Your search keyword '"Anna Liisa Prabhu"' showing total 10 results

1. A physical map of the highly heterozygous Populus genome: integration with the genome sequence and genetic map and analysis of haplotype variation

Author

Natasja Wye, Jane Grimwood, Ian Bosdet, Kermit Ritland, Carrie Mathewson, Jennifer Asano, Duane E. Smailus, Jeffery M. Stott, Jennifer Wilkin, Gerald A. Tuskan, Julia Vrebalov, James J. Giovannoni, Nicholas H. Putnam, Anna-Liisa Prabhu, Readman Chiu, Brian E. Ellis, Martin Krzywinski, Stephen P. DiFazio, Miranda Tsai, Katie O’Connor, Jeremy Schmutz, Teika Olson, Darlene Lee, Susanna Chan, Jörg Bohlmann, Tongming Yin, Jun Zhuang, Steven J.M. Jones, Stephen Leach, Heesun Shin, Chris Fjell, George S. Yang, Colin T. Kelleher, Robert A. Holt, Marco A. Marra, Alison Cloutier, Jacqueline E. Schein, Carl J. Douglas, Daniel S. Rokhsar, Noreen Girn, and Johar Ali

Subjects

Genetics, Whole genome sequencing, Contig, Sequence analysis, food and beverages, Sequence assembly, Genomics, Cell Biology, Plant Science, Genome project, Biology, Genome, Sequence-tagged site

Abstract

*† Summary As part of a larger project to sequence the Populus genome and generate genomic resources for this emerging model tree, we constructed a physical map of the Populus genome, representing one of the few such maps of an undomesticated, highly heterozygous plant species. The physical map, consisting of 2802 contigs, was constructed from fingerprinted bacterial artificial chromosome (BAC) clones. The map represents approximately 9.4-fold coverage of the Populus genome, which has been estimated from the genome sequence assembly to be 485 10 Mb in size. BAC ends were sequenced to assist long-range assembly of wholegenome shotgun sequence scaffolds and to anchor the physical map to the genome sequence. Simple sequence repeat-based markers were derived from the end sequences and used to initiate integration of the BAC and genetic maps. A total of 2411 physical map contigs, representing 97% of all clones assigned to contigs, were aligned to the sequence assembly (JGI Populus trichocarpa, version 1.0). These alignments represent a total coverage of 384 Mb (79%) of the entire poplar sequence assembly and 295 Mb (96%) of linkage group sequence assemblies. A striking result of the physical map contig alignments to the sequence assembly was the co-localization of multiple contigs across numerous regions of the 19 linkage groups. Targeted sequencing of BAC clones and genetic analysis in a small number of representative regions showed that these co-aligning contigs represent distinct haplotypes in the heterozygous individual sequenced, and revealed the nature of these haplotype sequence differences.

Published

2007

2. Application of massively parallel sequencing to microRNA profiling and discovery in human embryonic stem cells

Author

Connie J. Eaves, Thomas Zeng, Florian Kuchenbauer, Ryan D. Morin, Allen Delaney, Helen McDonald, Malachi Griffith, Michael D O'Connor, Marco A. Marra, Anna-Liisa Prabhu, Martin Hirst, and Yongjun Zhao

Subjects

Genetics, Regulation of gene expression, Massive parallel sequencing, Base Sequence, Sequence analysis, Sequence Analysis, RNA, Gene Expression Profiling, Molecular Sequence Data, Biology, Gene expression profiling, MicroRNAs, IsomiR, Gene Expression Regulation, microRNA, Methods, Gene silencing, Humans, RNA Processing, Post-Transcriptional, Genetics (clinical), Illumina dye sequencing, Embryonic Stem Cells

Abstract

MicroRNAs (miRNAs) are emerging as important, albeit poorly characterized, regulators of biological processes. Key to further elucidation of their roles is the generation of more complete lists of their numbers and expression changes in different cell states. Here, we report a new method for surveying the expression of small RNAs, including microRNAs, using Illumina sequencing technology. We also present a set of methods for annotating sequences deriving from known miRNAs, identifying variability in mature miRNA sequences, and identifying sequences belonging to previously unidentified miRNA genes. Application of this approach to RNA from human embryonic stem cells obtained before and after their differentiation into embryoid bodies revealed the sequences and expression levels of 334 known plus 104 novel miRNA genes. One hundred seventy-one known and 23 novel microRNA sequences exhibited significant expression differences between these two developmental states. Owing to the increased number of sequence reads, these libraries represent the deepest miRNA sampling to date, spanning nearly six orders of magnitude of expression. The predicted targets of those miRNAs enriched in either sample shared common features. Included among the high-ranked predicted gene targets are those implicated in differentiation, cell cycle control, programmed cell death, and transcriptional regulation.

Published

2008

3. A physical map of the highly heterozygous Populus genome: integration with the genome sequence and genetic map and analysis of haplotype variation

Author

Colin T, Kelleher, Readman, Chiu, Heesun, Shin, Ian E, Bosdet, Martin I, Krzywinski, Chris D, Fjell, Jennifer, Wilkin, Tongming, Yin, Stephen P, DiFazio, Johar, Ali, Jennifer K, Asano, Susanna, Chan, Alison, Cloutier, Noreen, Girn, Stephen, Leach, Darlene, Lee, Carrie A, Mathewson, Teika, Olson, Katie, O'connor, Anna-Liisa, Prabhu, Duane E, Smailus, Jeffery M, Stott, Miranda, Tsai, Natasja H, Wye, George S, Yang, Jun, Zhuang, Robert A, Holt, Nicholas H, Putnam, Julia, Vrebalov, James J, Giovannoni, Jane, Grimwood, Jeremy, Schmutz, Daniel, Rokhsar, Steven J M, Jones, Marco A, Marra, Gerald A, Tuskan, Jörg, Bohlmann, Brian E, Ellis, Kermit, Ritland, Carl J, Douglas, and Jacqueline E, Schein

Subjects

Chromosomes, Artificial, Bacterial, Polymorphism, Genetic, Populus, Haplotypes, Minisatellite Repeats, Sequence Analysis, DNA, Physical Chromosome Mapping, Sequence Alignment, Genome, Plant

Abstract

As part of a larger project to sequence the Populus genome and generate genomic resources for this emerging model tree, we constructed a physical map of the Populus genome, representing one of the few such maps of an undomesticated, highly heterozygous plant species. The physical map, consisting of 2802 contigs, was constructed from fingerprinted bacterial artificial chromosome (BAC) clones. The map represents approximately 9.4-fold coverage of the Populus genome, which has been estimated from the genome sequence assembly to be 485 +/- 10 Mb in size. BAC ends were sequenced to assist long-range assembly of whole-genome shotgun sequence scaffolds and to anchor the physical map to the genome sequence. Simple sequence repeat-based markers were derived from the end sequences and used to initiate integration of the BAC and genetic maps. A total of 2411 physical map contigs, representing 97% of all clones assigned to contigs, were aligned to the sequence assembly (JGI Populus trichocarpa, version 1.0). These alignments represent a total coverage of 384 Mb (79%) of the entire poplar sequence assembly and 295 Mb (96%) of linkage group sequence assemblies. A striking result of the physical map contig alignments to the sequence assembly was the co-localization of multiple contigs across numerous regions of the 19 linkage groups. Targeted sequencing of BAC clones and genetic analysis in a small number of representative regions showed that these co-aligning contigs represent distinct haplotypes in the heterozygous individual sequenced, and revealed the nature of these haplotype sequence differences.

Published

2007

4. Large-scale production of SAGE libraries from microdissected tissues, flow-sorted cells, and cell lines

Author

Stephanie Lee, Jennifer Asano, Noreen Dhalla, Pamela A. Hoodless, Robert A. Holt, David L. Charest, Connie J. Eaves, Scott Zuyderduyn, Anna-Liisa Prabhu, Adrian Ally, Yongjun Zhao, Richard Varhol, Danne Sa, Martin Hirst, Jaswinder Khattra, Asim Siddiqui, Jeffrey L Stott, Marco A. Marra, Helen McDonald, Allen Delaney, Angela Tam, Kevin Ma, Steven J.M. Jones, Sean A Rogers, and Pawan Pandoh

Subjects

Computational biology, Cell Separation, Biology, Genome, DNA sequencing, Cell Line, Mice, Genetics, Methods, Animals, Humans, Genomic library, Serial analysis of gene expression, Caenorhabditis elegans, Genetics (clinical), Embryonic Stem Cells, Zebrafish, Gene Library, SAGE, Gene Expression Profiling, Sequence Analysis, DNA, Flow Cytometry, Gene expression profiling, RNA extraction, Databases, Nucleic Acid, Microdissection, Sorted Cells, Software

Abstract

We describe the details of a serial analysis of gene expression (SAGE) library construction and analysis platform that has enabled the generation of >298 high-quality SAGE libraries and >30 million SAGE tags primarily from sub-microgram amounts of total RNA purified from samples acquired by microdissection. Several RNA isolation methods were used to handle the diversity of samples processed, and various measures were applied to minimize ditag PCR carryover contamination. Modifications in the SAGE protocol resulted in improved cloning and DNA sequencing efficiencies. Bioinformatic measures to automatically assess DNA sequencing results were implemented to analyze the integrity of ditag structure, linker or cross-species ditag contamination, and yield of high-quality tags per sequence read. Our analysis of singleton tag errors resulted in a method for correcting such errors to statistically determine tag accuracy. From the libraries generated, we produced an essentially complete mapping of reliable 21-base-pair tags to the mouse reference genome sequence for a meta-library of ∼5 million tags. Our analyses led us to reject the commonly held notion that duplicate ditags are artifacts. Rather than the usual practice of discarding such tags, we conclude that they should be retained to avoid introducing bias into the results and thereby maintain the quantitative nature of the data, which is a major theoretical advantage of SAGE as a tool for global transcriptional profiling.

Published

2007

5. Integrated and sequence-ordered BAC- and YAC-based physical maps for the rat genome

Author

Andre Marziali, Derek Albracht, Susanna Chan, Alison Cloutier, Darlene Lee, Miranda Tsai, Detlev Ganten, Stephen Leach, Tina Graves, Heesun Shin, Heinz Himmelbauer, Chris Fjell, Dan Layman, Jason Thompson, Jacqueline E. Schein, Martin Krzywinski, John Douglas Mcpherson, Michael Mayo, Anna Liisa Prabhu, Asim Sarosh Siddiqui, Ian Bosdet, Steve Chand, Natasja Wye, Readman Chiu, Carrie Mathewson, Thomas Kreitler, George S. Yang, Jonathon Davito, Norbert Hubner, Baoli Zhu, Sarah Barber, Jason Walker, Noreen Girn, Kurtis Guggenheimer, Richard K. Wilson, Wes Warren, Jennifer Asano, Teika Olson, Mabel Brown-John, Marco A. Marra, Shaying Zhao, Simone Tänzer, Pieter J. de Jong, John W. Wallis, Claudia Gosele, Steven J.M. Jones, Tony Gaige, Heike Zimdahl, Elaine R. Mardis, Pawan Pandoh, Kelly Mead, LaDeana W. Hillier, Kazutoyo Osoegawa, Mandeep Sekhon, Oliver Hummel, and Hans Lehrach

Subjects

Genetic Markers, Yeast artificial chromosome, Chromosomes, Artificial, Bacterial, Sequence assembly, Biology, Polymerase Chain Reaction, Genome, Chromosomes, Contig Mapping, Automation, 03 medical and health sciences, 0302 clinical medicine, Genetics, Animals, Cloning, Molecular, Chromosomes, Artificial, Yeast, Genetics (clinical), 030304 developmental biology, 0303 health sciences, Bacterial artificial chromosome, Contig, Physical Chromosome Mapping, Computational Biology, food and beverages, Sequence Analysis, DNA, Genome project, DNA Fingerprinting, Resources, Rats, Cardiovascular and Metabolic Diseases, 030217 neurology & neurosurgery

Abstract

As part of the effort to sequence the genome ofRattus norvegicus, we constructed a physical map comprised of fingerprinted bacterial artificial chromosome (BAC) clones from the CHORI-230 BAC library. These BAC clones provide ∼13-fold redundant coverage of the genome and have been assembled into 376 fingerprint contigs. A yeast artificial chromosome (YAC) map was also constructed and aligned with the BAC map via fingerprinted BAC and P1 artificial chromosome clones (PACs) sharing interspersed repetitive sequence markers with the YAC-based physical map. We have annotated 95% of the fingerprint map clones in contigs with coordinates on the version 3.1 rat genome sequence assembly, using BAC-end sequences and in silico mapping methods. These coordinates have allowed anchoring 358 of the 376 fingerprint map contigs onto the sequence assembly. Of these, 324 contigs are anchored to rat genome sequences localized to chromosomes, and 34 contigs are anchored to unlocalized portions of the rat sequence assembly. The remaining 18 contigs, containing 54 clones, still require placement. The fingerprint map is a high-resolution integrative data resource that provides genome-ordered associations among BAC, YAC, and PAC clones and the assembled sequence of the rat genome.

Published

2004

6. A set of BAC clones spanning the human genome

Author

Miranda Tsai, Anna Liisa Prabhu, Steve Chand, Noreen Girn, Mabel Brown-John, Alison Cloutier, Marco A. Marra, Readman Chiu, Carrie Mathewson, Shaying Zhao, Amara Masson, Susanna Chan, Duane E. Smailus, Michael Mayo, Martin Krzywinski, Chik On Choy, Sarah Barber, Jacqueline E. Schein, Ian Bosdet, Teika Olson, Steven J.M. Jones, Eric F.P.M. Schoenmakers, Donna G. Albertson, Kazutoyo Osoegawa, Pawan Pandoh, Wan L. Lam, Natasja Wye, Pieter J. de Jong, and Darlene Lee

Subjects

Cancer genome sequencing, clone (Java method), Genetics, Chromosomes, Artificial, Bacterial, Bacterial artificial chromosome, Base Sequence, Genome, Human, Articles, Genome project, Biology, Physical Chromosome Mapping, ENCODE, Genome, Humans, Human genome, Cloning, Molecular, Reference genome, Molecular diagnosis, prognosis and monitoring [UMCN 1.2]

Abstract

Contains fulltext : 57492.pdf (Publisher’s version ) (Open Access) Using the human bacterial artificial chromosome (BAC) fingerprint-based physical map, genome sequence assembly and BAC end sequences, we have generated a fingerprint-validated set of 32 855 BAC clones spanning the human genome. The clone set provides coverage for at least 98% of the human fingerprint map, 99% of the current assembled sequence and has an effective resolving power of 79 kb. We have made the clone set publicly available, anticipating that it will generally facilitate FISH or array-CGH-based identification and characterization of chromosomal alterations relevant to disease.

Published

2004

7. A physical map of the mouse genome

Author

Asif T. Chinwalla, Daniel A. Russell, Richard D. Hutton, Rebecca McGrane, Pawan Pandoh, Catharine Gray, Margaret Krol, Kazutoyo Osoegawa, Mandeep Sekhon, Ewan Birney, Marco A. Marra, Michael Heaney, Reta Kutsche, R Evans, Pieter J. de Jong, Soo Sen Lee, Tony Cox, Elizabeth Gebregeorgis, Carol Scott, Jacqueline E. Schein, Duane E Smailus, David R. Bentley, Parvaneh Saeedi, Glen Threadgold, Ian R Mullenger, Suganthi Chittaranjan, Chris Fjell, Robert H. Waterston, Jim Stalker, Letticia Hsiao, Jason Maas, Martin Krzywinski, Jason Carter, John Douglas Mcpherson, Kelly Mead, Simon G. Gregory, Ian Bosdet, Bola Ayodeji, Anna-Liisa Prabhu, Joel A. Malek, George S. Yang, Dan Layman, Tony Gaige, Keita Geer, Jane Rogers, Tamara Feldblyum, Miranda Tsai, Larry Overton, Sara Jaeger, LaDeana W. Hillier, Kristine M. Wylie, Colin Kremitzki, Sheryl Taylor, Carrie Mathewson, Jyoti Shetty, Wesley Terpstra, James Smith, Getahun Tsegaye, Christopher A Fox, Steve Messervier, Natasja Wye, Candice McLeavy, Jill Vardy, William C. Nierman, Lorraine Spence, Alla Shvartsbeyn, Sofiya Shatsman, Readman Chiu, Claire M. Fraser, Michael Smith, John W. Wallis, Michael C. Holmes, Tim Hubbard, Ran Guin, Shaying Zhao, Jeffrey L Stott, Noreen Girn, Kimbly J Phillips, Rebecca S. Walker, Paul W. Burridge, Joseph J. Catanese, Steven J.M. Jones, Steven R. Ness, Dan Fuhrmann, Susanna Chan, and Jennifer Asano

Subjects

Molecular Sequence Data, Sequence alignment, Computational biology, Biology, Genome, Synteny, Contig Mapping, Chromosomes, Mice, Species Specificity, Sequence Homology, Nucleic Acid, Animals, Humans, Cloning, Molecular, Conserved Sequence, Genetics, Radiation Hybrid Mapping, Multidisciplinary, Contig, Genome, Human, Genome project, Physical Chromosome Mapping, Human genome, Chromosomes, Human, Pair 6, Sequence Alignment, Reference genome

Abstract

A physical map of a genome is an essential guide for navigation, allowing the location of any gene or other landmark in the chromosomal DNA. We have constructed a physical map of the mouse genome that contains 296 contigs of overlapping bacterial clones and 16,992 unique markers. The mouse contigs were aligned to the human genome sequence on the basis of 51,486 homology matches, thus enabling use of the conserved synteny (correspondence between chromosome blocks) of the two genomes to accelerate construction of the mouse map. The map provides a framework for assembly of whole-genome shotgun sequence data, and a tile path of clones for generation of the reference sequence. Definition of the human-mouse alignment at this level of resolution enables identification of a mouse clone that corresponds to almost any position in the human genome. The human sequence may be used to facilitate construction of other mammalian genome maps using the same strategy.

Published

2002

8. An efficient strategy for large-scale high-throughput transposon-mediated sequencing of cDNA clones

Author

Steven J.M. Jones, Teika Olson, Martin Krzywinski, Jeff M. Stott, Carrie Mathewson, Jennifer Asano, Anna-Liisa Prabhu, Soo Sen Lee, George S. Yang, Yaron S. Butterfield, Jacqueline E. Schein, Ursula Skalska, Marco A. Marra, Angelique Schnerch, Susanna Y. Chan, Kim W. K. MacDonald, Pawan Pandoh, Scott Zuyderduyn, Miranda I. Tsai, Duane E Smailus, and Ranabir Guin

Subjects

Transposable element, DNA, Complementary, Time Factors, Genetic Vectors, Biology, Sensitivity and Specificity, DNA sequencing, Deep sequencing, Article, Substrate Specificity, Bacteriophage mu, Complementary DNA, Genetics, Genomic library, Cloning, Molecular, Sequence (medicine), DNA Primers, Gene Library, Recombination, Genetic, Base Composition, Physical Chromosome Mapping, Sequence Analysis, DNA, Mutagenesis, Insertional, DNA Transposable Elements, Bacteriophage Mu, Monte Carlo Method

Abstract

We describe an efficient high-throughput method for accurate DNA sequencing of entire cDNA clones. Developed as part of our involvement in the Mammalian Gene Collection full-length cDNA sequencing initiative, the method has been used and refined in our laboratory since September 2000. Amenable to large scale projects, we have used the method to generate >7 Mb of accurate sequence from 3695 candidate full-length cDNAs. Sequencing is accomplished through the insertion of Mu transposon into cDNAs, followed by sequencing reactions primed with Mu-specific sequencing primers. Transposon insertion reactions are not performed with individual cDNAs but rather on pools of up to 96 clones. This pooling strategy reduces the number of transposon insertion sequencing libraries that would otherwise be required, reducing the costs and enhancing the efficiency of the transposon library construction procedure. Sequences generated using transposon-specific sequencing primers are assembled to yield the full-length cDNA sequence, with sequence editing and other sequence finishing activities performed as required to resolve sequence ambiguities. Although analysis of the many thousands (22 785) of sequenced Mu transposon insertion events revealed a weak sequence preference for Mu insertion, we observed insertion of the Mu transposon into 1015 of the possible 1024 5mer candidate insertion sites.

Published

2002

9. LongSAGE profiling of nine human embryonic stem cell lines

Author

Deryck R Persaud, Noreen Dhalla, James A. Thomson, Agnes Baross, Anna-Liisa Prabhu, Adrian Ally, Anne Go, Stephanie Menzies, Yongjun Zhao, Asim Siddiqui, Michael D O'Connor, Keith Fichter, Marco A. Marra, Pawan Pandoh, Sean A Rogers, Jaswinder Khattra, Ryan D. Morin, Neil Chahal, Jennifer Asano, Allen Delaney, Connie J. Eaves, Angelique Schnerch, Stephanie Lee, Diana Mah, Michelle Moksa, Kevin Ma, Helen McDonald, Robert A. Holt, Steven J.M. Jones, Thomas Zeng, Daniela S. Gerhard, and Martin Hirst

Subjects

Pluripotent Stem Cells, Cellular differentiation, Method, Sequence alignment, RNA-binding protein, Biology, Cell Line, 03 medical and health sciences, 0302 clinical medicine, Humans, Induced pluripotent stem cell, Embryonic Stem Cells, reproductive and urinary physiology, 030304 developmental biology, 0303 health sciences, Base Sequence, urogenital system, Gene Expression Profiling, RNA-Binding Proteins, Molecular biology, Embryonic stem cell, Human genetics, Cell biology, Gene expression profiling, Cell culture, embryonic structures, biological phenomena, cell phenomena, and immunity, Sequence Alignment, 030217 neurology & neurosurgery

Abstract

Analysis of a 2.6 million longSAGE sequence tag resource generated from nine human embryonic stem cell lines reveals an enrichment of RNA binding proteins and novel ES-specific transcripts., To facilitate discovery of novel human embryonic stem cell (ESC) transcripts, we generated 2.5 million LongSAGE tags from 9 human ESC lines. Analysis of this data revealed that ESCs express proportionately more RNA binding proteins compared with terminally differentiated cells, and identified novel ESC transcripts, at least one of which may represent a marker of the pluripotent state.

Published

2007

10. Resuspension of DNA sequencing reaction products in agarose increases sequence quality on an automated sequencer

Author

Duane E Smailus, Robin Coope, Ranabir Guin, G. Vatcher, Andre Marziali, Teika Olson, Martin Krzywinski, Jeffrey L Stott, Susanna Y. Chan, George S. Yang, Miranda Tsai, Jennifer Asano, Anna-Liisa Prabhu, Marco A. Marra, Pawan Pandoh, Jacquie Schein, and Steven J.M. Jones

Subjects

chemistry.chemical_compound, Chromatography, chemistry, Plasmid dna, Agarose, Sample preparation, Biology, Alkaline lysis, Molecular biology, General Biochemistry, Genetics and Molecular Biology, DNA sequencing, Biotechnology, Sequence (medicine)

Abstract

We are investigating approaches to increase DNA sequencing quality. Since a major factor in sequence generation is the cost of reagents and sample preparations, we have developed and optimized methods to sequence directly plasmid DNA isolated from alkaline lysis preparations. These methods remove the costly PCR and postsequencing purification steps but can result in low sequence quality when using standard resuspension protocols on some sequencing platforms. This work outlines a simple, robust, and inexpensive resuspension protocol for DNA sequencing to correct this shortcoming. Resuspending the sequenced products in agarose before electrophoresis results in a substantial and reproducible increase in sequence quality and read length over resuspension in deionized water and has allowed us to use the aforementioned sample preparation methods to cut considerably the overall sequencing costs without sacrificing sequence quality. We demonstrate that resuspension of unpurified sequence products generated from template DNA isolated by a modified alkaline lysis technique in low concentrations of agarose yields a 384% improvement in sequence quality compared to resuspension in deionized water. Utilizing this protocol, we have produced more than 74 000 high-quality, long-read-length sequences from plasmid DNA template on the MegaBACETM 1000 platform.