Jeff M. Stott
BC Cancer Agency
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Publication
Featured researches published by Jeff M. Stott.
Proceedings of the National Academy of Sciences of the United States of America | 2006
Michael P. McLeod; René L. Warren; William W. L. Hsiao; Naoto Araki; Matthew Myhre; Clinton Fernandes; Daisuke Miyazawa; Wendy Wong; Anita L. Lillquist; Dennis Wang; Manisha Dosanjh; Hirofumi Hara; Anca Petrescu; Ryan D. Morin; George P. Yang; Jeff M. Stott; Jacqueline E. Schein; Heesun Shin; Duane E. Smailus; Asim Siddiqui; Marco A. Marra; Steven J.M. Jones; Robert A. Holt; Fiona S. L. Brinkman; Keisuke Miyauchi; Masao Fukuda; Julian Davies; William W. Mohn; Lindsay D. Eltis
Rhodococcus sp. RHA1 (RHA1) is a potent polychlorinated biphenyl-degrading soil actinomycete that catabolizes a wide range of compounds and represents a genus of considerable industrial interest. RHA1 has one of the largest bacterial genomes sequenced to date, comprising 9,702,737 bp (67% G+C) arranged in a linear chromosome and three linear plasmids. A targeted insertion methodology was developed to determine the telomeric sequences. RHA1s 9,145 predicted protein-encoding genes are exceptionally rich in oxygenases (203) and ligases (192). Many of the oxygenases occur in the numerous pathways predicted to degrade aromatic compounds (30) or steroids (4). RHA1 also contains 24 nonribosomal peptide synthase genes, six of which exceed 25 kbp, and seven polyketide synthase genes, providing evidence that rhodococci harbor an extensive secondary metabolism. Among sequenced genomes, RHA1 is most similar to those of nocardial and mycobacterial strains. The genome contains few recent gene duplications. Moreover, three different analyses indicate that RHA1 has acquired fewer genes by recent horizontal transfer than most bacteria characterized to date and far fewer than Burkholderia xenovorans LB400, whose genome size and catabolic versatility rival those of RHA1. RHA1 and LB400 thus appear to demonstrate that ecologically similar bacteria can evolve large genomes by different means. Overall, RHA1 appears to have evolved to simultaneously catabolize a diverse range of plant-derived compounds in an O2-rich environment. In addition to establishing RHA1 as an important model for studying actinomycete physiology, this study provides critical insights that facilitate the exploitation of these industrially important microorganisms.
Nature | 2002
Simon G. Gregory; Mandeep Sekhon; Jacqueline E. Schein; Shaying Zhao; Kazutoyo Osoegawa; Carol Scott; Richard S. Evans; Paul W. Burridge; Tony Cox; Christopher A. Fox; Richard D. Hutton; Ian R. Mullenger; Kimbly J. Phillips; James Smith; Jim Stalker; Glen Threadgold; Ewan Birney; Kristine M. Wylie; Asif T. Chinwalla; John W. Wallis; LaDeana W. Hillier; Jason Carter; Tony Gaige; Sara Jaeger; Colin Kremitzki; Dan Layman; Jason Maas; Rebecca McGrane; Kelly Mead; Rebecca Walker
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.
Molecular Plant Pathology | 2007
Guanggan Hu; Rob Linning; Brent McCallum; Travis W. Banks; Sylvie Cloutier; Yaron S N Butterfield; Jerry Liu; Robert Kirkpatrick; Jeff M. Stott; George P. Yang; Duane E. Smailus; Steven J.M. Jones; Marco A. Marra; Jacqueline E. Schein; Guus Bakkeren
SUMMARY Thirteen cDNA libraries constructed from small amounts of leaf rust mRNA using optimized methods served as the source for the generation of 25 558 high-quality DNA sequence reads. Five life-cycle stages were sampled: resting urediniospores, urediniospores germinated over water or plant extract, compatible, interactive stages during appressorium or haustorium formation just before sporulation, and an incompatible interaction. mRNA populations were subjected to treatments such as full-length cDNA production, subtractive and normalizing hybridizations, and size selection methods combined with PCR amplification. Pathogen and host sequences from interactive libraries were differentiated in silico using cereal and fungal sequences, codon usage analyses, and by means of a partial prototype cDNA microarray hybridized with genomic DNAs. This yielded a non-redundant unigene set of 9760 putative fungal sequences consisting of 6616 singlets and 3144 contigs, representing 4.7 Mbp. At an E-value 10(-5), 3670 unigenes (38%) matched sequences in various databases and collections but only 694 unigenes (7%) were similar to genes with known functions. In total, 296 unigenes were identified as most probably wheat and ten as rRNA sequences. Annotation rates were low for germinated urediniospores (4%) and appressoria (2%). Gene sets obtained from the various life-cycle stages appear to be remarkably different, suggesting drastic reprogramming of the transcriptome during these major differentiation processes. Redundancy within contigs yielded information about possible expression levels of certain genes among stages. Many sequences were similar to genes from other rusts such as Uromyces and Melampsora species; some of these genes have been implicated in pathogenicity and virulence.
BioTechniques | 2002
G. Vatcher; Duane E. Smailus; Martin Krzywinski; Ranabir Guin; Jeff M. Stott; M. Tsai; Susanna Y. Chan; Pawan Pandoh; George S. Yang; Jennifer Asano; Teika Olson; Anna-Liisa Prabhu; Robin Coope; A. Marziali; Jacquie Schein; Steven J.M. Jones; Marco A. Marra
We are investigating approaches to increase DNA sequencing quality. Since a majorfactor 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 post-sequencing 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 MegaBACET 1000 platform.
Science | 2003
Marco A. Marra; Steven J.M. Jones; Caroline R. Astell; Robert A. Holt; Angela Brooks-Wilson; Yaron S N Butterfield; Jaswinder Khattra; Jennifer Asano; Sarah Barber; Susanna Y. Chan; Alison Cloutier; Shaun M. Coughlin; Doug Freeman; Noreen Girn; Obi L. Griffith; Stephen Leach; Michael Mayo; Helen McDonald; Stephen B. Montgomery; Pawan Pandoh; Anca Petrescu; A. Gordon Robertson; Jacqueline E. Schein; Asim Siddiqui; Duane E. Smailus; Jeff M. Stott; George S. Yang; Francis A. Plummer; Anton Andonov; Harvey Artsob
Genome Research | 2004
Matthew L. Rise; Kristian R. von Schalburg; Gordon D. Brown; Melanie A. Mawer; Robert H. Devlin; Nathanael Kuipers; Maura Busby; Marianne Beetz-Sargent; Roberto Alberto; A. Ross Gibbs; Peter Hunt; Robert Shukin; Jeffrey A. Zeznik; Colleen C. Nelson; Simon R. M. Jones; Duane E. Smailus; Steven J.M. Jones; Jacqueline E. Schein; Marco A. Marra; Yaron S N Butterfield; Jeff M. Stott; Siemon H.S. Ng; William S. Davidson; Ben F. Koop
Genome Research | 2005
Julius Halaschek-Wiener; Jaswinder Khattra; Sheldon J. McKay; Anatoli Timofeyevich Pouzyrev; Jeff M. Stott; George S. Yang; Robert A. Holt; Steven J.M. Jones; Marco A. Marra; Angela Brooks-Wilson; Donald L Riddle
Proceedings of the National Academy of Sciences of the United States of America | 2005
Asim Siddiqui; Jaswinder Khattra; Allen Delaney; Yongjun Zhao; Caroline R. Astell; Jennifer Asano; Ryan Babakaiff; Sarah Barber; Jaclyn Beland; Slavita Bohacec; Mabel Brown-John; Steve Chand; David L. Charest; Anita M. Charters; Rebecca Cullum; Noreen Dhalla; Ruth Featherstone; Daniela S. Gerhard; Brad G. Hoffman; Robert A. Holt; Juan Hou; Byron Yu-Lin Kuo; Lisa L C Lee; Stephanie Lee; Derek Leung; Kevin Ma; Corey Matsuo; Michael Mayo; Helen McDonald; Anna Iiisa Prabhu
BMC Genomics | 2005
Nathalie Pavy; Charles Paule; Lee S. Parsons; John A. Crow; Marie Josee Morency; Janice E. K. Cooke; James E. Johnson; Etienne Noumen; Carine Guillet-Claude; Yaron S N Butterfield; Sarah Barber; George S. Yang; Jerry Liu; Jeff M. Stott; Robert Kirkpatrick; Asim Siddiqui; Robert A. Holt; Marco A. Marra; Armand Séguin; Ernest F. Retzel; Jean Bousquet; John MacKay
Journal of Bacteriology | 2004
René L. Warren; William W. L. Hsiao; Hisashi Kudo; Matt Myhre; Manisha Dosanjh; Anca Petrescu; Hiroyuki Kobayashi; Satoru Shimizu; Keisuke Miyauchi; Eiji Masai; George P. Yang; Jeff M. Stott; Jacquie Schein; Heesun Shin; Jaswinder Khattra; Duane E. Smailus; Yaron S N Butterfield; Asim Siddiqui; Robert A. Holt; Marco A. Marra; Steven J.M. Jones; William W. Mohn; Fiona S. L. Brinkman; Masao Fukuda; Julian Davies; Lindsay D. Eltis
