Your search keyword '"Andrew Fire"' showing total 215 results

101. Functional Anatomy of a dsRNA Trigger

Author

Andrew Fire, Craig C. Mello, Susan Parrish, SiQun Xu, and Jamie Fleenor

Subjects

Genetics, RNA silencing, Duplex (building), RNA interference, Sense (molecular biology), Nucleic acid, Homologous chromosome, RNA, Cell Biology, Biology, Molecular Biology, Antisense RNA, Cell biology

Abstract

In RNA-mediated interference (RNAi), externally provided mixtures of sense and antisense RNA trigger concerted degradation of homologous cellular RNAs. We show that RNAi requires duplex formation between the two trigger strands, that the duplex must include a region of identity between trigger and target RNAs, and that duplexes as short as 26 bp can trigger RNAi. Consistent with in vitro observations, a fraction of input dsRNA is converted in vivo to short segments of approximately 25 nt. Interference assays with modified dsRNAs indicate precise chemical requirements for both bases and backbone of the RNA trigger. Strikingly, certain modifications are well tolerated on the sense, but not the antisense, strand, indicating that the two trigger strands have distinct roles in the interference process.

Published

2000

102. Identification and molecular-genetic characterization of a LAMP/CD68-like protein from Caenorhabditis elegans

Author

Andrew Fire, Douglas M. Fambrough, and Mitch Kostich

Subjects

Endosome, Amino Acid Motifs, Molecular Sequence Data, Mutant, Population, Antigens, Differentiation, Myelomonocytic, Cytoplasmic Granules, Antigens, CD, Organelle, Animals, Cloning, Molecular, Caenorhabditis elegans, Caenorhabditis elegans Proteins, education, Peptide sequence, RNA, Double-Stranded, Sequence Deletion, Macrosialin, Expressed Sequence Tags, education.field_of_study, Membrane Glycoproteins, Sequence Homology, Amino Acid, biology, Computational Biology, Lysosome-Associated Membrane Glycoproteins, Helminth Proteins, Cell Biology, biology.organism_classification, Protein Structure, Tertiary, Cell biology, Intestines, Phenotype, Membrane protein

Abstract

Lysosome associated membrane proteins (LAMPs) constitute a family of vertebrate proteins located predominantly in lysosomes, with lesser amounts present in endosomes and at the cell surface. Macrosialin/CD68s are similar to LAMPs in their subcellular distribution and amino acid sequence and presumed structure across the carboxyl terminal two thirds of their length. The functions of LAMPs and CD68s are not known. In the present study, a bioinformatics approach was used to identify a Caenorhabditis elegans protein (LMP-1) with sequence and presumed structural similarity to LAMPs and CD68s. LMP-1 appears to be the only membrane protein in C. elegans that carries a GYXX(phi) vertebrate lysosomal targeting sequence at its C terminus (where (phi) is a large, hydrophobic residue). LMP-1 was found to be present from early embryonic stages through adulthood and to be predominantly localized at the periphery of a population of large, membrane-bound organelles, called granules, that are seen throughout the early embryo but in later stages are restricted to the cells of the intestine. Analysis of an LMP-1 deficient C. elegans mutant revealed that LMP-1 is not required for viability under laboratory conditions, but the absence of LMP-1 leads to an alteration in intestinal granule populations, with apparent loss of one type of granule.

Published

2000

103. The RING finger/B-Box factor TAM-1 and a retinoblastoma-like protein LIN-35 modulate context-dependent gene silencing in Caenorhabditis elegans

Author

Paul W. Sternberg, Jenny Hsieh, Andrew Fire, Jing Liu, Stephen A. Kostas, and Chieh Chang

Subjects

Transgene, Molecular Sequence Data, Mutant, Muscle Proteins, Chromatin silencing, Cell Cycle Proteins, Genetics, Ring finger, medicine, Animals, Gene silencing, Amino Acid Sequence, Gene Silencing, Transgenes, Nuclear protein, Caenorhabditis elegans, Caenorhabditis elegans Proteins, Gene, biology, Nuclear Proteins, Helminth Proteins, biology.organism_classification, Repressor Proteins, Genes, ras, Phenotype, medicine.anatomical_structure, Sequence Alignment, Signal Transduction, Research Paper, Developmental Biology

Abstract

Context-dependent gene silencing is used by many organisms to stably modulate gene activity for large chromosomal regions. We have used tandem array transgenes as a model substrate in a screen for Caenorhabditis elegans mutants that affect context-dependent gene silencing in somatic tissues. This screen yielded multiple alleles of a previously uncharacterized gene, designated tam-1 (for tandem-array-modifier). Loss-of-function mutations in tam-1 led to a dramatic reduction in the activity of numerous highly repeated transgenes. These effects were apparently context dependent, as nonrepetitive transgenes retained activity in a tam-1 mutant background. In addition to the dramatic alterations in transgene activity, tam-1 mutants showed modest alterations in expression of a subset of endogenous cellular genes. These effects include genetic interactions that place tam-1 into a group called the class B synMuv genes (for a Synthetic Multivulva phenotype); this family plays a negative role in the regulation of RAS pathway activity in C. elegans. Loss-of-function mutants in other members of the class-B synMuv family, including lin-35, which encodes a protein similar to the tumor suppressor Rb, exhibit a hypersilencing in somatic transgenes similar to that of tam-1 mutants. Molecular analysis reveals that tam-1 encodes a broadly expressed nuclear protein with RING finger and B-box motifs.

Published

1999

104. RNA-triggered gene silencing

Author

Andrew Fire

Subjects

Genetics, Models, Genetic, fungi, Immunity, Gene Expression, RNA-dependent RNA polymerase, RNA, Biology, Plants, Genetically Modified, biology.organism_classification, Biological Evolution, Planaria, Animals, Genetically Modified, RNA silencing, Gene expression, DNA methylation, Animals, Gene silencing, Gene, RNA, Double-Stranded

Abstract

Double-stranded RNA (dsRNA) has recently been shown to trigger sequence-specific gene silencing in a wide variety of organisms, including nematodes, plants, trypanosomes, fruit flies and planaria; meanwhile an as yet uncharacterized RNA trigger has been shown to induce DNA methylation in several different plant systems. In addition to providing a surprisingly effective set of tools to interfere selectively with gene function, these observations are spurring new inquiries to understand RNA-triggered genetic-control mechanisms and their biological roles.

Published

1999

105. Two-Color GFP Expression System for C. elegans

Author

D.W. Piston, N.S. Desai, S. Xu, David M. Miller, J. Fleenor, Andrew Fire, G.H. Patterson, and D.C. Hardin

Subjects

Signal peptide, Green Fluorescent Proteins, Gene Expression, Context (language use), macromolecular substances, Biology, medicine.disease_cause, General Biochemistry, Genetics and Molecular Biology, Green fluorescent protein, Animals, Genetically Modified, Gene expression, medicine, Animals, Coding region, Caenorhabditis elegans, Genetics, Mutation, Expression vector, Muscles, fungi, biology.organism_classification, Cell biology, Luminescent Proteins, Spectrometry, Fluorescence, Amino Acid Substitution, Evaluation Studies as Topic, Plasmids, Biotechnology

Abstract

We describe the use of modified versions of the Aequora victoria green fluorescent protein (GFP) to simultaneously follow the expression and distribution of two different proteins in the nematode, Caenorhabditis elegans. A cyan-colored GFP derivative, designated CFP, contains amino acid (aa) substitutions Y66W, N146I, M153T and V163A relative to the original GFP sequence and is similar to the previously reported “W7” form. A yellow-shifted GFP derivative, designated YFP, contains aa substitutions S65G, V68A, S72A and T203Y and is similar to the previously described “10C” variant. Coding regions for CFP and YFP were constructed in the context of a high-activity C. elegans expression system. Previously characterized promoters and localization signals have been used to express CFP and YFP in C. elegans. Filter sets designed to distinguish YFP and CFP fluorescence spectra allowed visualization of the two distinct forms of GFP in neurons and in muscle cells. A series of expression vectors carrying CFP and YFP have been constructed and are being made available to the scientific community.

Published

1999

106. RNA as a target of double-stranded RNA-mediated genetic interference in Caenorhabditis elegans

Author

SiQun Xu, Andrew Fire, and Mary K. Montgomery

Subjects

Transcription, Genetic, Muscle Proteins, Animals, Genetically Modified, Exon, Transcription (biology), DNA-directed RNA interference, Operon, Animals, RNA, Messenger, Caenorhabditis elegans, Caenorhabditis elegans Proteins, Genes, Helminth, RNA, Double-Stranded, Messenger RNA, Multidisciplinary, Models, Genetic, biology, RNA, Exons, Helminth Proteins, Biological Sciences, biology.organism_classification, Molecular biology, mRNA surveillance, RNA silencing, Gene Expression Regulation, Mutagenesis, Calmodulin-Binding Proteins, RNA, Helminth

Abstract

Introduction of exogenous double-stranded RNA (dsRNA) into Caenorhabditis elegans has been shown to specifically and potently disrupt the activity of genes containing homologous sequences. In this study we present evidence that the primary interference effects of dsRNA are post-transcriptional. First, we examined the primary DNA sequence after dsRNA-mediated interference and found no evidence for alterations. Second, we found that dsRNA-mediated interference with the upstream gene in a polar operon had no effect on the activity of the downstream gene; this finding argues against an effect on initiation or elongation of transcription. Third, we observed by in situ hybridization that dsRNA-mediated interference produced a substantial, although not complete, reduction in accumulation of nascent transcripts in the nucleus, while cytoplasmic accumulation of transcripts was virtually eliminated. These results indicate that the endogenous mRNA is the target for interference and suggest a mechanism that degrades the targeted RNA before translation can occur. This mechanism is not dependent on the SMG system, an mRNA surveillance system in C. elegans responsible for targeting and destroying aberrant messages. We suggest a model of how dsRNA might function in a catalytic mechanism to target homologous mRNAs for degradation.

Published

1998

107. Analysis of a Caenorhabditis elegans Twist homolog identifies conserved and divergent aspects of mesodermal patterning

Author

Jun Liu, Brian D. Harfe, Ana Vaz Gomes, Andrew Fire, Michael Krause, and Cynthia Kenyon

Subjects

Mesoderm, animal structures, Molecular Sequence Data, Biology, Twist transcription factor, Genetics, medicine, Animals, Amino Acid Sequence, Caenorhabditis elegans, Caenorhabditis elegans Proteins, Promoter Regions, Genetic, Body Patterning, Homeodomain Proteins, Regulation of gene expression, Base Sequence, Sequence Homology, Amino Acid, Muscles, Twist-Related Protein 1, Mesodermal cell fate specification, Genes, Homeobox, Nuclear Proteins, biology.organism_classification, Receptors, Fibroblast Growth Factor, Enhancer Elements, Genetic, medicine.anatomical_structure, Gene Expression Regulation, embryonic structures, Mesoderm formation, Homeobox, Ectopic expression, Dimerization, Transcription Factors, Research Paper, Developmental Biology

Abstract

Mesodermal development is a multistep process in which cells become increasingly specialized to form specific tissue types. InDrosophila and mammals, proper segregation and patterning of the mesoderm involves the bHLH factor Twist. We investigated the activity of a Twist-related factor, CeTwist, during Caenorhabditis elegans mesoderm development. Embryonic mesoderm in C. elegans derives from a number of distinct founder cells that are specified during the early lineages; in contrast, a single blast cell (M) is responsible for all nongonadal mesoderm formation during postembryonic development. Using immunofluorescence and reporter fusions, we determined the activity pattern of the gene encoding CeTwist. No activity was observed during specification of mesodermal lineages in the early embryo; instead, the gene was active within the M lineage and in a number of mesodermal cells with nonstriated muscle fates. A role for CeTwist in postembryonic mesodermal cell fate specification was indicated by ectopic expression and genetic interference assays. These experiments showed that CeTwist was responsible for activating two target genes normally expressed in specific subsets of nonstriated muscles derived from the M lineage. In vitro and in vivo assays suggested that CeTwist cooperates with theC. elegans E/Daughterless homolog in directly activating these targets. The two target genes that we have studied,ceh-24 and egl-15, encode an NK-2 class homeodomain and an FGF receptor (FGFR) homolog, respectively. Twist activates FGFR and NK-homeodomain target genes during mesodermal patterning ofDrosophila and similar target interactions have been proposed to modulate mesenchymal growth during closure of the vertebrate skull. These results suggest the possibility that a conserved pathway may be used for diverse functions in mesodermal specification.

Published

1998

108. Chromatin silencing and the maintenance of a functional germline in Caenorhabditis elegans

Author

William G. Kelly and Andrew Fire

Subjects

Male, Zygote, Recombinant Fusion Proteins, Transgene, Green Fluorescent Proteins, Mutant, Disorders of Sex Development, Chromatin silencing, Biology, Article, Germline, Animals, Genetically Modified, Genes, Reporter, Polycomb-group proteins, Animals, Gene silencing, Caenorhabditis elegans, Molecular Biology, Crosses, Genetic, Genes, Helminth, Genetics, Helminth Proteins, biology.organism_classification, Chromatin, Repressor Proteins, Luminescent Proteins, Fertility, Female, Infertility, Female, Developmental Biology

Abstract

The germline of the nematode Caenorhabditis elegans exhibits a remarkable ability to specifically silence transgenic DNA. We have shown that this silencing mechanism is disrupted in animals mutant for the maternal effect sterile genes mes-2, mes-3, mes-4 and mes-6. The proteins encoded by mes-2 and mes-6 have been shown to be related to the Polycomb Group of transcriptional repressors (Holdeman, R., Nehrt, S. and Strome, S. (1998). Development 125, 2457-2467; Korf, I., Fan, F. and Strome, S. (1998). Development 125, 2469-2478). These results suggest that a genetic silencing process is essential for sustained germline function, and that this silencing is mediated, at least in part, by Polycomb Group proteins.

Published

1998

109. Double-stranded RNA as a mediator in sequence-specific genetic silencing and co-suppression

Author

Mary K. Montgomery and Andrew Fire

Subjects

Genetics, Regulation of gene expression, biology, Gene Expression Regulation, Developmental, RNA, Double stranded rna, Plants, biology.organism_classification, Cell biology, Mediator, Gene expression, Animals, Gene silencing, Caenorhabditis elegans, RNA, Double-Stranded, Sequence (medicine)

Published

1998

110. Muscle and nerve-specific regulation of a novel NK-2 class homeodomain factor in Caenorhabditis elegans

Author

Brian D. Harfe and Andrew Fire

Subjects

Cell type, animal structures, Molecular Sequence Data, Mutant, Biology, MyoD, Vulva, Animals, Genetically Modified, Pharyngeal muscles, medicine, Animals, Amino Acid Sequence, RNA, Messenger, Caenorhabditis elegans, Caenorhabditis elegans Proteins, Promoter Regions, Genetic, Enhancer, Molecular Biology, Genes, Helminth, Sequence Deletion, Homeodomain Proteins, Motor Neurons, Genetics, Base Sequence, Sequence Homology, Amino Acid, Activator (genetics), Muscles, Genes, Homeobox, Gene Expression Regulation, Developmental, biology.organism_classification, Cell biology, Enhancer Elements, Genetic, Phenotype, medicine.anatomical_structure, embryonic structures, Pharyngeal Muscles, Homeobox, Female, Head, Developmental Biology

Abstract

We have identified a new Caenorhabditis elegans NK-2 class homeobox gene, designated ceh-24. Distinct cis-acting elements generate a complex neuronal and mesodermal expression pattern. A promoter-proximal enhancer mediates expression in a single pharyngeal muscle, the donut-shaped m8 cell at the posterior end of the pharynx. A second mesodermal enhancer is active in a set of eight nonstriated vulval muscles used in egg laying. Activation in the egg laying muscles requires an ‘NdE-box’ consensus motif (CATATG) which is related to, but distinct from, the standard E-box motif bound by the MyoD family of transcriptional activators. Ectodermal expression of ceh-24 is limited to a subset of sublateral motor neurons in the head of the animal; this activity requires a cis-acting activator element that is distinct from the control elements for pharyngeal and vulval muscle expression. Activation of ceh-24 in each of the three cell types coincides with the onset of differentiation. Using a set of transposon-induced null mutations, we show that ceh-24 is not essential for the formation of any of these cells. Although ceh-24 mutants have no evident defects under laboratory conditions, the pattern of ceh-24 activity is apparently important for Rhabditid nematodes: the related species C. briggsae contains a close homologue of C. elegans ceh-24 including a highly conserved and functionally equivalent set of cis-acting control signals.

Published

1998

111. The Caenorhabditis elegans NK-2 homeobox gene ceh-22 activates pharyngeal muscle gene expression in combination with pha-1 and is required for normal pharyngeal development

Author

Wei Chen, Andrew Fire, Peter G. Okkema, Christina Haun, and Eunju Ha

Subjects

Transcriptional Activation, animal structures, Pharyngeal muscles, Myosin, Gene expression, medicine, Animals, Drosophila Proteins, Caenorhabditis elegans, Caenorhabditis elegans Proteins, Enhancer, Molecular Biology, Homeodomain Proteins, Regulation of gene expression, biology, Myogenesis, Pharynx, Genes, Homeobox, Gene Expression Regulation, Developmental, biology.organism_classification, Molecular biology, medicine.anatomical_structure, embryonic structures, Pharyngeal Muscles, Transcription Factors, Developmental Biology

Abstract

Pharyngeal muscle development in the nematode Caenorhabditis elegans appears to share similarities with cardiac muscle development in other species. We have previously described CEH-22, an NK-2 class homeodomain transcription factor similar to Drosophila tinman and vertebrate Nkx2-5, which is expressed exclusively in the pharyngeal muscles. In vitro, CEH-22 binds the enhancer from myo-2, a pharyngeal muscle-specific myosin heavy chain gene. In this paper, we examine the role CEH-22 plays in pharyngeal muscle development and gene activation by (a) ectopically expressing ceh-22 in transgenic C. elegans and (b) examining the phenotype of a ceh-22 loss-of-function mutant. These experiments indicate that CEH-22 is an activator of myo-2 expression and that it is required for normal pharyngeal muscle development. However, ceh-22 is necessary for neither formation of the pharyngeal muscles, nor for myo-2 expression. Our data suggest parallel and potentially compensating pathways contribute to pharyngeal muscle differentiation. We also examine the relationship between ceh-22 and the pharyngeal organ-specific differentiation gene pha-1. Mutations in ceh-22 and pha-1 have strongly synergistic effects on pharyngeal muscle gene expression; in addition, a pha-1 mutation enhances the lethal phenotype caused by a mutation in ceh-22. Wild-type pha-1 is not required for the onset of ceh-22 expression but it appears necessary for maintained expression of ceh-22.

Published

1997

112. Distinct Requirements for Somatic and Germline Expression of a Generally Expressed Caernorhabditis elegans Gene

Author

William G. Kelly, Mary K. Montgomery, Andrew Fire, and SiQun Xu

Subjects

Genetics, Sequence Homology, Amino Acid, biology, Transgene, Molecular Sequence Data, Nuclear Proteins, RNA-Binding Proteins, Investigations, biology.organism_classification, Chromosomes, Germline, Conserved sequence, Animals, Genetically Modified, Germ Cells, Essential gene, Gene expression, Animals, Gene silencing, Amino Acid Sequence, Transgenes, Caenorhabditis elegans, Caenorhabditis elegans Proteins, Gene

Abstract

In screening for embryonic-lethal mutations in Caernorhabditis elegans, we defined an essential gene (let-858) that encodes a nuclear protein rich in acidic and basic residues. We have named this product nucampholin. Closely homologous sequences in yeast, plants, and mammals demonstrate strong evolutionary conservation in eukaryotes. Nucampholin resides in all nuclei of C. elegans and is essential in early development and in differentiating tissue. Antisense-mediated depletion of LET-858 activity in early embryos causes a lethal phenotype similar to characterized treatments blocking embryonic gene expression. Using transgene-rescue, we demonstrated the additional requirement for let-858 in the larval germline. The broad requirements allowed investigation of soma-germline differences in gene expression. When introduced into standard transgene arrays, let-858 (like many other C. elegans genes) functions well in soma but poorly in germline. We observed incremental silencing of simple let-858 arrays in thefirstfew generations following transformation and hypothesized that silencing might reflect recognition of arrays as repetitive or heterochromatin-like. To give the transgene a more physiological context, we included an excess of random genomic fragments with the injected DNA. The resulting transgenes show robust expression in both germline and soma. Our results suggest the possibility of concerted mechanisms for silencing unwanted germline expression of repetitive sequences.

Published

1997

113. Unusual DNA packaging characteristics in endoreduplicated Caenorhabditis elegans oocytes defined by in vivo accessibility to an endogenous nuclease activity

Author

James D. McGhee, Barbara Goszczynski, Sam Guoping Gu, and Andrew Fire

Subjects

Genetics, 0303 health sciences, Nuclease, biology, Research, Endogeny, Cell fate determination, biology.organism_classification, Genome, Cell biology, Chromatin, Major sperm protein, 03 medical and health sciences, 0302 clinical medicine, biology.protein, Molecular Biology, 030217 neurology & neurosurgery, Caenorhabditis elegans, 030304 developmental biology, Micrococcal nuclease

Abstract

Background Germ cells in animals are highly specialized to preserve the genome. A distinct set of chromatin structures must be properly established in germ cells to maintain cell fate and genome integrity. We describe DNA-surface interactions in activated Caenorhabditis elegans oocytes that are revealed through the activity of an endogenous nuclease ('endocleavage’). Results Our analysis began with an unexpected observation that a majority (>50%) of DNA from ovulated but unfertilized C. elegans oocytes can be recovered in fragments of approximately 500 base pairs or shorter, cleaved at regular intervals (10 to 11 nt) along the DNA helix. In some areas of the genome, DNA cleavage patterns in these endoreduplicated oocytes appear consistent from cell-to-cell, indicating coherent rotational positioning of the DNA in chromatin. Particularly striking in this analysis are arrays of sensitive sites with a periodicity of approximately 10 bp that persist for several hundred base pairs of genomic DNA, longer than a single nucleosome core. Genomic regions with a strong bias toward a 10-nt periodic occurrence of A(n)/T(n) (so-called PATC regions) appear to exhibit a high degree of rotational constraint in endocleavage phasing, with a strong tendency for the periodic A(n)/T(n) sites to remain on the face of the helix protected from nuclease digestion. Conclusion The present analysis provides evidence for an unusual structure in C. elegans oocytes in which genomic DNA and associated protein structures are coherently linked.

Published

2013

114. Comprehensive whole-genome sequencing of an early-stage primary myelofibrosis patient defines low mutational burden and non-recurrent candidate genes

Author

Rhonda Hewitt, Dana Ng, Carol D. Jones, Michael Snyder, Jason D. Merker, Krishna M. Roskin, James L. Zehnder, Jasmine J. King, Scott D. Boyd, Linda Gojenola, Lawrence M. Okumoto, Athena M. Cherry, Parveen Abidi, Michael Stadler, Tracy I. George, Dianna G. Fisk, Andrew Fire, Bing Zhang, Cuiping Pan, Ramona A. Hoh, Jason Gotlib, and Michael J. Clark

Subjects

Genetics, Male, Mutation, Essential thrombocythemia, Point mutation, Nonsense mutation, Genetic Variation, Hematology, Articles, Biology, Middle Aged, medicine.disease_cause, medicine.disease, Genome, Germline mutation, Primary Myelofibrosis, medicine, Humans, Myelofibrosis, Gene, Cells, Cultured, Genetic Association Studies, Genome-Wide Association Study

Abstract

In order to identify novel somatic mutations associated with classic BCR/ABL1-negative myeloproliferative neoplasms, we performed high-coverage genome sequencing of DNA from peripheral blood granulocytes and cultured skin fibroblasts from a patient with MPL W515K-positive primary myelofibrosis. The primary myelofibrosis genome had a low somatic mutation rate, consistent with that observed in similar hematopoietic tumor genomes. Interfacing of whole-genome DNA sequence data with RNA expression data identified three somatic mutations of potential functional significance: i) a nonsense mutation in CARD6, implicated in modulation of NF-kappaB activation; ii) a 19-base pair deletion involving a potential regulatory region in the 5'-untranslated region of BRD2, implicated in transcriptional regulation and cell cycle control; and iii) a non-synonymous point mutation in KIAA0355, an uncharacterized protein. Additional mutations in three genes (CAP2, SOX30, and MFRP) were also evident, albeit with no support for expression at the RNA level. Re-sequencing of these six genes in 178 patients with polycythemia vera, essential thrombocythemia, and myelofibrosis did not identify recurrent somatic mutations in these genes. Finally, we describe methods for reducing false-positive variant calls in the analysis of hematologic malignancies with a low somatic mutation rate. This trial is registered with ClinicalTrials.gov (NCT01108159).

Published

2013

115. The transcription start site landscape of C. elegans

Author

Thomas Blumenthal, Taro Saito, Shinichi Morishita, Michael Stadler, John Morton, Sam Guoping Gu, Andrew Fire, and Shin-ichi Hashimoto

Subjects

Resource, Sequence analysis, Population, Trans-splicing, Helminth genetics, RNA polymerase II, Biology, Primary transcript, Trans-Splicing, Genetics, Animals, RNA, Messenger, education, Caenorhabditis elegans, Promoter Regions, Genetic, Gene, Genetics (clinical), Conserved Sequence, Genes, Helminth, education.field_of_study, Base Sequence, Molecular Sequence Annotation, Sequence Analysis, DNA, biology.organism_classification, Gene Expression Regulation, Organ Specificity, biology.protein, RNA, Helminth, Transcription Initiation Site, 5' Untranslated Regions

Abstract

More than half of Caenorhabditis elegans pre-mRNAs lose their original 5′ ends in a process termed “trans-splicing” in which the RNA extending from the transcription start site (TSS) to the site of trans-splicing of the primary transcript, termed the “outron,” is replaced with a 22-nt spliced leader. This complicates the mapping of TSSs, leading to a lack of available TSS mapping data for these genes. We used growth at low temperature and nuclear isolation to enrich for transcripts still containing outrons, applying a modified SAGE capture procedure and high-throughput sequencing to characterize 5′ termini in this transcript population. We report from this data both a landscape of 5′-end utilization for C. elegans and a representative collection of TSSs for 7351 trans-spliced genes. TSS distributions for individual genes were often dispersed, with a greater average number of TSSs for trans-spliced genes, suggesting that trans-splicing may remove selective pressure for a single TSS. Upstream of newly defined TSSs, we observed well-known motifs (including TATAA-box and SP1) as well as novel motifs. Several of these motifs showed association with tissue-specific expression and/or conservation among six worm species. Comparing TSS features between trans-spliced and non-trans-spliced genes, we found stronger signals among outron TSSs for preferentially positioning of flanking nucleosomes and for downstream Pol II enrichment. Our data provide an enabling resource for both experimental and theoretical analysis of gene structure and function in C. elegans.

Published

2013

116. Convergent antibody signatures in human dengue

Author

Poornima Parameswaran, Karen L. Artiles, Kim R. McGowan, Birgitte B. Simen, Ji-Yeun Lee, Katherine K.L. Jackson, Nader Pourmand, Angel Balmaseda, Simona Zompi, Scott D. Boyd, Eva Harris, Krishna M. Roskin, Yi Liu, Andrew Fire, Daphne Koller, Maria José Vargas, Bozena Hanczaruk, Muhammad Tariq, and Vaishali P. Dixit

Subjects

Cancer Research, Secondary infection, Complementarity determining region, Dengue virus, medicine.disease_cause, Antibodies, Viral, Microbiology, Article, Dengue fever, Dengue, 03 medical and health sciences, 0302 clinical medicine, Immune system, Immunology and Microbiology(all), Virology, medicine, Humans, Molecular Biology, B cell, 030304 developmental biology, 0303 health sciences, B-Lymphocytes, biology, Dengue Virus, medicine.disease, Complementarity Determining Regions, 3. Good health, medicine.anatomical_structure, Immunology, biology.protein, Parasitology, Viral disease, Antibody, Immunologic Memory, 030215 immunology

Abstract

SummaryDengue is the most prevalent mosquito-borne viral disease in humans, and the lack of early prognostics, vaccines, and therapeutics contributes to immense disease burden. To identify patterns that could be used for sequence-based monitoring of the antibody response to dengue, we examined antibody heavy-chain gene rearrangements in longitudinal peripheral blood samples from 60 dengue patients. Comparing signatures between acute dengue, postrecovery, and healthy samples, we found increased expansion of B cell clones in acute dengue patients, with higher overall clonality in secondary infection. Additionally, we observed consistent antibody sequence features in acute dengue in the highly variable major antigen-binding determinant, complementarity-determining region 3 (CDR3), with specific CDR3 sequences highly enriched in acute samples compared to postrecovery, healthy, or non-dengue samples. Dengue thus provides a striking example of a human viral infection where convergent immune signatures can be identified in multiple individuals. Such signatures could facilitate surveillance of immunological memory in communities.

Published

2013

117. Conserved translatome remodeling in nematode species executing a shared developmental transition

Author

Andrew Fire and Michael Stadler

Subjects

Cancer Research, Translational efficiency, lcsh:QH426-470, Biology, Diapause, Ribosome, Evolution, Molecular, 03 medical and health sciences, 0302 clinical medicine, Species Specificity, Gene expression, Translational regulation, Genetics, Animals, RNA, Messenger, Ribosome profiling, Molecular Biology, Phylogeny, Genetics (clinical), Ecology, Evolution, Behavior and Systematics, 030304 developmental biology, Regulation of gene expression, 0303 health sciences, Genome, Gene Expression Regulation, Developmental, biology.organism_classification, Cell biology, Caenorhabditis, lcsh:Genetics, Protein Biosynthesis, Ribosomes, 030217 neurology & neurosurgery, Research Article

Abstract

Nematodes of the genus Caenorhabditis enter a developmental diapause state after hatching in the absence of food. To better understand the relative contributions of distinct regulatory modalities to gene expression changes associated with this developmental transition, we characterized genome-wide changes in mRNA abundance and translational efficiency associated with L1 diapause exit in four species using ribosome profiling and mRNA-seq. We found a strong tendency for translational regulation and mRNA abundance processes to act synergistically, together effecting a dramatic remodeling of the gene expression program. While gene-specific differences were observed between species, overall translational dynamics were broadly and functionally conserved. A striking, conserved feature of the response was strong translational suppression of ribosomal protein production during L1 diapause, followed by activation upon resumed development. On a global scale, ribosome footprint abundance changes showed greater similarity between species than changes in mRNA abundance, illustrating a substantial and genome-wide contribution of translational regulation to evolutionary maintenance of stable gene expression., Author Summary Working with a set of four related animal species, we have studied a conserved developmental and metabolic transition at the level of protein production and regulation of RNA levels. Strikingly, regulatory effects at the level of RNA accumulation and protein synthesis act together to achieve the observed metabolic shift. In addition to a general conservation of the underlying basis for the regulation of individual genes, alterations of these two processes—mRNA production and protein synthesis—can compensate for one another during evolution to maintain stable amounts of functional gene products. A salient feature of the observed regulation was the storage of idle mRNAs encoding key members of the protein synthesis machinery during metabolic arrest (diapause). Maintenance of this pool facilitates re-activation upon feeding, with the rapid regeneration of protein synthesis capacity an early and critical function during adaptation to a major metabolic shift.

Published

2013

118. An inductive interaction in 4-cell stage C. elegans embryos involves APX-1 expression in the signalling cell

Author

James R Priess, Andrew Fire, Craig C. Mello, Mary K. Montgomery, and Katherine M. Mickey

Subjects

Male, Blastomeres, genetic structures, Period (gene), Mutant, Biology, medicine.disease_cause, Sodium Channels, medicine, Animals, Caenorhabditis elegans, Caenorhabditis elegans Proteins, Molecular Biology, Embryonic Induction, Genetics, Mutation, Embryogenesis, Membrane Proteins, food and beverages, Embryo, Blastomere, Cell biology, RNA, Female, Signal transduction, Signal Transduction, Developmental Biology

Abstract

During the 4-cell stage of C. elegans embryogenesis, the P2 blastomere provides a signal that allows two initially equivalent sister blastomeres, called ABa and ABp, to adopt different fates. Preventing P2 signalling in wild-type embryos results in defects in ABp development that are similar to those caused by mutations in the glp-1 and apx-1 genes, which are homologs of the Drosophila genes Notch and Delta, respectively. Previous studies have shown that GLP-1 protein is expressed in 4-cell stage embryos in both ABa and ABp. In this report, we show that APX-1 protein is expressed in the P2 blastomere and that a temperature-sensitive apx-1 mutant has a temperature-sensitive period between the 4-cell and 8-cell stages. We propose that APX-1 is part or all of the P2 signal that induces ABp to adopt a fate different than ABa.

Published

1996

119. Rolling replication of short DNA circles

Author

SiQun Xu and Andrew Fire

Subjects

DNA Replication, DNA Ligases, Molecular Sequence Data, chemistry.chemical_compound, Tandem repeat, Escherichia coli, Direct repeat, Repeated sequence, Repetitive Sequences, Nucleic Acid, Genetics, Multidisciplinary, Base Sequence, Models, Genetic, biology, DNA replication, DNA Polymerase I, Biological Evolution, Oligodeoxyribonucleotides, chemistry, Rolling circle replication, biology.protein, DNA, Circular, DNA polymerase I, Systematic evolution of ligands by exponential enrichment, DNA, Research Article

Abstract

Natural genes and proteins often contain tandemly repeated sequence motifs that dramatically increase physiological specificity and activity. Given the selective value of such repeats, it is likely that several different mechanisms have been responsible for their generation. One mechanism that has been shown to generate relatively long tandem repeats (in the kilobase range) is rolling circle replication. In this communication, we demonstrate that rolling circle synthesis in a simple enzymatic system can produce tandem repeats of monomers as short as 34 bp. In addition to suggesting possible origins for natural tandem repeats, these observations provide a facile means for constructing libraries of repeated motifs for use in "in vitro evolution" experiments designed to select molecules with defined biological or chemical properties.

Published

1995

120. 289. Sequence Modified Antibiotic Resistance Genes Provide Sustained Plasmid Mediated Transgene Expression in Mammals

Author

Jiamiao Lu, Feijie Zhang, Andrew Fire, and Mark Kay

Subjects

Pharmacology, Drug Discovery, Genetics, Molecular Medicine, Molecular Biology

Published

2016

121. Antibody lineages with evidence of somatic hypermutation persisting for >4 years in a South African subject with broad neutralizing activity

Author

Thaddeus C. Gurley, Hua-Xin Liao, Drinker, Joshua D. Amos, R Parks, Kyunga Seo, Krissey E. Lloyd, Georgia D. Tomaras, Tho D. Pham, Chun Yen Tsao, Ramona A. Hoh, Scott D. Boyd, Ji-Yeun Lee, Krishna M. Roskin, Lawrence C. Armand, S Wang, Lynn Morris, Andrew Fire, Thomas B. Kepler, Ashley M. Trama, Josh A Eudailey, Elin S. Gray, Barton F. Haynes, Garnett Kelsoe, Katherine J. L. Jackson, Mattia Bonsignori, and M. A. Moody

Subjects

lcsh:Immunologic diseases. Allergy, Infectious Diseases, Virology, Poster Presentation, biology.protein, Somatic hypermutation, Biology, Antibody, lcsh:RC581-607, Bioinformatics

Abstract

Antibody lineages with evidence of somatic hypermutation persisting for >4 years in a South African subject with broad neutralizing activity M Moody, AM Trama, M Bonsignori, C Tsao, MS Drinker, TC Gurley, JD Amos, JA Eudailey, LC Armand, R Parks, KE Lloyd, S Wang, K Seo, J Lee, KJ Jackson, R Hoh, T Pham, KM Roskin, SD Boyd, AZ Fire, ES Gray, L Morris, H Liao, GD Tomaras, TB Kepler, G Kelsoe, BF Haynes

Published

2012

122. Immunobiology of naïve and genetically-modified HLA I knockdown human embryonic stem cells

Author

H. Reichenspurner, Tobias Deuse, Sonja Schrepfer, X. Hua, Mark A. Kay, Martina Seifert, Neil Phillips, H.-D. Volk, D Tyan, Joachim Velden, P.S. Tsao, Andrew Fire, Robert C. Robbins, and T Eiermann

Subjects

Pulmonary and Respiratory Medicine, Gene knockdown, business.industry, Immunology, Medicine, Surgery, Cardiology and Cardiovascular Medicine, business, Embryonic stem cell, Genetically modified organism, Cell biology

Published

2012

123. Elements Regulating Cell- and Stage-Specific Expression of the C. elegans MyoD Family Homolog hlh-1

Author

Si Qun Xu, Michael Krause, Andrew Fire, Susan M. W. Harrison, and Lihsia Chen

Subjects

Caenorhabditis briggsae, Blastomeres, Embryo, Nonmammalian, Recombinant Fusion Proteins, Molecular Sequence Data, Gene Expression, Muscle Proteins, Regulatory Sequences, Nucleic Acid, Muscle Development, MyoD, Species Specificity, Sequence Homology, Nucleic Acid, Animals, Amino Acid Sequence, Caenorhabditis elegans, Caenorhabditis elegans Proteins, Molecular Biology, Gene, Conserved Sequence, MyoD Protein, Sequence Deletion, Gene Rearrangement, Genetics, Regulation of gene expression, Reporter gene, Base Sequence, biology, Muscles, Nuclear Proteins, Helminth Proteins, Cell Biology, Gene rearrangement, beta-Galactosidase, biology.organism_classification, Introns, Gene Expression Regulation, Myogenic Regulatory Factors, Regulatory sequence, Myogenic regulatory factors, Transcription Factors, Developmental Biology

Abstract

We investigated the cis-acting sequences regulating expression of the Caenorhabditis elegans gene hlh-1, a homolog of the MyoD family of myogenic regulatory factors. The hlh-1 gene is expressed in mature body wall muscle, in clonal muscle precursors, in a set of early embryonic blastomeres (the MS-granddaughters), and in six glial-like cells called GLRs. The entire natural hlh-1 expression pattern is recapitulated in transgenic animals containing an hlh-1::lacZ fusion with 5.1 kb of hlh-1 sequences beginning upstream of the coding region and extending into the second exon. Deletions and rearrangements in this 5.1-kb sequence were assayed for their effects on reporter gene expression in transgenic animals. Deletions removing a segment 434-550 bp upstream of the coding region resulted in a loss of all aspects of the expression pattern, suggesting that at least one common regulatory factor is required for all expression. Deletions of other regulatory elements affected distinct aspects of the expression pattern; hence, each expression subpattern exhibits a different set of sequence requirements. Interspecies sequence comparison and lacZ expression constructs with the related nematode Caenorhabditis briggsae indicated that the C. briggsae and C. elegans genes contain equivalent sets of control signals. The results from this work implicate the hlh-1 promoter as an integration point for diverse temporal and spatial control signals.

Published

1994

124. The Caenorhabditis elegans NK-2 class homeoprotein CEH-22 is involved in combinatorial activation of gene expression in pharyngeal muscle

Author

Andrew Fire and Peter G. Okkema

Subjects

DNA Mutational Analysis, Molecular Sequence Data, Myosins, Biology, MyoD, Pharyngeal muscles, Myosin, Morphogenesis, medicine, Animals, Caenorhabditis elegans, Enhancer, Molecular Biology, Base Sequence, Myogenesis, Muscles, Pharynx, Genes, Homeobox, biology.organism_classification, Molecular biology, Enhancer Elements, Genetic, medicine.anatomical_structure, Gene Expression Regulation, Homeobox, Developmental Biology

Abstract

The pharyngeal muscles of Caenorhabditis elegans are single sarcomere muscles used for feeding. Like vertebrate cardiac and smooth muscles, C. elegans pharyngeal muscle does not express any of the known members of the MyoD family of myogenic factors. To identify mechanisms regulating gene expression in this tissue, we have characterized a pharyngeal muscle-specific enhancer from myo-2, a myosin heavy chain gene expressed exclusively in pharyngeal muscle. Assaying enhancer function in transgenic animals, we identified three subelements, designated A, B and C, that contribute to myo-2 enhancer activity. These subelements are individually inactive; however, any combination of two or more subelements forms a functional enhancer. The B and C subelements have distinct cell type specificities. A duplication of B activates transcription in a subset of pharyngeal muscles (m3, m4, m5 and m7). A duplication of C activates transcription in all pharyngeal cells, muscle and non-muscle. Thus, the activity of the myo-2 enhancer is regulated by a combination of pharyngeal muscle-type-specific and organ-specific signals. Screening a cDNA expression library, we identified a gene encoding an NK-2 class homeodomain protein, CEH-22, that specifically binds a site necessary for activity of the B subelement. CEH-22 protein is first expressed prior to myogenic differentiation and is present in the same subset of pharyngeal muscles in which B is active. Expression continues throughout embryonic and larval development. This expression pattern suggests CEH-22 plays a key role in pharyngeal muscle-specific activity of the myo-2 enhancer.

Published

1994

125. Loss of the Putative RNA-Directed RNA Polymerase RRF-3 Makes C. elegans Hypersensitive to RNAi

Author

Andrew Fire, Ronald H.A. Plasterk, Marcel Tijsterman, Michael L. Nonet, Susan Parrish, Julie Ahringer, Sandhya P. Koushika, and Femke Simmer

Subjects

Mutant, Biology, General Biochemistry, Genetics and Molecular Biology, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, RNA interference, RNA polymerase, Animals, Caenorhabditis elegans, Gene, Loss function, RNA, Double-Stranded, 030304 developmental biology, Genetics, 0303 health sciences, Agricultural and Biological Sciences(all), Biochemistry, Genetics and Molecular Biology(all), fungi, RNA, RNA-Dependent RNA Polymerase, Phenotype, Reverse genetics, chemistry, RNA Interference, General Agricultural and Biological Sciences, 030217 neurology & neurosurgery

Abstract

RNA interference (RNAi) is a broadly used reverse genetics method in C. elegans [1]. Unfortunately, RNAi does not inhibit all genes [2, 3]. We show that loss of function of a putative RNA-directed RNA polymerase (RdRP) of C. elegans, RRF-3, results in a substantial enhancement of sensitivity to RNAi in diverse tissues. This is particularly striking in the nervous system; neurons that are generally refractory to RNAi in a wild-type genetic background can respond effectively to interference in an rrf-3 mutant background. These data provide the first indication of physiological negative modulation of the RNAi response and implicate an RdRP-related factor in this effect. The rrf-3 strain can be useful to study genes that, in wild-type, do not show a phenotype after RNAi, and it is probably the strain of choice for genome-wide RNAi screens.

Published

2002

126. The inference of phased haplotypes for the immunoglobulin H chain V region gene loci by analysis of VDJ gene rearrangements

Author

Zhiliang Chen, Bruno A. Gaëta, Scott D. Boyd, Lyndon N. Zhang, Mark M. Tanaka, Katherine J. L. Jackson, Andrew Fire, Andrew M. Collins, Marie J. Kidd, and Yan Wang

Subjects

Heterozygote, Genotype, Immunology, Population, Immunoglobulin Variable Region, Locus (genetics), Biology, Article, Immunology and Allergy, Humans, Allele, education, Gene, Genetics, Gene Rearrangement, education.field_of_study, Polymorphism, Genetic, Genes, Immunoglobulin, Haplotype, Gene rearrangement, V(D)J Recombination, Haplotypes, Genetic Loci, IGHD, IGHV@, Immunoglobulin Heavy Chains

Abstract

The existence of many highly similar genes in the lymphocyte receptor gene loci makes them difficult to investigate, and the determination of phased “haplotypes” has been particularly problematic. However, V(D)J gene rearrangements provide an opportunity to infer the association of Ig genes along the chromosomes. The chromosomal distribution of H chain genes in an Ig genotype can be inferred through analysis of VDJ rearrangements in individuals who are heterozygous at points within the IGH locus. We analyzed VDJ rearrangements from 44 individuals for whom sufficient unique rearrangements were available to allow comprehensive genotyping. Nine individuals were identified who were heterozygous at the IGHJ6 locus and for whom sufficient suitable VDJ rearrangements were available to allow comprehensive haplotyping. Each of the 18 resulting IGHV│IGHD│IGHJ haplotypes was unique. Apparent deletion polymorphisms were seen that involved as many as four contiguous, functional IGHV genes. Two deletion polymorphisms involving multiple contiguous IGHD genes were also inferred. Three previously unidentified gene duplications were detected, where two sequences recognized as allelic variants of a single gene were both inferred to be on a single chromosome. Phased genomic data brings clarity to the study of the contribution of each gene to the available repertoire of rearranged VDJ genes. Analysis of rearrangement frequencies suggests that particular genes may have substantially different yet predictable propensities for rearrangement within different haplotypes. Together with data highlighting the extent of haplotypic variation within the population, this suggests that there may be substantial variability in the available Ab repertoires of different individuals.

Published

2011

127. High-throughput VDJ sequencing for quantification of minimal residual disease in chronic lymphocytic leukemia and immune reconstitution assessment

Author

Michael N. Mindrinos, Eleanor L. Marshall, Wenzhong Xiao, Randall Armstrong, Aaron C Logan, Bita Sahaf, Ismael Buño, Chunlin Wang, James L. Zehnder, Scott D. Boyd, Ronald W. Davis, Kenneth I. Weinberg, Carol D. Jones, Hong Gao, David B. Miklos, and Andrew Fire

Subjects

Oncology, medicine.medical_specialty, Neoplasm, Residual, medicine.medical_treatment, Chronic lymphocytic leukemia, Oligonucleotides, Hematopoietic stem cell transplantation, Biology, Polymerase Chain Reaction, Sensitivity and Specificity, law.invention, law, immune system diseases, Internal medicine, hemic and lymphatic diseases, medicine, Secondary Prevention, Humans, Transplantation, Homologous, Polymerase chain reaction, B cell, Multidisciplinary, Hematopoietic Stem Cell Transplantation, Cancer, Computational Biology, High-Throughput Nucleotide Sequencing, Biological Sciences, medicine.disease, Flow Cytometry, Minimal residual disease, Leukemia, Lymphocytic, Chronic, B-Cell, Transplantation, Leukemia, medicine.anatomical_structure, Immunology, Immunoglobulin Heavy Chains

Abstract

The primary cause of poor outcome following allogeneic hematopoietic cell transplantation (HCT) for chronic lymphocytic leukemia (CLL) is disease recurrence. Detection of increasing minimal residual disease (MRD) following HCT may permit early intervention to prevent clinical relapse; however, MRD quantification remains an uncommon diagnostic test because of logistical and financial barriers to widespread use. Here we describe a method for quantifying CLL MRD using widely available consensus primers for amplification of all Ig heavy chain (IGH) genes in a mixture of peripheral blood mononuclear cells, followed by high-throughput sequencing (HTS) for disease-specific IGH sequence quantification. To achieve accurate MRD quantification, we developed a systematic bioinformatic methodology to aggregate cancer clone sequence variants arising from systematic and random artifacts occurring during IGH-HTS. We then compared the sensitivity of IGH-HTS, flow cytometry, and allele-specific oligonucleotide PCR for MRD quantification in 28 samples collected from 6 CLL patients following allogeneic HCT. Using amplimer libraries generated with consensus primers from patient blood samples, we demonstrate the sensitivity of IGH-HTS with 454 pyrosequencing to be 10 −5 , with a high correlation between quantification by allele-specific oligonucleotide PCR and IGH-HTS ( r = 0.85). From the same dataset used to quantify MRD, IGH-HTS also allowed us to profile IGH repertoire reconstitution after HCT—information not provided by the other MRD methods. IGH-HTS using consensus primers will broaden the availability of MRD quantification in CLL and other B cell malignancies, and this approach has potential for quantitative evaluation of immune diversification following transplant and nontransplant therapies.

Published

2011

128. Wobble base-pairing slows in vivo translation elongation in metazoans

Author

Michael Stadler and Andrew Fire

Subjects

Reading frame, Peptide Chain Elongation, Translational, Wobble base pair, Biology, RNA, Transfer, Report, Prokaryotic translation, Anticodon, Animals, Humans, Ribosome profiling, RNA, Messenger, Codon degeneracy, Caenorhabditis elegans, Codon, Molecular Biology, Base Pairing, Genetics, Binding Sites, Base Sequence, Gene Expression Profiling, Translation (biology), Stop codon, Gene Expression Regulation, Codon usage bias, Ribosomes, HeLa Cells

Abstract

In the universal genetic code, most amino acids can be encoded by multiple trinucleotide codons, and the choice among available codons can influence position-specific translation elongation rates. By using sequence-based ribosome profiling, we obtained transcriptome-wide profiles of in vivo ribosome occupancy as a function of codon identity in Caenorhabditis elegans and human cells. Particularly striking in these profiles was a universal trend of higher ribosome occupancy for codons translated via G:U wobble base-pairing compared with synonymous codons that pair with the same tRNA family using G:C base-pairing. These data support a model in which ribosomal translocation is slowed at wobble codon positions.

Published

2011

129. Human Leukocyte Antigen I Knockdown Human Embryonic Stem Cells Induce Host Ignorance and Achieve Prolonged Xenogeneic Survival

Author

Thomas Eiermann, Andrew Fire, Neil Phillips, Joachim Velden, Mark A. Kay, Dolly B. Tyan, Hans-Dieter Volk, Philip S. Tsao, Xiaoqin Hua, Tobias Deuse, Sonja Schrepfer, Robert C. Robbins, Martina Seifert, and Hermann Reichenspurner

Subjects

Male, Time Factors, Cell Survival, T-Lymphocytes, Genetic enhancement, Transplantation, Heterologous, Mice, Nude, Mice, SCID, Human leukocyte antigen, Intrabody, Immune tolerance, Mice, HLA Antigens, In vivo, Physiology (medical), Immune Tolerance, Animals, Humans, Cells, Cultured, Embryonic Stem Cells, Immunosuppression Therapy, Mice, Knockout, Mice, Inbred BALB C, Gene knockdown, biology, Graft Survival, equipment and supplies, Embryonic stem cell, Transplantation, Gene Knockdown Techniques, Models, Animal, embryonic structures, Immunology, biology.protein, Cancer research, Cardiology and Cardiovascular Medicine, Stem Cell Transplantation

Abstract

Background— Although human embryonic stem cells (hESC) have enormous potential for cell replacement therapy of heart failure, immune rejection of hESC derivatives inevitably would occur after transplantation. We therefore aimed to generate a hypoantigeneic hESC line with improved survival characteristics. Methods and Results— Using various in vivo, nonischemic, hindlimb xenotransplant models (immunocompetent and defined immunodefective mouse strains) as well as human in vitro T-cell and natural killer (NK)-cell assays, we revealed a central role for T cells in mediating hESC rejection. The NK-cell susceptibility of hESC in vivo was found to be low, and the NK response to hESC challenge in vitro was negligible. To reduce the antigenicity of hESC, we successfully generated human leukocyte antigen (HLA) I knockdown cells (hESC siRNA+IB ) using both HLA I RNA interference (siRNA) and intrabody (IB) technology. HLA I expression was ≈99% reduced after 7 days and remained low for weeks. Cellular immune recognition of these hESC siRNA+IB was strongly reduced in both xenogeneic and allogeneic settings. Immune rejection was profoundly mitigated after hESC siRNA+IB transplantation into immunocompetent mice, and even long-term graft survival was achieved in one third of the animals without any immunosuppression. The survival benefit of hESC siRNA+IB was further confirmed under ischemic conditions in a left anterior descending coronary artery ligation model. Conclusions— HLA I knockdown hESC siRNA+IB provoke T-cell ignorance and experience largely mitigated xenogeneic rejection. By generating hypoantigeneic hESC lines, the generation of acceptable hESC derivatives may become a practical concept and push cell replacement strategies forward.

Published

2011

130. Immunobiology of naïve and genetically modified HLA-class-I-knockdown human embryonic stem cells

Author

Hermann Reichenspurner, Martina Seifert, Mark A. Kay, Neil Phillips, Dolly B. Tyan, Hans-Dieter Volk, Thomas Eiermann, Robert C. Robbins, Tobias Deuse, Sonja Schrepfer, Andrew Fire, Joachim Velden, Philip S. Tsao, and Xiaoqin Hua

Subjects

Graft Rejection, Male, T cell, Cell, Transplantation, Heterologous, Human leukocyte antigen, Mice, SCID, Mice, Immune system, HLA Antigens, medicine, Animals, Humans, reproductive and urinary physiology, Embryonic Stem Cells, Mice, Inbred BALB C, biology, Cell Biology, T helper cell, equipment and supplies, Embryonic stem cell, Transplantation, medicine.anatomical_structure, Gene Knockdown Techniques, embryonic structures, Immunology, biology.protein, biological phenomena, cell phenomena, and immunity, Antibody

Abstract

Human embryonic stem cells (hESCs) can serve as a universal cell source for emerging cell or tissue replacement strategies, but immune rejection of hESC derivatives remains an unsolved problem. Here, we sought to describe the mechanisms of rejection for naïve hESCs and upon HLA class I (HLA I) knockdown (hESCKD). hESCs were HLA I-positive but negative for HLA II and co-stimulatory molecules. Transplantation of naïve hESC into immunocompetent Balb/c mice induced substantial T helper cell 1 and 2 (Th1 and Th2) responses with rapid cell death, but hESCs survived in immunodeficient SCID-beige recipients. Histology revealed mainly macrophages and T cells, but only scattered natural killer (NK) cells. A surge of hESC-specific antibodies against hESC class I, but not class II antigens, was observed. Using HLA I RNA interference and intrabody technology, HLA I surface expression of hESCKD was 88%–99% reduced. T cell activation after hESCKD transplantation into Balb/c was significantly diminished, antibody production was substantially alleviated, the levels of graft-infiltrating immune cells were reduced and the survival of hESCKD was prolonged. Because of their very low expression of stimulatory NK ligands, NK-susceptibility of naïve hESCs and hESCKD was negligible. Thus, HLA I recognition by T cells seems to be the primary mechanism of hESC recognition, and T cells, macrophages and hESC-specific antibodies participate in hESC killing.

Published

2011

131. Chromatin-Associated Periodicity in Genetic Variation Downstream of Transcriptional Start Sites

Author

Shin Sasaki, Cecilia C. Mello, Atsuko Shimada, Yoichiro Nakatani, Shin-ichi Hashimoto, Masako Ogawa, Kouji Matsushima, Sam Guoping Gu, Masahiro Kasahara, Budrul Ahsan, Atsushi Sasaki, Taro Saito, Yutaka Suzuki, Sumio Sugano, Yuji Kohara, Hiroyuki Takeda, Andrew Fire, and Shinichi Morishita

Published

2011

132. The novel metallothionein genes of Caenorhabditis elegans. Structural organization and inducible, cell-specific expression

Author

D. Dixon, Jonathan H. Freedman, Andrew Fire, Charles S. Rubin, and L.W. Slice

Subjects

Reporter gene, biology, Transgene, Intron, Promoter, Cell Biology, biology.organism_classification, Biochemistry, Molecular biology, Fusion gene, Gene expression, Molecular Biology, Gene, psychological phenomena and processes, Caenorhabditis elegans

Abstract

Two genes (mtl-1 and mtl-2) that encode the novel metallothioneins (MTs) of Caenorhabditis elegans (CeMTs) were cloned and characterized. Both genes contain a single intron that interrupts codon 6 and short 3‘-untranslated regions. However, their promotor regions are distinctively non-homologous. The mtl-2 promoter contains a TATAA box and a single putative metal regulatory element. These elements are absent in the mtl-1 promoter. Nevertheless, both CeMT1 and CeMT2 mRNAs are induced by cadmium and contain precisely initiated, 5‘-untranslated sequences. The inducibility and cell type specificity of metallothionein gene expression were investigated in transgenic C. elegans that carry the lacZ (beta-galactosidase) reporter gene under the control of an mtl-1 or mtl-2 promoter sequence. Upon treatment of transgenic C. elegans with cadmium or heat stress, the mtl-2:lacZ fusion gene is abundantly and exclusively expressed in the intestinal cells of larvae and adult animals. Expression is not detected in the absence of metal or heat shock. In contrast, an mtl-1:lacZ construct is constitutively expressed in the pharynx and induced by cadmium and heat shock in the intestinal cells of C. elegans larvae. The metal-inducible expression of the mtl-1:lacZ gene is attenuated in adult transgenic nematodes. Thus, the activity of each mtl promoter is modulated by metals as well as developmental and environmental factors.

Published

1993

133. Up-regulated Dicer expression in patients with cutaneous melanoma

Author

Soheil S. Dadras, Elizabeth Fleming, David S. Cassarino, Helen Swede, Andrew Fire, and Zhihai Ma

Subjects

Ribonuclease III, Melanomas, Pathology, Skin Neoplasms, lcsh:Medicine, Dermatologic Pathology, Metastasis, RNA interference, Gene expression, Basic Cancer Research, lcsh:Science, Melanoma, Skin Tumors, Multidisciplinary, biology, Reverse Transcriptase Polymerase Chain Reaction, Malignant Melanoma, Basal Cell Carcinomas, Squamous Cell Carcinomas, Immunohistochemistry, Up-Regulation, Oncology, Medicine, Epigenetics, Basal Cell Carcinoma, Research Article, medicine.medical_specialty, Histology, Malignant Skin Neoplasms, Dermatology, Cell Line, Diagnostic Medicine, microRNA, medicine, Genetics, Cancer Genetics, Humans, Squamous Cell Carcinoma, Biology, lcsh:R, Cancer, Cancers and Neoplasms, medicine.disease, enzymes and coenzymes (carbohydrates), RNA processing, Tumor progression, Cutaneous melanoma, biology.protein, Cancer research, Benign Skin Neoplasms, lcsh:Q, Biomarkers, Dicer, General Pathology

Abstract

Background MicroRNAs (miRNAs) are small non-coding RNAs (18–24 nucleotides) that have recently been shown to regulate gene expression during cancer progression. Dicer, a central enzyme in the multi-component miRNA biogenesis pathway, is involved in cutting precursor miRNAs to functionally mature forms. Emerging evidence shows that Dicer expression is deregulated in some human malignancies and it correlates with tumor progression, yet this role has not yet been investigated in skin cancers. Methods and Findings Using an anti-human monoclonal antibody against Dicer and immunohistochemistry, we compared the expression of Dicer protein among 404 clinically annotated controls and skin tumors consisting of melanocytic nevi (n = 71), a variety of melanomas (n = 223), carcinomas (n = 73) and sarcomas (n = 12). Results showed a cell-specific up-regulated Dicer in 81% of cutaneous, 80% of acrolentiginous and 96% of metastatic melanoma specimens compared to carcinoma or sarcoma specimens (P

Published

2010

134. Distributed probing of chromatin structure in vivo reveals pervasive chromatin accessibility for expressed and non-expressed genes during tissue differentiation in C. elegans

Author

Sam Guoping Gu, Ky Sha, Jamie Fleenor, Luiz C Pantalena-Filho, Daniel Blanchard, Amy Goh, Chaya Krishna, and Andrew Fire

Subjects

lcsh:QH426-470, lcsh:Biotechnology, Chromatin remodeling, Histones, 03 medical and health sciences, lcsh:TP248.13-248.65, Genetics, Animals, Nucleosome, Caenorhabditis elegans, DNA Modification Methylases, Gene, ChIA-PET, 030304 developmental biology, Genome, Helminth, 0303 health sciences, biology, Methodology Article, Gene Expression Profiling, 030302 biochemistry & molecular biology, Gene Expression Regulation, Developmental, Sequence Analysis, DNA, Epigenome, Chromatin, Cell biology, lcsh:Genetics, Histone, biology.protein, DNA microarray, Biotechnology

Abstract

Background Tissue differentiation is accompanied by genome-wide changes in the underlying chromatin structure and dynamics, or epigenome. By controlling when, where, and what regulatory factors have access to the underlying genomic DNA, the epigenome influences the cell's transcriptome and ultimately its function. Existing genomic methods for analyzing cell-type-specific changes in chromatin generally involve two elements: (i) a source for purified cells (or nuclei) of distinct types, and (ii) a specific treatment that partitions or degrades chromatin by activity or structural features. For many cell types of great interest, such assays are limited by our inability to isolate the relevant cell populations in an organism or complex tissue containing an intertwined mixture of other cells. This limitation has confined available knowledge of chromatin dynamics to a narrow range of biological systems (cell types that can be sorted/separated/dissected in large numbers and tissue culture models) or to amalgamations of diverse cell types (tissue chunks, whole organisms). Results Transgene-driven expression of DNA/chromatin modifying enzymes provides one opportunity to query chromatin structures in expression-defined cell subsets. In this work we combine in vivo expression of a bacterial DNA adenine methyltransferase (DAM) with high throughput sequencing to sample tissue-specific chromatin accessibility on a genome-wide scale. We have applied the method (DALEC: Direct Asymmetric Ligation End Capture) towards mapping a cell-type-specific view of genome accessibility as a function of differentiated state. Taking advantage of C. elegans strains expressing the DAM enzyme in diverse tissues (body wall muscle, gut, and hypodermis), our efforts yield a genome-wide dataset measuring chromatin accessibility at each of 538,000 DAM target sites in the C. elegans (diploid) genome. Conclusions Validating the DALEC mapping results, we observe a strong association between observed coverage by nucleosomes and low DAM accessibility. Strikingly, we observed no extended regions of inaccessible chromatin for any of the tissues examined. These results are consistent with "local choreography" models in which differential gene expression is driven by intricate local rearrangements of chromatin structure rather than gross impenetrability of large chromosomal regions.

Published

2010

135. An in vitro-identified high-affinity nucleosome-positioning signal is capable of transiently positioning a nucleosome in vivo

Author

Anton Valouev, Andrew Fire, Zhi-Ying Chen, Mark A. Kay, Arend Sidow, Lia Gracey, and Jay M. Maniar

Subjects

Genetics, 0303 health sciences, lcsh:QH426-470, Research, Eukaryotic DNA replication, Context (language use), Biology, Genome, DNA sequencing, Cell biology, Chromatin, 03 medical and health sciences, chemistry.chemical_compound, lcsh:Genetics, 0302 clinical medicine, chemistry, In vivo, Nucleosome, Molecular Biology, 030217 neurology & neurosurgery, DNA, 030304 developmental biology

Abstract

Background The physiological function of eukaryotic DNA occurs in the context of nucleosomal arrays that can expose or obscure defined segments of the genome. Certain DNA sequences are capable of strongly positioning a nucleosome in vitro, suggesting the possibility that favorable intrinsic signals might reproducibly structure chromatin segments. As high-throughput sequencing analyses of nucleosome coverage in vitro and in vivo have become possible, a vigorous debate has arisen over the degree to which intrinsic DNA:nucleosome affinities orchestrate the in vivo positions of nucleosomes, thereby controlling physical accessibility of specific sequences in DNA. Results We describe here the in vivo consequences of placing a synthetic high-affinity nucleosome-positioning signal, the 601 sequence, into a DNA plasmid vector in mice. Strikingly, the 601 sequence was sufficient to position nucleosomes during an early phase after introduction of the DNA into the mice (when the plasmid vector transgene was active). This positioning capability was transient, with a loss of strong positioning at a later time point when the transgenes had become silent. Conclusions These results demonstrate an ability of DNA sequences selected solely for nucleosome affinity to organize chromatin in vivo, and the ability of other mechanisms to overcome these interactions in a dynamic nuclear environment.

Published

2010

136. Ultra-high throughput sequencing-based small RNA discovery and discrete statistical biomarker analysis in a collection of cervical tumours and matched controls

Author

Sam Guoping Gu, Weng-Onn Lui, Andrew Fire, Daniela Witten, and Robert Tibshirani

Subjects

False discovery rate, Small RNA, DNA, Complementary, Physiology, Sequence analysis, Plant Science, Biology, General Biochemistry, Genetics and Molecular Biology, DNA sequencing, 03 medical and health sciences, 0302 clinical medicine, Structural Biology, Research article, microRNA, Cluster Analysis, Biomarker Analysis, lcsh:QH301-705.5, Ecology, Evolution, Behavior and Systematics, Gene Library, 030304 developmental biology, Genetics, 0303 health sciences, Agricultural and Biological Sciences(all), Biochemistry, Genetics and Molecular Biology(all), Gene Expression Profiling, Computational Biology, RNA, Sequence Analysis, DNA, Cell Biology, Gene expression profiling, MicroRNAs, lcsh:Biology (General), 030220 oncology & carcinogenesis, Linear Models, General Agricultural and Biological Sciences, Developmental Biology, Biotechnology

Abstract

Background Ultra-high throughput sequencing technologies provide opportunities both for discovery of novel molecular species and for detailed comparisons of gene expression patterns. Small RNA populations are particularly well suited to this analysis, as many different small RNAs can be completely sequenced in a single instrument run. Results We prepared small RNA libraries from 29 tumour/normal pairs of human cervical tissue samples. Analysis of the resulting sequences (42 million in total) defined 64 new human microRNA (miRNA) genes. Both arms of the hairpin precursor were observed in twenty-three of the newly identified miRNA candidates. We tested several computational approaches for the analysis of class differences between high throughput sequencing datasets and describe a novel application of a log linear model that has provided the most effective analysis for this data. This method resulted in the identification of 67 miRNAs that were differentially-expressed between the tumour and normal samples at a false discovery rate less than 0.001. Conclusions This approach can potentially be applied to any kind of RNA sequencing data for analysing differential sequence representation between biological sample sets.

Published

2010

137. Human tRNA-derived small RNAs in the global regulation of RNA silencing

Author

Mark A. Kay, Yong Huang, Ashley Lau, Andrew Fire, Poornima Parameswaran, and Dirk Haussecker

Subjects

Genetics, Small RNA, RNA-induced silencing complex, Trans-acting siRNA, Argonaute, Biology, HCT116 Cells, Models, Biological, Long non-coding RNA, Article, RNA silencing, MicroRNAs, RNA, Transfer, RasiRNA, Humans, RNA Interference, Small nucleolar RNA, RNA, Small Interfering, Molecular Biology, RNA, Double-Stranded

Abstract

Competition between mammalian RNAi-related gene silencing pathways is well documented. It is therefore important to identify all classes of small RNAs to determine their relationship with RNAi and how they affect each other functionally. Here, we identify two types of 5′-phosphate, 3′-hydroxylated human tRNA-derived small RNAs (tsRNAs). tsRNAs differ from microRNAs in being essentially restricted to the cytoplasm and in associating with Argonaute proteins, but not MOV10. The first type belongs to a previously predicted Dicer-dependent class of small RNAs that we find can modestly down-regulate target genes in trans. The 5′ end of type II tsRNA was generated by RNaseZ cleavage downstream from a tRNA gene, while the 3′ end resulted from transcription termination by RNA polymerase III. Consistent with their preferential association with the nonslicing Argonautes 3 and 4, canonical gene silencing activity was not observed for type II tsRNAs. The addition, however, of an oligonucleotide that was sense to the reporter gene, but antisense to an overexpressed version of the type II tsRNA, triggered robust, >80% gene silencing. This correlated with the redirection of the thus reconstituted fully duplexed double-stranded RNA into Argonaute 2, whereas Argonautes 3 and 4 were skewed toward less structured small RNAs, particularly single-strand RNAs. We observed that the modulation of tsRNA levels had minor effects on the abundance of microRNAs, but more pronounced changes in the silencing activities of both microRNAs and siRNAs. These findings support that tsRNAs are involved in the global control of small RNA silencing through differential Argonaute association, suggesting that small RNA-mediated gene regulation may be even more finely regulated than previously realized.

Published

2010

138. Functional conservation of nematode and vertebrate myogenic regulatory factors

Author

Stephen J. Tapscott, Andrew Fire, Michael Krause, Susan White-Harrison, and Harold Weintraub

Subjects

Genetics, biology, Myogenesis, Muscles, Molecular Sequence Data, Muscle Proteins, Cell Biology, biology.organism_classification, MyoD, Gene Expression Regulation, Cell culture, Consensus Sequence, Myogenic regulatory factors, Gene expression, Morphogenesis, Trans-Activators, Animals, Myocyte, Amino Acid Sequence, Promoter Regions, Genetic, Caenorhabditis elegans, Myogenin, MyoD Protein

Abstract

Summary The Caenorhabditis elegans protein, CeMyoD, is related to the vertebrate myogenic regulatory factors MyoD, myogenin, MRF-4 and Myf-5. Like its vertebrate counterparts, CeMyoD accumulates in the nucleus of striated muscle cells prior to the onset of terminal differentiation. CeMyoD also shares functional similarities with the vertebrate myogenic regulatory factors. Viral LTR driven expression of CeMyoD in mouse 10T1/2 cells can convert this cell line into myoblasts as well as efficiently trans-activate mouse muscle-specific promoters. Furthermore, mouse MyoD expression can activate a CeMyoD-β-galactosidase reporter construct in a 10T1/2 co-transfection assay.

Published

1992

139. A Caenorhabditis elegans RNA-directed RNA polymerase in sperm development and endogenous RNA interference

Author

Antoine Baudrimont, Andrew Fire, Verena Jantsch, Jonathan I. Gent, Anne M. Villeneuve, Sam Guoping Gu, and Mara Schvarzstein

Subjects

Male, Small RNA, Small interfering RNA, X Chromosome, Cell Survival, Trans-acting siRNA, Disorders of Sex Development, RNA-dependent RNA polymerase, Down-Regulation, Embryonic Development, Biology, Investigations, Microtubules, RNA interference, Spermatocytes, Genetics, Gene silencing, Animals, RNA, Antisense, RNA, Messenger, RNA, Small Interfering, Caenorhabditis elegans, Spermatogenesis, RNA, Gene Expression Regulation, Developmental, Sequence Analysis, DNA, RNA-Dependent RNA Polymerase, Spermatozoa, RNA silencing, Mutation, RNA Interference, Cell Division

Abstract

Short interfering RNAs (siRNAs) are a class of regulatory effectors that enforce gene silencing through formation of RNA duplexes. Although progress has been made in identifying the capabilities of siRNAs in silencing foreign RNA and transposable elements, siRNA functions in endogenous gene regulation have remained mysterious. In certain organisms, siRNA biosynthesis involves novel enzymes that act as RNA-directed RNA polymerases (RdRPs). Here we analyze the function of a Caenorhabditis elegans RdRP, RRF-3, during spermatogenesis. We found that loss of RRF-3 function resulted in pleiotropic defects in sperm development and that sperm defects led to embryonic lethality. Notably, sperm nuclei in mutants of either rrf-3 or another component of the siRNA pathway, eri-1, were frequently surrounded by ectopic microtubule structures, with spindle abnormalities in a subset of the resulting embryos. Through high-throughput small RNA sequencing, we identified a population of cellular mRNAs from spermatogenic cells that appear to serve as templates for antisense siRNA synthesis. This set of genes includes the majority of genes known to have enriched expression during spermatogenesis, as well as many genes not previously known to be expressed during spermatogenesis. In a subset of these genes, we found that RRF-3 was required for effective siRNA accumulation. These and other data suggest a working model in which a major role of the RRF-3/ERI pathway is to generate siRNAs that set patterns of gene expression through feedback repression of a set of critical targets during spermatogenesis.

Published

2009

140. Profiling and discovery of novel miRNAs from formalin-fixed, paraffin-embedded melanoma and nodal specimens

Author

Soheil S. Dadras, Zhihai Ma, Andrew Fire, and Weng-Onn Lui

Subjects

Male, Small RNA, Tissue Fixation, Technical Advances, Biology, In Vitro Techniques, Polymerase Chain Reaction, Pathology and Forensic Medicine, law.invention, Metastasis, law, Formaldehyde, Neoplasms, microRNA, medicine, Gene silencing, Humans, Child, Melanoma, Polymerase chain reaction, Paraffin Embedding, Ribosomal RNA, Middle Aged, medicine.disease, Blotting, Northern, Molecular biology, Blot, MicroRNAs, Cancer research, Molecular Medicine

Abstract

Archived formalin-fixed, paraffin-embedded human tumors are widely available and represent a unique source of morphologically defined material. Formalin-fixed, paraffin-embedded tissue is known to contain a wealth of molecular information in the form of microRNAs (miRNAs), which could be correlated with clinical outcome for improved prognostication and/or treatment response. miRNAs are endogenous, noncoding RNAs ( approximately 22 nucleotides) and may function as tumor suppressors or oncogenes. A reliable, robust methodology is needed to take full advantage of archived human cancers, especially for those where fresh-frozen tumor banks are unavailable, for example, malignant melanoma. To this end, we applied a simple-to-use protocol for extracting total RNA from various formalin-fixed, paraffin-embedded specimens (colon, liver, prostate, thyroid, uterus, and skin), optimized for small RNA recovery. Using a "poison primer" strategy (ie, primer silencing), we blocked the amplification of ribosomal RNA, enabling the successful sequencing of 17 novel and 53 known miRNAs (including small RNAs) from 10-year-old archived normal skin, cutaneous scalp melanoma, and sentinel lymph nodes (both negative and positive for metastasis) excised from a 52-year-old man. The cloning incidence provided an estimation of the level of specific miRNA expression, which was confirmed by Northern analysis and quantitative real-time polymerase chain reaction. This methodology can therefore be used to facilitate miRNA discovery from archived human cancers.

Published

2009

141. Distinct phases of siRNA synthesis in an endogenous RNAi pathway in C. elegans soma

Author

Jonathan I. Gent, Derek M. Pavelec, Poornima Parameswaran, Scott Kennedy, Jay M. Maniar, Andrew Fire, Ayelet T. Lamm, and Li Tao

Subjects

Ribonuclease III, Small interfering RNA, Transcription, Genetic, RNA Stability, RNA-dependent RNA polymerase, RNA-binding protein, Biology, RNA interference, Eukaryotic initiation factor, Animals, RNA, Messenger, Eukaryotic Initiation Factors, Phosphorylation, RNA, Small Interfering, Caenorhabditis elegans, Caenorhabditis elegans Proteins, Molecular Biology, Genetics, RNA, RNA-Binding Proteins, Cell Biology, Argonaute, RNA-Dependent RNA Polymerase, Cell biology, Exoribonucleases, Mutation, biology.protein, RNA Interference, Dicer

Abstract

Summary Endogenous RNA-directed RNA polymerases (RdRPs) are cellular components capable of synthesizing new complementary RNAs from existing RNA templates. We present evidence for successive engagement of two different RdRPs in an endogenous siRNA-based mechanism targeting specific mRNAs in C. elegans soma. In the initiation stage of this process, a group of mRNA species are chosen as targets for downregulation, leading to accumulation of rare 26 nt 5′-phosphorylated antisense RNAs that depend on the RdRP homolog RRF-3, the Argonaute ERGO-1, DICER, and a series of associated ("ERI") factors. This primary process leads to production of a much more abundant class of 22 nt antisense RNAs, dependent on a secondary RdRP (RRF-1) and associating with at least one distinct Argonaute (NRDE-3). The requirement for two RdRP/Argonaute combinations and initiation by a rare class of uniquely structured siRNAs in this pathway illustrate the caution and flexibility used as biological systems exploit the physiological copying of RNA.

Published

2009

142. Production of antisense RNA leads to effective and specific inhibition of gene expression in C. elegans muscle

Author

Donald G. Moerman, Donna G. Albertson, Susan White Harrison, and Andrew Fire

Subjects

Muscles, Microfilament Proteins, Gene Expression, RNA, Biology, Non-coding RNA, Molecular biology, Antisense RNA, RNA silencing, Phenotype, Gene Expression Regulation, RNA interference, Gene expression, Sense (molecular biology), Caenorhabditis, Animals, RNA, Antisense, Molecular Biology, Gene, Developmental Biology

Abstract

We have used an antisense strategy to effectively disrupt the expression of two genes encoding myofilament proteins present in C. elegans body wall muscles. DNA segments from the unc-22 and unc-54 genes have been placed in reverse orientation in vectors designed to produce RNA in body wall muscles. When the resulting plasmids are injected into oocytes, progeny with defects in muscle function are produced. These animals have phenotypes consistent with reduction and/or elimination of function of the gene to which antisense RNA has been produced: twitching and disorganization of muscle filaments for the unc-22 antisense constructs and lack of muscle tone, slow movement, and egg laying defects for the unc-54 antisense constructs. A fraction of the affected animals transmit the defective-muscle trait to subsequent generations. In these cases the transforming DNA is present at high copy number and cosegregates with the observed muscle defects. We have examined several of the unc-22 antisense plasmid transformed lines to determine the mechanistic basis for the observed phenotypes. The RNA product of the endogenous unc-22 locus is present at normal levels and this RNA is properly spliced in the region homologous to the antisense RNA. No evidence for modification of this RNA by deamination of adenosine to inosine was found. In affected animals the level of protein product from the endogenous unc-22 locus is greatly reduced. Antisense RNA produced from the transforming DNA was detected and was much more abundant than ‘sense’ RNA from the endogenous locus. These data suggest that the observed phenotypes result from interference with a late step in gene expression, such as transport into the cytoplasm or translation.

Published

1991

143. Chromatin-associated periodicity in genetic variation downstream of transcriptional start sites

Author

Shinichi Morishita, Sam Guoping Gu, Atsushi Sasaki, Masahiro Kasahara, Atsuko Shimada, Sumio Sugano, Yoichiro Nakatani, Budrul Ahsan, Taro Saito, Hiroyuki Takeda, Cecilia C. Mello, Masako Ogawa, Shin Sasaki, Andrew Fire, Shin-ichi Hashimoto, Yuji Kohara, Yutaka Suzuki, and Kouji Matsushima

Subjects

DNA Repair, Transcription, Genetic, Oryzias, Biology, DNA sequencing, chemistry.chemical_compound, INDEL Mutation, Transcription (biology), Genetic variation, Nucleosome, Animals, Point Mutation, Promoter Regions, Genetic, Genetics, Base Composition, Multidisciplinary, Genome, Base Sequence, Point mutation, Genetic Variation, DNA, biology.organism_classification, Chromatin, Nucleosomes, chemistry, Mutagenesis, Mutation, Transcription Initiation Site

Abstract

Might DNA sequence variation reflect germline genetic activity and underlying chromatin structure? We investigated this question using medaka (Japanese killifish, Oryzias latipes ), by comparing the genomic sequences of two strains (Hd-rR and HNI) and by mapping ∼37.3 million nucleosome cores from Hd-rR blastulae and 11,654 representative transcription start sites from six embryonic stages. We observed a distinctive ∼200–base pair (bp) periodic pattern of genetic variation downstream of transcription start sites; the rate of insertions and deletions longer than 1 bp peaked at positions of approximately +200, +400, and +600 bp, whereas the point mutation rate showed corresponding valleys. This ∼200-bp periodicity was correlated with the chromatin structure, with nucleosome occupancy minimized at positions 0, +200, +400, and +600 bp. These data exemplify the potential for genetic activity (transcription) and chromatin structure to contribute to molding the DNA sequence on an evolutionary time scale.

Published

2008

144. CED-9 and mitochondrial homeostasis in C. elegans muscle

Author

Andrew Fire, Frederick J. Tan, R. Blake Hill, Michelle Husain, Marijke Koppenol, and Cara Marie Manlandro

Subjects

Dynamins, Mitochondrion, Biology, Mitochondrial Size, Mitochondrial apoptosis-induced channel, Membrane Fusion, Models, Biological, Article, GTP Phosphohydrolases, Mitochondrial Proteins, Membrane fission, Animals, Homeostasis, Humans, Caenorhabditis elegans, Caenorhabditis elegans Proteins, fungi, Cell Biology, Cell biology, Mitochondria, mitochondrial fusion, Proto-Oncogene Proteins c-bcl-2, Mitochondrial Membranes, DNAJA3, Mitochondrial fission, ATP–ADP translocase, Microtubule-Associated Proteins

Abstract

Mitochondrial homeostasis reflects a dynamic balance between membrane fission and fusion events thought essential for mitochondrial function. We report here that altered expression of the C. elegans BCL2 homolog CED-9 affects both mitochondrial fission and fusion. Although striated muscle cells lacking CED-9 have no alteration in mitochondrial size or ultrastructure, these cells appear more sensitive to mitochondrial fragmentation. By contrast, increased CED-9 expression in these cells produces highly interconnected mitochondria. This mitochondrial phenotype is partially suppressed by increased expression of the dynamin-related GTPase DRP-1, with suppression dependent on the BH3 binding pocket of CED-9. This suppression suggests that CED-9 directly regulates DRP-1, a model supported by our finding that CED-9 activates the GTPase activity of human DRP1. Thus, CED-9 is capable of regulating the mitochondrial fission-fusion cycle but is not essential for either fission or fusion.

Published

2008

145. Transmission dynamics of heritable silencing induced by double-stranded RNA in Caenorhabditis elegans

Author

Rosa Alcazar, Rueyling Lin, and Andrew Fire

Subjects

Male, Transcription, Genetic, Population, Investigations, RNA interference, Spermatocytes, Genetics, Gene silencing, Animals, Epigenetics, Gene Silencing, RNA, Small Interfering, education, Caenorhabditis elegans, Caenorhabditis elegans Proteins, Gene, RNA, Double-Stranded, Regulation of gene expression, education.field_of_study, biology, biology.organism_classification, Phenotype, Gene Expression Regulation, Mutation, Oocytes, Female, Carrier Proteins

Abstract

Heritable silencing effects are gene suppression phenomena that can persist for generations after induction. In the majority of RNAi experiments conducted in Caenorhabditis elegans, the silencing response results in a hypomorphic phenotype where the effects recede after the F1 generation. F2 and subsequent generations revert to the original phenotype. Specific examples of transgenerational RNAi in which effects persist to the F2 generation and beyond have been described. In this study, we describe a systematic pedigree-based analysis of heritable silencing processes resulting from initiation of interference targeted at the C. elegans oocyte maturation factor oma-1. Heritable silencing of oma-1 is a dose-dependent process where the inheritance of the silencing factor is unequally distributed among the population. Heritability is not constant over generational time, with silenced populations appearing to undergo a bottleneck three to four generations following microinjection of RNA. Transmission of silencing through these generations can be through either maternal or paternal gamete lines and is surprisingly more effective through the male gametic line. Genetic linkage tests reveal that silencing in the early generations is transmitted independently of the original targeted locus, in a manner indicative of a diffusible epigenetic element.

Published

2008

146. A high-resolution, nucleosome position map of C. elegans reveals a lack of universal sequence-dictated positioning

Author

Steven M. Johnson, Kevin McKernan, Kathy Zeng, Anton Valouev, Heather E. Peckham, Joel A. Malek, Gina Costa, Swati Ranade, Jeffrey Ichikawa, Thaisan Tonthat, Jeremy R. Stuart, Arend Sidow, and Andrew Fire

Subjects

Genetics, Nucleosome organization, Genetic Markers, education.field_of_study, Genome, Helminth, Letter, Base Sequence, Population, Chromosome Mapping, Helminth genetics, Genome browser, Computational biology, Biology, DNA, Helminth, Chromatin, Nucleosomes, Genetic model, Nucleosome, Animals, education, Caenorhabditis elegans, Genetics (clinical), ChIA-PET

Abstract

Using the massively parallel technique of sequencing by oligonucleotide ligation and detection (SOLiD; Applied Biosystems), we have assessed the in vivo positions of more than 44 million putative nucleosome cores in the multicellular genetic model organism Caenorhabditis elegans. These analyses provide a global view of the chromatin architecture of a multicellular animal at extremely high density and resolution. While we observe some degree of reproducible positioning throughout the genome in our mixed stage population of animals, we note that the major chromatin feature in the worm is a diversity of allowed nucleosome positions at the vast majority of individual loci. While absolute positioning of nucleosomes can vary substantially, relative positioning of nucleosomes (in a repeated array structure likely to be maintained at least in part by steric constraints) appears to be a significant property of chromatin structure. The high density of nucleosomal reads enabled a substantial extension of previous analysis describing the usage of individual oligonucleotide sequences along the span of the nucleosome core and linker. We release this data set, via the UCSC Genome Browser, as a resource for the high-resolution analysis of chromatin conformation and DNA accessibility at individual loci within the C. elegans genome.

Published

2008

147. Cellular responses to genetic change

Author

Andrew Fire

Subjects

Evolutionary biology, Genetics, Genetic Change, Biology, Molecular Biology, Biochemistry, Biotechnology

Published

2008

148. Gene Silencing by Double-Stranded RNA (Nobel Lecture)

Author

Andrew Fire

Subjects

History, Chemistry, Media studies, General Chemistry, General Medicine, Double stranded rna, Catalysis, Nobel Prize, Immune System, medicine, Animals, Humans, RNA Interference, Gene Silencing, medicine.symptom, Double stranded, RNA, Double-Stranded, Confusion

Abstract

I would like to thank the Nobel Assembly of the Karolinska Institute for the opportunity to describe some recent work on RNA-triggered gene silencing. First a few disclaimers, however. Telling the full story of gene silencing would be a mammoth enterprise that would take me many years to write and would take you well into the night to read. So we'll need to abbreviate the story more than a little. Second (and as you will see) we are only in the dawn of our knowledge; so consider the following to be primer ... the best we could do as of December 8th 2006. And third, please understand that the story that I am telling represents the work of several generations of biologists, chemists, and many shades in between. I'm pleased and proud that work from my laboratory has contributed to the field, and that this has led to my being chosen as one of the messengers to relay the story in this forum. At the same time, I hope that there will be no confusion of equating our modest contributions with those of the much grander RNAi enterprise.

Published

2007

149. MicroRNA expression signature of human sarcomas

Author

Christopher L. Corless, Weng-Onn Lui, C-H Lee, Inigo Espinosa, M van de Rijn, Andrew Fire, Subree Subramanian, Michael Heinrich, and Torsten O. Nielsen

Subjects

Cancer Research, Biology, Bioinformatics, Mice, RNA interference, microRNA, Gene expression, Genetics, medicine, Gene silencing, Animals, Humans, Cloning, Molecular, Muscle, Skeletal, Molecular Biology, Oligonucleotide Array Sequence Analysis, Gene Expression Profiling, Muscle, Smooth, Sarcoma, medicine.disease, Gene expression profiling, MicroRNAs, Cancer research, Gene chip analysis, DNA microarray

Abstract

MicroRNAs (miRNAs) are approximately 22 nucleotide-long noncoding RNAs involved in several biological processes including development, differentiation and proliferation. Recent studies suggest that knowledge of miRNA expression patterns in cancer may have substantial value for diagnostic and prognostic determinations as well as for eventual therapeutic intervention. We performed comprehensive analysis of miRNA expression profiles of 27 sarcomas, 5 normal smooth muscle and 2 normal skeletal muscle tissues using microarray technology and/or small RNA cloning approaches. The miRNA expression profiles are distinct among the tumor types as demonstrated by an unsupervised hierarchical clustering, and unique miRNA expression signatures were identified in each tumor class. Remarkably, the miRNA expression patterns suggested that two of the sarcomas had been misdiagnosed and this was confirmed by reevaluation of the tumors using histopathologic and molecular analyses. Using the cloning approach, we also identified 31 novel miRNAs or other small RNA effectors in the sarcomas and normal skeletal muscle tissues examined. Our data show that different histological types of sarcoma have distinct miRNA expression patterns, reflecting the apparent lineage and differentiation status of the tumors. The identification of unique miRNA signatures in each tumor type may indicate their role in tumorigenesis and may aid in diagnosis of soft tissue sarcomas.

Published

2007

150. Connector inversion probe technology: a powerful one-primer multiplex DNA amplification system for numerous scientific applications

Author

Pål Nyrén, Ronald W. Davis, Michael S. Akhras, Sreedevi Thiyagarajan, Andrew Fire, Nader Pourmand, and Magnus Unemo

Subjects

lcsh:Medicine, Computational biology, Biology, Molecular Inversion Probe, Multiplexing, 03 medical and health sciences, Microbiology/Applied Microbiology, 0302 clinical medicine, Infectious Diseases/Viral Infections, Infectious Diseases/Sexually Transmitted Diseases, Biotechnology/Applied Microbiology, Multiplex, Typing, Human papillomavirus, lcsh:Science, Genotyping, 030304 developmental biology, Genetics, 0303 health sciences, Multidisciplinary, Infectious Diseases/Gynecologic Infections, Hybridization probe, lcsh:R, Genetics and Genomics, Drug Resistance, Microbial, Virology/Diagnosis, DNA, 030220 oncology & carcinogenesis, Mutation, lcsh:Q, Biotechnology/Bioengineering, Primer (molecular biology), DNA Probes, Research Article

Abstract

We combined components of a previous assay referred to as Molecular Inversion Probe (MIP) with a complete gap filling strategy, creating a versatile powerful one-primer multiplex amplification system. As a proof-of-concept, this novel method, which employs a Connector Inversion Probe (CIPer), was tested as a genetic tool for pathogen diagnosis, typing, and antibiotic resistance screening with two distinct systems: i) a conserved sequence primer system for genotyping Human Papillomavirus (HPV), a cancer-associated viral agent and ii) screening for antibiotic resistance mutations in the bacterial pathogen Neisseria gonorrhoeae. We also discuss future applications and advances of the CIPer technology such as integration with digital amplification and next-generation sequencing methods. Furthermore, we introduce the concept of two-dimension informational barcodes, i.e. “multiplex multiplexing padlocks” (MMPs). For the readers' convenience, we also provide an on-line tutorial with user-interface software application CIP creator 1.0.1, for custom probe generation from virtually any new or established primer-pairs.

Published

2007