genes. The transcripts of these genes consist of several RNA species similar in size. A 35-nucleotide spliced leader sequence is present at the 5' end of each mRNA but is not encoded by DNA contiguous to these genes. We have identified two different sites for the fusion of the leader to the mRNA. These results strongly support the idea that a novel, possibly discontinuous, transcription mechanism is used by these parasites.

Published

1985

106. Alu sequences are processed 7SL RNA genes

Author

Elisabetta Ullu and Christian Tschudi

Subjects

Genetics, Multidisciplinary, Base Sequence, Transcription, Genetic, Xenopus, Nucleic acid sequence, RNA, Alu element, Biology, Biological Evolution, Short Interspersed Element, Drosophila melanogaster, Genes, Species Specificity, Short Interspersed Nucleotide Elements, Animals, Humans, Signal recognition particle RNA, Repeated sequence, Gene

Abstract

7SL RNA is an abundant cytoplasmic RNA which functions in protein secretion as a component of the signal recognition particle. Alu sequences are the most abundant family of human and rodent middle repetitive DNA sequences (reviewed in ref. 2). The primary structure of human 7SL RNA consists of an Alu sequence interrupted by a 155-base pair (bp) sequence that is unique to 7SL RNA. In order to obtain information about the evolution of the Alu domain of 7SL RNA, we have determined the nucleotide sequence of a cDNA copy of Xenopus laevis 7SL RNA and of the 7SL RNA gene of Drosophila melanogaster. We find that the Xenopus sequence is 87% homologous with its human counterpart and the Drosophila 7SL RNA is 64% homologous to both the human and amphibian molecules. Despite the evolutionary distance between the species, significant blocks of homology to both the Alu and 7SL-specific portions of mammalian 7SL RNA can be found in the insect sequence. These results clearly demonstrate that the Alu sequence in 7SL RNA appeared in evolution before the mammalian radiation. We suggest that mammalian Alu sequences were derived from 7SL RNA (or DNA) by a deletion of the central 7SL-specific sequence, and are therefore processed 7SL RNA genes.

Published

1984

107. Sequence and heterogeneity in the 5S RNA gene cluster of Drosophila melanogaster

Author

Christian Tschudi and Vincenzo Pirrotta

Subjects

Genetics, Electrophoresis, Agar Gel, biology, Base Sequence, RNA, Spacer DNA, DNA Restriction Enzymes, biology.organism_classification, Restriction enzyme, chemistry.chemical_compound, Drosophila melanogaster, chemistry, Gene cluster, Coding region, Animals, Electrophoresis, Polyacrylamide Gel, Cloning, Molecular, Gene, DNA, Research Article

Abstract

The sequence of the entire 5S RNA gene of Drosophila melanogaster was determined by sequencing collectively 23 copies contained in a cloned fragment of Drosophila DNA and by sequencing individually four subcloned gene copies. A repetitive heptamer (GCTG CCT) present in variable numbers immediately following the coding sequence, is responsible for the length heterogeneity in the spacer region. Some of the gene copies contain a nucleotide change in the coding region which results in a new site for the restriction enzyme Mn1 I. The variant 5S RNA produced by these gene copies has not been detected in vivo. Two other single nucleotide variations were identified in the spacer region.

Published

1980

108. The 5S genes of Drosophila melanogaster

Author

Vincenzo Pirrotta, Paul Schedl, Spyros Artavanis-Tsakonas, Christian Tschudi, Ruth Steward, and Walter J. Gehring

Subjects

Genetics, Base Sequence, Transcription, Genetic, Base pair, Chromosome Mapping, DNA, DNA Restriction Enzymes, Biology, biology.organism_classification, Molecular biology, General Biochemistry, Genetics and Molecular Biology, Insert (molecular biology), Molecular Weight, Plasmid, Restriction map, Drosophila melanogaster, Tandem repeat, Genes, RNA, Ribosomal, Culture Techniques, Hybrid plasmid, Repeat unit, Plasmids

Abstract

We have cloned embryonic Drosophila DNA using the poly (dA-DT) connector method (Lobban and Kaiser, 1973) and the ampicillin-resistant plasmid pSF2124 (So, Gill and Falkow, 1975) as a cloning vehicle. Two clones, containing hybrid plasmids with sequences complementary to a 5S RNA probe isolated from Drosophila tissue culture cells, were identified by the Grunstein and Hogness (1975) colony hybridization procedure. One hybrid plasmid has a Drosophila insert which is comprised solely of tandem repeats of the 5S gene plus spacer sequences. The other plasmid contains an insert which has about 20 tandem 5S repeat units plus an additional 4 kilobases of adjacent sequences. The size of the 5S repeat unit was determined by gel electrophoresis and was found to be approximately 375 base pairs. We present a restriction map of both plasmids, and a detailed map of of the5S repeat unit. The 5S repat unit shows slight length and sequence heterogeneity. We present evidence suggesting that the 5S genes in Drosophila melanogaster may be arranged in a single continuous cluster.

Published

1977

109. Analysis of gene function in Trypanosoma brucei using RNA interference

Author

Appolinaire Djikeng, Shuiyuan Shen, Christian Tschudi, and Elisabetta Ullu

Subjects

Electroporation, Transcription, Genetic, Genetic Vectors, Genes, Protozoan, Trypanosoma brucei brucei, Animals, RNA Interference, RNA, Messenger, Cloning, Molecular, RNA, Small Interfering, Molecular Biology, RNA, Protozoan, RNA, Double-Stranded

Abstract

Trypanosoma brucei, a flagellate protozoa of the family Trypanosomatidae, has become one of the model systems for unicellular pathogens to study fundamentally important biological phenomena. The method of choice today to examine gene function in these organisms is RNA interference (RNAi). Messenger RNA (mRNA) degradation is triggered by double-stranded RNA (dsRNA) produced in vivo from transgenes transcribed from opposing tetracycline (tet)-inducible T7 RNA polymerase promoters, or hairpin RNA transcribed from the tet-inducible procyclic acidic repetitive protein promoter. This chapter describes some of the methods we employ for ablation of gene expression by RNAi in T. brucei with particular emphasis on transfection and cloning of procyclic cells, induction of dsRNA expression, isolation of RNA, and analysis of dsRNA and target mRNA.

110. Determinants for cap trimethylation of the U2 small nuclear RNA are not conserved between Trypanosoma brucei and higher eukaryotic organisms

Author

Albrecht Bindereif, Christian Tschudi, Elisabetta Ullu, and Arthur Günzl

Subjects

RNA Caps, Five-prime cap, Molecular Sequence Data, Trypanosoma brucei brucei, RNA polymerase II, Regulatory Sequences, Nucleic Acid, Transfection, Primary transcript, Methylation, Article, Cell Line, RNA, Small Nuclear, Genetics, Animals, snRNP, Promoter Regions, Genetic, Conserved Sequence, Binding Sites, Cap binding complex, Base Sequence, Guanosine, biology, urogenital system, Ribonucleoprotein particle, RNA, Ribonucleoproteins, Small Nuclear, Precipitin Tests, Molecular biology, Cell biology, Mutation, biology.protein, Nucleic Acid Conformation, RNA, Protozoan, Small nuclear RNA, Protein Binding

Abstract

In most eukaryotic organisms the U2 small nuclear RNA (snRNA) gene is transcribed by RNA polymerase II to generate a primary transcript with a 5' terminal 7-methylguanosine cap structure. Following nuclear export, the U2 snRNA is assembled into a core ribonucleoprotein particle (RNP). This involves binding a set of proteins that are shared by spliceosomal snRNPs to the highly conserved Sm site. Prior to nuclear import, the snRNA-(guanosine-N:2)-methyltransferase appears to interact with the core RNP and hypermethylates the cap structure to 2,2, 7-trimethylguanosine (m(3)G). In the protist parasite Trypanosoma brucei, U-snRNAs are complexed with a set of common proteins that are analogous to eukaryotic Sm antigens but do not have a highly conserved Sm sequence motif, and most U-snRNAs are synthesised by RNA polymerase III. Here, we examined the determinants for m(3)G cap formation in T.brucei by expressing mutant U2 snRNAs in vivo and assaying trimethylation and RNP assembly by immunoprecipitation. Surprisingly, these studies revealed that the Sm-analogous region is not required either for binding of the common proteins or for cap trimethylation. Furthermore, except for the first 24 nt which are part of the U2 promoter, the U2 coding region could be substituted or deleted without affecting cap trimethylation.

111. Ingress Throttling and its Applications in IEEE 802.11 Based MANETs

Author

Evgeny Osipov and Christian Tschudin

Subjects

Computer software, QA76.75-76.765

Abstract

One of the stumbling blocks which prevents multihop ad hoc networks from wide deployment is a known problem of unfair bandwidth distribution between competing data sessions. Practically, a combination of the current IEEE 802.11 technology and the standard TCP protocol allows only a couple of up to three hops connections co-exist simultaneously while providing fairly stable and acceptable service to end users. In this article we describe ingress throttling, a resource protection layer which restores fair bandwidth sharing between plain TCP as well as arbitrary UDP sources. We summarize analytical as well as simulation studies of our solution and demonstrate itsapplications for determining scaling limits of ad hoc specificsimulations and evaluating the effect of ad hoc routing onperformance of data communications.

Published

2006

112. TCP-Friendly Bandwidth Sharing in Mobile Ad Hoc Networks: From Theory to Reality

Author

Evgeny Osipov and Christian Tschudin

Subjects

Telecommunication, TK5101-6720, Electronics, TK7800-8360

Abstract

This article addresses a problem of the severe unfairness between multiple TCP sessions in a wireless context also known as “TCP capture†phenomenon. We present an adapted max-min fairness framework to the specifics of MANETs. We introduce a practically implementable cross-layer network architecture which enforces our formal model. We have verified with simulations and real world experiments that under our adaptive rate limiting scheme unfair behavior virtually vanishes. The direct consequence of this work guaranteed stable services for TCP-based applications in MANETs, including traditional FTP, web as well as for UDP-based sessions.

Published

2007

113. Small interfering RNA-producing loci in the ancient parasitic eukaryote Trypanosoma brucei

Author

Joseph B. Franklin, Christian Tschudi, Elisabetta Ullu, and Huafang Shi

Subjects

Ribonuclease III, Convergent transcription unit, lcsh:QH426-470, Retroelements, lcsh:Biotechnology, Trypanosoma brucei brucei, Trans-acting siRNA, Protozoan Proteins, Dicer-deficient, Trypanosome, RNA interference, lcsh:TP248.13-248.65, Genetics, Retrotransposon, RasiRNA, RNA, Small Interfering, biology, Inverted Repeat Sequences, Retroposon, RNA, Argonaute, Inverted repeat, lcsh:Genetics, RNA silencing, Genetic Loci, siRNA, Argonaute Proteins, biology.protein, RNA Interference, Research Article, Dicer, Biotechnology

Abstract

Background At the core of the RNA interference (RNAi) pathway in Trypanosoma brucei is a single Argonaute protein, Tb AGO1, with an established role in controlling retroposon and repeat transcripts. Recent evidence from higher eukaryotes suggests that a variety of genomic sequences with the potential to produce double-stranded RNA are sources for small interfering RNAs (siRNAs). Results To test whether such endogenous siRNAs are present in T. brucei and to probe the individual role of the two Dicer-like enzymes, we affinity purified Tb AGO1 from wild-type procyclic trypanosomes, as well as from cells deficient in the cytoplasmic (Tb DCL1) or nuclear (Tb DCL2) Dicer, and subjected the bound RNAs to Illumina high-throughput sequencing. In wild-type cells the majority of reads originated from two classes of retroposons. We also considerably expanded the repertoire of trypanosome siRNAs to encompass a family of 147-bp satellite-like repeats, many of the regions where RNA polymerase II transcription converges, large inverted repeats and two pseudogenes. Production of these newly described siRNAs is strictly dependent on the nuclear DCL2. Notably, our data indicate that putative centromeric regions, excluding the CIR147 repeats, are not a significant source for endogenous siRNAs. Conclusions Our data suggest that endogenous RNAi targets may be as evolutionarily old as the mechanism itself.