@article {49793, title = {Maligner: a fast ordered restriction map aligner.}, journal = {Bioinformatics}, volume = {32}, year = {2016}, month = {2016 Apr 1}, pages = {1016-22}, abstract = {

MOTIVATION: The Optical Mapping System discovers structural variants and potentiates sequence assembly of genomes via scaffolding and comparisons that globally validate or correct sequence assemblies. Despite its utility, there are few publicly available tools for aligning optical mapping datasets.

RESULTS: Here we present software, named {\textquoteright}Maligner{\textquoteright}, for the alignment of both single molecule restriction maps (Rmaps) and in silico restriction maps of sequence contigs to a reference. Maligner provides two modes of alignment: an efficient, sensitive dynamic programming implementation that scales to large eukaryotic genomes, and a faster indexed based implementation for finding alignments with unmatched sites in the reference but not the query. We compare our software to other publicly available tools on Rmap datasets and show that Maligner finds more correct alignments in comparable runtime. Lastly, we introduce the M-Score statistic for normalizing alignment scores across restriction maps and demonstrate its utility for selecting high quality alignments.

AVAILABILITY AND IMPLEMENTATION: The Maligner software is written in C ++ and is available at https://github.com/LeeMendelowitz/maligner under the GNU General Public License.

CONTACT: mpop@umiacs.umd.edu.

}, issn = {1367-4811}, doi = {10.1093/bioinformatics/btv711}, author = {Mendelowitz, Lee M and Schwartz, David C and Pop, Mihai} } @article {49800, title = {Mash: fast genome and metagenome distance estimation using MinHash}, journal = {Genome Biology}, year = {2016}, month = {Jan-12-2016}, doi = {10.1186/s13059-016-0997-x}, url = {http://genomebiology.biomedcentral.com/articles/10.1186/s13059-016-0997-xhttp://link.springer.com/content/pdf/10.1186/s13059-016-0997-x}, author = {Ondov, Brian D. and Todd Treangen and Melsted, {\'a}ll and Mallonee, Adam B. and Bergman, Nicholas H. and Koren, Sergey and Phillippy, Adam M.} } @article {49785, title = {Metabolic Network Prediction of Drug Side Effects}, journal = {Cell Systems}, volume = {2}, year = {2016}, month = {Jan-03-2016}, pages = {209 - 213}, issn = {24054712}, doi = {10.1016/j.cels.2016.03.001}, url = {http://linkinghub.elsevier.com/retrieve/pii/S2405471216300734http://api.elsevier.com/content/article/PII:S2405471216300734?httpAccept=text/xmlhttp://api.elsevier.com/content/article/PII:S2405471216300734?httpAccept=text/plain}, author = {Shaked, Itay and Oberhardt, ~A. and Atias, Nir and Sharan, Roded and Ruppin, Eytan} } @article {49823, title = {Metagenomic Assembly: Overview, Challenges and Applications}, journal = {Yale J Biol Med}, volume = {89}, year = {2016}, chapter = {353}, url = {https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5045144/}, author = {Jay S. Ghurye and Victoria Cepeda-Espinoza and Mihai Pop} } @article {49826, title = {methylFlow: cell-specific methylation pattern reconstruction from high-throughput bisulfite-converted DNA sequencing}, journal = {Bioinformatics}, volume = {32}, year = {2016}, month = {Jan-06-2016}, pages = {1618 - 1624}, issn = {1367-4803}, doi = {10.1093/bioinformatics/btw287}, url = {https://academic.oup.com/bioinformatics/article-lookup/doi/10.1093/bioinformatics/btw287https://academic.oup.com/bioinformatics/article/32/11/1618/1743421/methylFlow-cellspecific-methylation-pattern}, author = {Dorri, Faezeh and Mendelowitz, Lee and Corrada Bravo, {\'e}ctor} } @article {49758, title = {Maligner: a fast ordered restriction map aligner}, journal = {Bioinformatics}, year = {2015}, month = {Mar-12-2015}, pages = {btv711}, issn = {1367-4803}, doi = {10.1093/bioinformatics/btv711}, url = {http://bioinformatics.oxfordjournals.org/lookup/doi/10.1093/bioinformatics/btv711}, author = {Mendelowitz, Lee M. and Schwartz, David C. and Pop, Mihai} } @article {49612, title = {Microbiota that affect risk for shigellosis in children in low-income countries}, journal = {Emerg Infect DisEmerg Infect Dis}, volume = {21}, number = {2}, year = {2015}, note = {Lindsay, Brianna
Oundo, Joe
Hossain, M Anowar
Antonio, Martin
Tamboura, Boubou
Walker, Alan W
Paulson, Joseph N
Parkhill, Julian
Omore, Richard
Faruque, Abu S G
Das, Suman Kumar
Ikumapayi, Usman N
Adeyemi, Mitchell
Sanogo, Doh
Saha, Debasish
Sow, Samba
Farag, Tamer H
Nasrin, Dilruba
Li, Shan
Panchalingam, Sandra
Levine, Myron M
Kotloff, Karen
Magder, Laurence S
Hungerford, Laura
Sommerfelt, Halvor
Pop, Mihai
Nataro, James P
Stine, O Colin
U19 090873/PHS HHS/United States
Research Support, N.I.H., Extramural
Research Support, Non-U.S. Gov{\textquoteright}t
Research Support, U.S. Gov{\textquoteright}t, Non-P.H.S.
United States
Emerg Infect Dis. 2015 Feb;21(2):242-50. doi: 10.3201/eid2101.140795.}, month = {Feb}, pages = {242-50}, edition = {2015/01/28}, abstract = {Pathogens in the gastrointestinal tract exist within a vast population of microbes. We examined associations between pathogens and composition of gut microbiota as they relate to Shigella spp./enteroinvasive Escherichia coli infection. We analyzed 3,035 stool specimens (1,735 nondiarrheal and 1,300 moderate-to-severe diarrheal) from the Global Enteric Multicenter Study for 9 enteropathogens. Diarrheal specimens had a higher number of enteropathogens (diarrheal mean 1.4, nondiarrheal mean 0.95; p<0.0001). Rotavirus showed a negative association with Shigella spp. in cases of diarrhea (odds ratio 0.31, 95\% CI 0.17-0.55) and had a large combined effect on moderate-to-severe diarrhea (odds ratio 29, 95\% CI 3.8-220). In 4 Lactobacillus taxa identified by 16S rRNA gene sequencing, the association between pathogen and disease was decreased, which is consistent with the possibility that Lactobacillus spp. are protective against Shigella spp.-induced diarrhea. Bacterial diversity of gut microbiota was associated with diarrhea status, not high levels of the Shigella spp. ipaH gene.}, isbn = {1080-6059 (Electronic)
1080-6040 (Linking)}, author = {Lindsay, B. and Oundo, J. and Hossain, M. A. and Antonio, M. and Tamboura, B. and Walker, A. W. and Paulson, J. N. and Parkhill, J. and Omore, R. and Faruque, A. S. and Das, S. K. and Ikumapayi, U. N. and Adeyemi, M. and Sanogo, D. and Saha, D. and Sow, S. and Farag, T. H. and Nasrin, D. and Li, S. and Panchalingam, S. and Levine, M. M. and Kotloff, K. and Magder, L. S. and Hungerford, L. and Sommerfelt, H. and Pop, M. and Nataro, J. P. and Stine, O. C.} } @article {49573, title = {Modeling cancer metabolism on a genome scale}, volume = {11}, year = {2015}, month = {Jan-06-2015}, pages = {817 - 817}, doi = {10.15252/msb.20145307}, url = {http://msb.embopress.org/cgi/doi/10.15252/msb.20145307}, author = {Yizhak, K. and Chaneton, B. and Gottlieb, E. and Ruppin, E.} } @article {49511, title = {A molecular phylogeny for the oldest (nonditrysian) lineages of extant Lepidoptera, with implications for classification, comparative morphology and life-history evolution}, journal = {Systematic Entomology}, year = {2015}, month = {05/2015}, pages = {n/a - n/a}, doi = {10.1111/syen.12129}, author = {Regier, Jerome C and Mitter, Charles and KRISTENSEN, NIELS P. and Davis, Donald R. and VAN NIEUKERKEN, ERIK J. and ROTA, JADRANKA and Simonsen, Thomas J. and Mitter, Kim T. and Kawahara, Akito Y. and Yen, Shen-Horn and Michael P. Cummings and Zwick, Andreas} } @article {49582, title = {Moving ahead on harnessing synthetic lethality to fight cancer}, volume = {2}, year = {2015}, month = {Mar-04-2015}, pages = {e977150}, doi = {10.4161/23723556.2014.977150}, url = {http://www.tandfonline.com/doi/abs/10.4161/23723556.2014.977150}, author = {Jerby-Arnon, Livnat and Ruppin, Eytan} } @article {49588, title = {Maximal Sum of Metabolic Exchange Fluxes Outperforms Biomass Yield as a Predictor of Growth Rate of Microorganisms}, volume = {9}, year = {2014}, month = {Mar-05-2016}, pages = {e98372}, doi = {10.1371/journal.pone.0098372}, url = {http://journals.plos.org/plosone/article?id=10.1371/journal.pone.0098372}, author = {Zarecki, Raphy and Oberhardt, Matthew A. and Yizhak, Keren and Wagner, Allon and Shtifman Segal, Ella and Freilich, Shiri and Henry, Christopher S. and Gophna, Uri and Ruppin, Eytan}, editor = {Fong, Stephen S.} } @article {49605, title = {Minfi: a flexible and comprehensive Bioconductor package for the analysis of Infinium DNA methylation microarrays.}, volume = {30}, year = {2014}, month = {2014 May 15}, pages = {1363-9}, abstract = {

MOTIVATION: The recently released Infinium HumanMethylation450 array (the {\textquoteright}450k{\textquoteright} array) provides a high-throughput assay to quantify DNA methylation (DNAm) at \~{}450 000 loci across a range of genomic features. Although less comprehensive than high-throughput sequencing-based techniques, this product is more cost-effective and promises to be the most widely used DNAm high-throughput measurement technology over the next several years.

RESULTS: Here we describe a suite of computational tools that incorporate state-of-the-art statistical techniques for the analysis of DNAm data. The software is structured to easily adapt to future versions of the technology. We include methods for preprocessing, quality assessment and detection of differentially methylated regions from the kilobase to the megabase scale. We show how our software provides a powerful and flexible development platform for future methods. We also illustrate how our methods empower the technology to make discoveries previously thought to be possible only with sequencing-based methods.

AVAILABILITY AND IMPLEMENTATION: http://bioconductor.org/packages/release/bioc/html/minfi.html.

CONTACT: khansen@jhsph.edu; rafa@jimmy.harvard.edu

SUPPLEMENTARY INFORMATION: Supplementary data are available at Bioinformatics online.

}, keywords = {Aged, algorithms, Colonic Neoplasms, DNA Methylation, Genome, High-Throughput Nucleotide Sequencing, HUMANS, Oligonucleotide Array Sequence Analysis, Polymorphism, Single Nucleotide, software}, issn = {1367-4811}, doi = {10.1093/bioinformatics/btu049}, author = {Aryee, Martin J and Jaffe, Andrew E and Corrada-Bravo, Hector and Ladd-Acosta, Christine and Feinberg, Andrew P and Hansen, Kasper D and Irizarry, Rafael A} } @article {49514, title = {A molecular phylogeny and revised classification for the oldest ditrysian moth lineages (Lepidoptera: Tineoidea), with implications for ancestral feeding habits of the mega-diverse Ditrysia}, journal = {Systematic Entomology}, volume = {40}, year = {2014}, month = {04/2015}, pages = {409 - 432}, doi = {10.1111/syen.12110}, author = {Regier, Jerome C and Mitter, Charles and Davis, Donald R. and HARRISON, TERRY L. and Sohn, Jae-Cheon and Michael P. Cummings and Zwick, Andreas and Mitter, Kim T.} } @article {38372, title = {MetAMOS: a modular and open source metagenomic assembly and analysis pipeline}, journal = {Genome BiolGenome Biol}, volume = {14}, year = {2013}, note = {Treangen, Todd JKoren, SergeySommer, Daniel DLiu, BoAstrovskaya, IrinaOndov, BrianDarling, Aaron EPhillippy, Adam MPop, MihaiGenome Biol. 2013 Jan 15;14(1):R2.
Genome biology}, type = {10.1186/gb-2013-14-1-r2}, abstract = {ABSTRACT: We describe MetAMOS, an open source and modular metagenomic assembly and analysis pipeline. MetAMOS represents an important step towards fully automated metagenomic analysis, starting with next-generation sequencing reads and producing genomic scaffolds, open-reading frames and taxonomic or functional annotations. MetAMOS can aid in reducing assembly errors, commonly encountered when assembling metagenomic samples, and improves taxonomic assignment accuracy while also reducing computational cost. MetAMOS can be downloaded from: https://github.com/treangen/MetAMOS.}, isbn = {1465-6914 (Electronic)1465-6906 (Linking)}, author = {Todd Treangen and Koren, S. and Sommer, D. D. and Liu, B. and Irina Astrovskaya and Ondov, B. and Darling, A. E. and Phillippy, A. M. and M. Pop} } @article {38389, title = {A molecular phylogeny for Yponomeutoidea (Insecta, Lepidoptera, Ditrysia) and its implications for classification, biogeography and\ the evolution of host plant use}, journal = {PLoS One}, year = {2013}, author = {J. C. Sohn and Regier, J. C. and Mitter, C. and D. Davis and J. F. Landry and Zwick, A. and Michael P. Cummings} } @article {49517, title = {A molecular phylogeny for the leaf-roller moths (Lepidoptera: Tortricidae) and its implications for classification and life history evolution.}, journal = {PloS one}, volume = {7}, year = {2012}, month = {2012}, pages = {e35574}, abstract = {Tortricidae, one of the largest families of microlepidopterans, comprise about 10,000 described species worldwide, including important pests, biological control agents and experimental models. Understanding of tortricid phylogeny, the basis for a predictive classification, is currently provisional. We present the first detailed molecular estimate of relationships across the tribes and subfamilies of Tortricidae, assess its concordance with previous morphological evidence, and re-examine postulated evolutionary trends in host plant use and biogeography.}, author = {Regier, Jerome C and Brown, John W and Mitter, Charles and Baixeras, Joaquin and Cho, Soowon and Michael P. Cummings and Zwick, Andreas} } @article {49515, title = {A molecular phylogeny for the pyraloid moths (Lepidoptera: Pyraloidea) and its implications for higher-level classification}, journal = {Systematic Entomology}, volume = {37}, year = {2012}, month = {Jan-10-2012}, pages = {635 - 656}, doi = {10.1111/sen.2012.37.issue-410.1111/j.1365-3113.2012.00641.x}, url = {http://doi.wiley.com/10.1111/sen.2012.37.issue-4http://doi.wiley.com/10.1111/j.1365-3113.2012.00641.x}, author = {Regier, Jerome C. and Mitter, Charles and SOLIS, M. ALMA and HAYDEN, JAMES E. and LANDRY, BERNARD and NUSS, MATTHIAS and Simonsen, Thomas J. and Yen, Shen-Horn and Zwick, Andreas and Michael P. Cummings} } @article {49518, title = {MrBayes 3.2: Efficient Bayesian Phylogenetic Inference and Model Choice Across a Large Model Space}, journal = {Systematic Biology}, volume = {61}, year = {2012}, month = {05/2012}, pages = {539 - 542}, issn = {1076-836X}, doi = {10.1093/sysbio/sys029}, author = {F. Ronquist and Teslenko, M. and van der Mark, P. and Ayres, D. L. and Darling, A. and Hohna, S. and B. Larget and Liu, L. and Suchard, M. A. and J. P. Huelsenbeck} } @article {38393, title = {Myocardin-like Protein (MKL)-2 Regulates TGF-beta Signaling}, journal = {Embryonic Stem Cells and the Developing Vasculature DevelopmentEmbryonic Stem Cells and the Developing Vasculature Development}, year = {2012}, author = {Li, Jian and Nina, Bowens and Lan, Cheng and Mary, Chen and Sridhar Hannenhalli and Xiaohong, Zhu and Thomas, P. Cappola and Parmacek, Michael S.} } @proceedings {38367, title = {MDMap: A system for data-driven layout and exploration of molecular dynamics simulations}, year = {2011}, month = {2011}, type = {10.1109/BioVis.2011.6094055}, abstract = {Contemporary molecular dynamics simulations result in a glut of simulation data, making analysis and discovery a difficult and burdensome task. We present MDMap, a system designed to summarize long-running molecular dynamics (MD) simulations. We represent a molecular dynamics simulation as a state transition graph over a set of intermediate (stable and semi-stable) states. The transitions amongst the states together with their frequencies represent the flow of a biomolecule through the trajectory space. MDMap automatically determines potential intermediate conformations and the transitions amongst them by analyzing the conformational space explored by the MD simulation. MDMap is an automated system to visualize MD simulations as state-transition diagrams, and can replace the current tedious manual layouts of biomolecular folding landscapes with an automated tool. The layout of the representative states and the corresponding transitions among them is presented to the user as a visual synopsis of the long-running MD simulation. We compare and contrast multiple presentations of the state transition diagrams, such as conformational embedding, and spectral, hierarchical, and force-directed graph layouts. We believe this system could provide a road-map for the visualization of other stochastic time-varying simulations in a variety of different domains.}, keywords = {Biology, biomolecular, computing, data, digital, driven, DYNAMICS, exploration, folding, graph, landscapes, Layout, MDMap, method, molecular, processes, simulation, Simulations, space, state, Stochastic, THEORY, time-varying, Trajectory, transition}, author = {Patro, R. and Ip, Cheuk Yiu and Bista, S. and Cho, S. S. and Thirumalai, D. and Varshney, Amitabh} } @article {38370, title = {Metagenomic 16S rDNA Targeted PCR-DGGE in Determining Bacterial Diversity in Aquatic Ecosystem}, journal = {Bangladesh Journal of MicrobiologyBangladesh Journal of Microbiology}, volume = {27}, year = {2011}, type = {10.3329/bjm.v27i2.9171}, abstract = {Bacterial numbers in surface water samples, collected randomly from six different water bodies, were estimated by acridine orange direct counting (AODC) and conventional culture-based heterotrophic plate counting (HPC). Bacterial genomic DNA was prepared from water samples by employing methods used for stool samples, including the population dynamics, were determined by primer extension of the 16S rDNA (V6/V8 region) using polymerase chain reaction (PCR), followed by denaturing gradient gel electrophoresis (DGGE), a metagenomic tool that is capable of separating unrelated DNAs based on the differences in their sequences and GC contents. The bacterial numbers in water samples ranged from 103 {\textendash} 106 CFU/ mL for HPC and 104 {\textendash} 107 cells/ mL for AODC, showing that a great majority of bacteria prevail as uncultivable which do not respond to culture methods that are used widely for tracking bacterial pathogens. The acridine orange-stained bacteria varied in sizes and shapes, and appeared either as planktonic (solitary) cells or as clusters of biofilms, showing the presence of diverse community under the epifluorescence microscope. The DGGE of the ca. 457 bp amplicons, as confirmed by agarose gel electrophoresis, produced bands that ranged in intensities and numbers from 18 to 31, with each band possibly indicating the presence of one or more closely related bacterial species. The enrichment of pathogenic bacteria in the aquatic ecosystem is known to precede the seasonal diarrhoeal outbreaks; therefore, bacterial community dynamics determined by Metagenomic 16S PCR-DGGE during pre-epidemic enrichment appears promising in predicting the upcoming diarrheal outbreaks.}, isbn = {1011-9981}, author = {Hasan, Nur A. and Chowdhury, W. Bari and Rahim, Niaz and Sultana, Marzia and Shabnam, S. Antara and Mai, Volker and Ali, Afsar and Morris, Glen J. and Sack, R. Bradley and Huq, Anwar and Rita R. Colwell and Endtz, Hubert Ph and Cravioto, Alejandro and Alam, Munirul} } @article {38373, title = {MetaPath: identifying differentially abundant metabolic pathways in metagenomic datasets}, journal = {BMC ProceedingsBMC Proceedings}, volume = {5}, year = {2011}, type = {10.1186/1753-6561-5-S2-S9}, abstract = {Enabled by rapid advances in sequencing technology, metagenomic studies aim to characterize entire communities of microbes bypassing the need for culturing individual bacterial members. One major goal of metagenomic studies is to identify specific functional adaptations of microbial communities to their habitats. The functional profile and the abundances for a sample can be estimated by mapping metagenomic sequences to the global metabolic network consisting of thousands of molecular reactions. Here we describe a powerful analytical method (MetaPath) that can identify differentially abundant pathways in metagenomic datasets, relying on a combination of metagenomic sequence data and prior metabolic pathway knowledge.}, isbn = {1753-6561}, author = {Liu, Bo and M. Pop} } @article {49830, title = {A Model for Early Prediction of Facial Nerve Recovery After Vestibular Schwannoma Surgery}, journal = {Otology \& Neurotology}, volume = {32}, year = {2011}, month = {Jan-01-2011}, pages = {826 - 833}, issn = {1531-7129}, doi = {10.1097/MAO.0b013e31821b0afd}, url = {http://content.wkhealth.com/linkback/openurl?sid=WKPTLP:landingpage\&an=00129492-201107000-00019}, author = {Rivas, Alejandro and Boahene, Kofi D. and Bravo, H{\'e}ctor Corrada and Tan, Marietta and Tamargo, Rafael J. and Francis, Howard W.} } @proceedings {38374, title = {MetaPhyler: Taxonomic profiling for metagenomic sequences}, year = {2010}, month = {2010}, publisher = {IEEE}, type = {10.1109/BIBM.2010.5706544}, abstract = {A major goal of metagenomics is to characterize the microbial diversity of an environment. The most popular approach relies on 16S rRNA sequencing, however this approach can generate biased estimates due to differences in the copy number of the 16S rRNA gene between even closely related organisms, and due to PCR artifacts. The taxonomic composition can also be determined from whole-metagenome sequencing data by matching individual sequences against a database of reference genes. One major limitation of prior methods used for this purpose is the use of a universal classification threshold for all genes at all taxonomic levels. We propose that better classification results can be obtained by tuning the taxonomic classifier to each matching length, reference gene, and taxonomic level. We present a novel taxonomic profiler MetaPhyler, which uses marker genes as a taxonomic reference. Results on simulated datasets demonstrate that MetaPhyler outperforms other tools commonly used in this context (CARMA, Megan and PhymmBL). We also present interesting results obtained by applying MetaPhyler to a real metagenomic dataset.}, keywords = {Bioinformatics, CARMA comparison, Databases, Genomics, Linear regression, marker genes, matching length, Megan comparison, metagenomic sequences, metagenomics, MetaPhyler, microbial diversity, microorganisms, molecular biophysics, molecular configurations, Pattern classification, pattern matching, phylogenetic classification, Phylogeny, PhymmBL comparison, reference gene database, Sensitivity, sequence matching, taxonomic classifier, taxonomic level, taxonomic profiling, whole metagenome sequencing data}, isbn = {978-1-4244-8306-8}, author = {Liu, Bo and Gibbons, T. and Ghodsi, M. and M. Pop} } @article {38381, title = {Mimosa: Mixture model of co-expression to detect modulators of regulatory interaction}, journal = {Algorithms for Molecular BiologyAlgorithms for Molecular Biology}, volume = {5}, year = {2010}, type = {10.1186/1748-7188-5-4}, abstract = {Functionally related genes tend to be correlated in their expression patterns across multiple conditions and/or tissue-types. Thus co-expression networks are often used to investigate functional groups of genes. In particular, when one of the genes is a transcription factor (TF), the co-expression-based interaction is interpreted, with caution, as a direct regulatory interaction. However, any particular TF, and more importantly, any particular regulatory interaction, is likely to be active only in a subset of experimental conditions. Moreover, the subset of expression samples where the regulatory interaction holds may be marked by presence or absence of a modifier gene, such as an enzyme that post-translationally modifies the TF. Such subtlety of regulatory interactions is overlooked when one computes an overall expression correlation.}, isbn = {1748-7188}, author = {Hansen, Matthew and Everett, Logan and Singh, Larry and Sridhar Hannenhalli} } @article {49650, title = {A model for using a concept inventory as a tool for students{\textquoteright} assessment and faculty professional development.}, journal = {CBE Life Sci Educ}, volume = {9}, year = {2010}, month = {2010 Winter}, pages = {408-16}, abstract = {

This essay describes how the use of a concept inventory has enhanced professional development and curriculum reform efforts of a faculty teaching community. The Host Pathogen Interactions (HPI) teaching team is composed of research and teaching faculty with expertise in HPI who share the goal of improving the learning experience of students in nine linked undergraduate microbiology courses. To support evidence-based curriculum reform, we administered our HPI Concept Inventory as a pre- and postsurvey to approximately 400 students each year since 2006. The resulting data include student scores as well as their open-ended explanations for distractor choices. The data have enabled us to address curriculum reform goals of 1) reconciling student learning with our expectations, 2) correlating student learning with background variables, 3) understanding student learning across institutions, 4) measuring the effect of teaching techniques on student learning, and 5) demonstrating how our courses collectively form a learning progression. The analysis of the concept inventory data has anchored and deepened the team{\textquoteright}s discussions of student learning. Reading and discussing students{\textquoteright} responses revealed the gap between our understanding and the students{\textquoteright} understanding. We provide evidence to support the concept inventory as a tool for assessing student understanding of HPI concepts and faculty development.

}, keywords = {Curriculum, Faculty, Models, Theoretical, Research, Students, Teaching}, issn = {1931-7913}, doi = {10.1187/cbe.10-05-0069}, author = {Marbach-Ad, Gili and McAdams, Katherine C and Benson, Spencer and Briken, Volker and Cathcart, Laura and Chase, Michael and El-Sayed, Najib M and Frauwirth, Kenneth and Fredericksen, Brenda and Joseph, Sam W and Lee, Vincent and McIver, Kevin S and Mosser, David and Quimby, B Booth and Shields, Patricia and Song, Wenxia and Stein, Daniel C and Stewart, Richard and Thompson, Katerina V and Smith, Ann C} } @article {49833, title = {Model-Based Quality Assessment and Base-Calling for Second-Generation Sequencing Data}, journal = {Biometrics}, volume = {66}, year = {2010}, month = {Jan-09-2010}, pages = {665 - 674}, doi = {10.1111/j.1541-0420.2009.01353.x}, url = {http://doi.wiley.com/10.1111/j.1541-0420.2009.01353.xhttps://api.wiley.com/onlinelibrary/tdm/v1/articles/10.1111\%2Fj.1541-0420.2009.01353.x}, author = {Bravo, H{\'e}ctor Corrada and Irizarry, Rafael A.} } @article {49749, title = {Measuring differential gene expression by short read sequencing: quantitative comparison to 2-channel gene expression microarrays.}, journal = {BMC Genomics}, volume = {10}, year = {2009}, month = {2009}, pages = {221}, abstract = {

BACKGROUND: High-throughput cDNA synthesis and sequencing of poly(A)-enriched RNA is rapidly emerging as a technology competing to replace microarrays as a quantitative platform for measuring gene expression.

RESULTS: Consequently, we compared full length cDNA sequencing to 2-channel gene expression microarrays in the context of measuring differential gene expression. Because of its comparable cost to a gene expression microarray, our study focused on the data obtainable from a single lane of an Illumina 1 G sequencer. We compared sequencing data to a highly replicated microarray experiment profiling two divergent strains of S. cerevisiae.

CONCLUSION: Using a large number of quantitative PCR (qPCR) assays, more than previous studies, we found that neither technology is decisively better at measuring differential gene expression. Further, we report sequencing results from a diploid hybrid of two strains of S. cerevisiae that indicate full length cDNA sequencing can discover heterozygosity and measure quantitative allele-specific expression simultaneously.

}, keywords = {algorithms, DNA, Complementary, DNA, Fungal, Gene Expression Profiling, Oligonucleotide Array Sequence Analysis, Saccharomyces cerevisiae, sequence alignment, Sequence Analysis, DNA}, issn = {1471-2164}, doi = {10.1186/1471-2164-10-221}, author = {Bloom, Joshua S and Khan, Zia and Kruglyak, Leonid and Singh, Mona and Caudy, Amy A} } @article {49559, title = {Measuring differential gene expression by short read sequencing: quantitative comparison to 2-channel gene expression microarrays}, volume = {10}, year = {2009}, month = {Jan-01-2009}, pages = {221}, issn = {1471-2164}, doi = {10.1186/1471-2164-10-221}, url = {http://www.biomedcentral.com/1471-2164/10/221}, author = {Bloom, Joshua S and Khan, Zia and Kruglyak, Leonid and Singh, Mona and Caudy, Amy A} } @article {38379, title = {Microbial oceanography in a sea of opportunity}, journal = {NatureNature}, volume = {459}, year = {2009}, type = {10.1038/nature08056}, abstract = {Plankton use solar energy to drive the nutrient cycles that make the planet habitable for larger organisms. We can now explore the diversity and functions of plankton using genomics, revealing the gene repertoires associated with survival in the oceans. Such studies will help us to appreciate the sensitivity of ocean systems and of the ocean{\textquoteright}s response to climate change, improving the predictive power of climate models.}, keywords = {Astronomy, astrophysics, Biochemistry, Bioinformatics, Biology, biotechnology, cancer, cell cycle, cell signalling, climate change, Computational Biology, development, developmental biology, DNA, drug discovery, earth science, ecology, environmental science, Evolution, evolutionary biology, functional genomics, Genetics, Genomics, geophysics, immunology, interdisciplinary science, life, marine biology, materials science, medical research, medicine, metabolomics, molecular biology, molecular interactions, nanotechnology, Nature, neurobiology, neuroscience, palaeobiology, pharmacology, Physics, proteomics, quantum physics, RNA, Science, science news, science policy, signal transduction, structural biology, systems biology, transcriptomics}, isbn = {0028-0836}, author = {Bowler, Chris and Karl, David M. and Rita R. Colwell} } @article {38380, title = {Mimosa: mixture model of co-expression to detect modulators of regulatory interaction}, journal = {Algorithms in BioinformaticsAlgorithms in Bioinformatics}, year = {2009}, publisher = {Springer Berlin/Heidelberg}, author = {Hansen, M. and Everett, L. and Singh, L. and Sridhar Hannenhalli} } @article {38385, title = {Model-based quality assessment and base-calling for second-generation sequencing data}, journal = {Johns Hopkins University, Dept. of Biostatistics Working PapersJohns Hopkins University, Dept. of Biostatistics Working Papers}, year = {2009}, author = {Irizarry, R. A. and H{\'e}ctor Corrada Bravo} } @article {38386, title = {Modeling and visualization of human activities for multicamera networks}, journal = {EURASIP Journal on Image and Video ProcessingEURASIP Journal on Image and Video Processing}, volume = {2009}, year = {2009}, author = {Sankaranarayanan, A. C. and Patro, R. and Turaga, P. and Varshney, Amitabh and Chellappa, Rama} } @article {38391, title = {Motifs and cis-regulatory modules mediating the expression of genes co-expressed in presynaptic neurons}, journal = {Genome BiologyGenome Biology}, volume = {10}, year = {2009}, type = {10.1186/gb-2009-10-7-r72}, abstract = {Hundreds of proteins modulate neurotransmitter release and synaptic plasticity during neuronal development and in response to synaptic activity. The expression of genes in the pre- and post-synaptic neurons is under stringent spatio-temporal control, but the mechanism underlying the neuronal expression of these genes remains largely unknown.}, isbn = {1465-6906}, author = {Liu, Rui and Sridhar Hannenhalli and Bucan, Maja} } @inbook {38365, title = {The marine environment and human health: the cholera model}, booktitle = {Global Climate Change and Extreme Weather Events: Understanding the Contributions to Infectious Disease EmergenceGlobal Climate Change and Extreme Weather Events: Understanding the Contributions to Infectious Disease Emergence}, year = {2008}, publisher = {National Academies Press}, organization = {National Academies Press}, isbn = {9780309124027}, author = {Rita R. Colwell}, editor = {Relman, David} } @article {38366, title = {Maternal depletion of CTCF reveals multiple functions during oocyte and preimplantation embryo development}, journal = {DevelopmentDevelopment}, volume = {135}, year = {2008}, publisher = {The Company of Biologists Limited}, author = {Wan, L. B. and Pan, H. and Sridhar Hannenhalli and Cheng, Y. and Ma, J. and Fedoriw, A. and Lobanenkov, V. and Latham, K. E. and Schultz, R. M. and Bartolomei, M. S.} } @article {38383, title = {The minimum information about a genome sequence (MIGS) specification}, journal = {Nature biotechnologyNature biotechnology}, volume = {26}, year = {2008}, note = {http://www.ncbi.nlm.nih.gov/pubmed/18464787?dopt=Abstract}, type = {10.1038/nbt1360}, abstract = {With the quantity of genomic data increasing at an exponential rate, it is imperative that these data be captured electronically, in a standard format. Standardization activities must proceed within the auspices of open-access and international working bodies. To tackle the issues surrounding the development of better descriptions of genomic investigations, we have formed the Genomic Standards Consortium (GSC). Here, we introduce the minimum information about a genome sequence (MIGS) specification with the intent of promoting participation in its development and discussing the resources that will be required to develop improved mechanisms of metadata capture and exchange. As part of its wider goals, the GSC also supports improving the {\textquoteright}transparency{\textquoteright} of the information contained in existing genomic databases.}, keywords = {Chromosome mapping, Databases, Factual, information dissemination, Information Storage and Retrieval, Information Theory, Internationality}, author = {Field, Dawn and Garrity, George and Gray, Tanya and Morrison, Norman and J. Selengut and Sterk, Peter and Tatusova, Tatiana and Thomson, Nicholas and Allen, Michael J. and Angiuoli, Samuel V. and Ashburner, Michael and Axelrod, Nelson and Baldauf, Sandra and Ballard, Stuart and Boore, Jeffrey and Cochrane, Guy and Cole, James and Dawyndt, Peter and De Vos, Paul and DePamphilis, Claude and Edwards, Robert and Faruque, Nadeem and Feldman, Robert and Gilbert, Jack and Gilna, Paul and Gl{\"o}ckner, Frank Oliver and Goldstein, Philip and Guralnick, Robert and Haft, Dan and Hancock, David and Hermjakob, Henning and Hertz-Fowler, Christiane and Hugenholtz, Phil and Joint, Ian and Kagan, Leonid and Kane, Matthew and Kennedy, Jessie and Kowalchuk, George and Kottmann, Renzo and Kolker, Eugene and Kravitz, Saul and Kyrpides, Nikos and Leebens-Mack, Jim and Lewis, Suzanna E. and Li, Kelvin and Lister, Allyson L. and Lord, Phillip and Maltsev, Natalia and Markowitz, Victor and Martiny, Jennifer and Methe, Barbara and Mizrachi, Ilene and Moxon, Richard and Nelson, Karen and Parkhill, Julian and Proctor, Lita and White, Owen and Sansone, Susanna-Assunta and Spiers, Andrew and Stevens, Robert and Swift, Paul and Taylor, Chris and Tateno, Yoshio and Tett, Adrian and Turner, Sarah and Ussery, David and Vaughan, Bob and Ward, Naomi and Whetzel, Trish and San Gil, Ingio and Wilson, Gareth and Wipat, Anil} } @article {38388, title = {A molecular footprint of limb loss: sequence variation of the autopodial identity gene Hoxa-13}, journal = {J Mol EvolJ Mol Evol}, volume = {67}, year = {2008}, type = {10.1007/s00239-008-9156-7}, abstract = {The homeobox gene Hoxa-13 codes for a transcription factor involved in multiple functions, including body axis and hand/foot development in tetrapods. In this study we investigate whether the loss of one function (e.g., limb loss in snakes) left a molecular footprint in exon 1 of Hoxa-13 that could be associated with the release of functional constraints caused by limb loss. Fragments of the Hoxa-13 exon 1 were sequenced from 13 species and analyzed, with additional published sequences of the same region, using relative rates and likelihood-ratio tests. Five amino acid sites in exon 1 of Hoxa-13 were detected as evolving under positive selection in the stem lineage of snakes. To further investigate whether there is an association between limb loss and sequence variation in Hoxa-13, we used the random forest method on an alignment that included shark, basal fish lineages, and "eu-tetrapods" such as mammals, turtle, alligator, and birds. The random forest method approaches the problem as one of classification, where we seek to predict the presence or absence of autopodium based on amino acid variation in Hoxa-13 sequences. Different alignments tested were associated with similar error rates (18.42\%). The random forest method suggested that phenotypic states (autopodium present and absent) can often be correctly predicted based on Hoxa-13 sequences. Basal, nontetrapod gnat-hostomes that never had an autopodium were consistently classified as limbless together with the snakes, while eu-tetrapods without any history of limb loss in their phylogeny were also consistently classified as having a limb. Misclassifications affected mostly lizards, which, as a group, have a history of limb loss and limb re-evolution, and the urodele and caecilian in our sample. We conclude that a molecular footprint can be detected in Hoxa-13 that is associated with the lack of an autopodium; groups with classification ambiguity (lizards) are characterized by a history of repeated limb loss and possible limb re-evolution.}, author = {Kohlsdorf, T. and Michael P. Cummings and Lynch, V. J. and Stopper, G. F. and Takahashi, K. and Wagner, G. P.} } @article {49642, title = {Members of a large retroposon family are determinants of post-transcriptional gene expression in Leishmania.}, journal = {PLoS Pathog}, volume = {3}, year = {2007}, month = {2007 Sep 7}, pages = {1291-307}, abstract = {

Trypanosomatids are unicellular protists that include the human pathogens Leishmania spp. (leishmaniasis), Trypanosoma brucei (sleeping sickness), and Trypanosoma cruzi (Chagas disease). Analysis of their recently completed genomes confirmed the presence of non-long-terminal repeat retrotransposons, also called retroposons. Using the 79-bp signature sequence common to all trypanosomatid retroposons as bait, we identified in the Leishmania major genome two new large families of small elements--LmSIDER1 (785 copies) and LmSIDER2 (1,073 copies)--that fulfill all the characteristics of extinct trypanosomatid retroposons. LmSIDERs are approximately 70 times more abundant in L. major compared to T. brucei and are found almost exclusively within the 3{\textquoteright}-untranslated regions (3{\textquoteright}UTRs) of L. major mRNAs. We provide experimental evidence that LmSIDER2 act as mRNA instability elements and that LmSIDER2-containing mRNAs are generally expressed at lower levels compared to the non-LmSIDER2 mRNAs. The considerable expansion of LmSIDERs within 3{\textquoteright}UTRs in an organism lacking transcriptional control and their role in regulating mRNA stability indicate that Leishmania have probably recycled these short retroposons to globally modulate the expression of a number of genes. To our knowledge, this is the first example in eukaryotes of the domestication and expansion of a family of mobile elements that have evolved to fulfill a critical cellular function.

}, keywords = {3{\textquoteright} Untranslated Regions, Animals, Base Sequence, Biological Evolution, Down-Regulation, Gene Expression Regulation, Genome, Protozoan, Leishmania, Leishmania major, Molecular Sequence Data, Retroelements, RNA, Messenger, sequence alignment, Trypanosoma brucei brucei, Trypanosoma cruzi}, issn = {1553-7374}, doi = {10.1371/journal.ppat.0030136}, author = {Bringaud, Frederic and M{\"u}ller, Michaela and Cerqueira, Gustavo Coutinho and Smith, Martin and Rochette, Annie and el-Sayed, Najib M A and Papadopoulou, Barbara and Ghedin, Elodie} } @article {38375, title = {MetaProm: a neural network based meta-predictor for alternative human promoter prediction}, journal = {BMC genomicsBMC Genomics}, volume = {8}, year = {2007}, publisher = {BioMed Central Ltd}, author = {Wang, J. and Ungar, L. H. and Tseng, H. and Sridhar Hannenhalli} } @book {49866, title = {Methods in Molecular BiologyComparative GenomicsAnalyzing Patterns of Microbial Evolution Using the Mauve Genome Alignment System}, volume = {396}, year = {2007}, pages = {135 - 152}, publisher = {Humana Press}, organization = {Humana Press}, address = {Totowa, NJ}, isbn = {978-1-934115-37-4}, issn = {1064-3745}, doi = {10.1007/978-1-59745-515-210.1007/978-1-59745-515-2_10}, url = {http://www.springerlink.com/index/10.1007/978-1-59745-515-2http://www.springerlink.com/index/pdf/10.1007/978-1-59745-515-2http://link.springer.com/10.1007/978-1-59745-515-2_10http://www.springerlink.com/index/pdf/10.1007/978-1-59745-515-2_10}, author = {Darling, Aaron E and Todd Treangen and Messeguer, Xavier and Perna, Nicole T}, editor = {Walker, John M. and Bergman, Nicholas H.} } @article {38377, title = {Microarray analysis of gene expression induced by sexual contact in Schistosoma mansoni}, journal = {BMC GenomicsBMC Genomics}, volume = {8}, year = {2007}, type = {10.1186/1471-2164-8-181}, abstract = {BACKGROUND:The parasitic trematode Schistosoma mansoni is one of the major causative agents of Schistosomiasis, a disease that affects approximately 200 million people, mostly in developing countries. Since much of the pathology is associated with eggs laid by the female worm, understanding the mechanisms involved in oogenesis and sexual maturation is an important step towards the discovery of new targets for effective drug therapy. It is known that the adult female worm only develops fully in the presence of a male worm and that the rates of oviposition and maturation of eggs are significantly increased by mating. In order to study gene transcripts associated with sexual maturation and oviposition, we compared the gene expression profiles of sexually mature and immature parasites using DNA microarrays.RESULTS:For each experiment, three amplified RNA microarray hybridizations and their dye swaps were analyzed. Our results show that 265 transcripts are differentially expressed in adult females and 53 in adult males when mature and immature worms are compared. Of the genes differentially expressed, 55\% are expressed at higher levels in paired females while the remaining 45\% are more expressed in unpaired ones and 56.6\% are expressed at higher levels in paired male worms while the remaining 43.4\% are more expressed in immature parasites. Real-time RT-PCR analysis validated the microarray results. Several new maturation associated transcripts were identified. Genes that were up-regulated in single-sex females were mostly related to energy generation (i.e. carbohydrate and protein metabolism, generation of precursor metabolites and energy, cellular catabolism, and organelle organization and biogenesis) while genes that were down-regulated related to RNA metabolism, reactive oxygen species metabolism, electron transport, organelle organization and biogenesis and protein biosynthesis.CONCLUSION:Our results confirm previous observations related to gene expression induced by sexual maturation in female schistosome worms. They also increase the list of S. mansoni maturation associated transcripts considerably, therefore opening new and exciting avenues for the study of the conjugal biology and development of new drugs against schistosomes.}, isbn = {1471-2164}, author = {Waisberg, Michael and Lobo, Francisco and Cerqueira, Gustavo and Passos, Liana and Carvalho, Omar and Franco, Gloria and Najib M. El-Sayed} } @article {38384, title = {Minimus: a fast, lightweight genome assembler}, journal = {BMC bioinformaticsBMC Bioinformatics}, volume = {8}, year = {2007}, publisher = {BioMed Central Ltd}, author = {Sommer, D. and Delcher, A. and Salzberg, S. and M. Pop} } @article {38364, title = {A mammalian promoter model links cis elements to genetic networks}, journal = {Biochemical and Biophysical Research CommunicationsBiochemical and Biophysical Research Communications}, volume = {347}, year = {2006}, type = {16/j.bbrc.2006.06.062}, abstract = {An accurate identification of gene promoters remains an important challenge. Computational approaches for this problem rely on promoter sequence attributes that are believed to be critical for transcription initiation. Here we report a probabilistic model that captures two important properties of promoters, not used by previous methods, viz., the location preference and co-occurrence of promoter elements. Additionally, we found that many of the position-specific DNA elements are strongly linked with the function of the gene product. For instance, a highly conserved motif CCTTT at -1 position is strongly associated with protein synthesis, cellular and tissue development. Our comparative analysis of promoter classes reveals that the promoters devoid of CpG islands are more conserved and have fewer alternative transcription start sites. The discovered links between promoter elements and gene function allows us to infer genetic networks from promoter elements. The web server for the PSPA promoter predictor is available at http://cagr.pcbi.upenn.edu/PSPA.}, keywords = {conservation, Core promoter prediction, CpG island, Genetic networks, Position-specific motif, Propensity, Transcription factor binding site (TFBS)}, isbn = {0006-291X}, author = {Wang, Junwen and Sridhar Hannenhalli} } @article {49560, title = {MCMC data association and sparse factorization updating for real time multitarget tracking with merged and multiple measurements.}, volume = {28}, year = {2006}, month = {2006 Dec}, pages = {1960-72}, abstract = {

In several multitarget tracking applications, a target may return more than one measurement per target and interacting targets may return multiple merged measurements between targets. Existing algorithms for tracking and data association, initially applied to radar tracking, do not adequately address these types of measurements. Here, we introduce a probabilistic model for interacting targets that addresses both types of measurements simultaneously. We provide an algorithm for approximate inference in this model using a Markov chain Monte Carlo (MCMC)-based auxiliary variable particle filter. We Rao-Blackwellize the Markov chain to eliminate sampling over the continuous state space of the targets. A major contribution of this work is the use of sparse least squares updating and downdating techniques, which significantly reduce the computational cost per iteration of the Markov chain. Also, when combined with a simple heuristic, they enable the algorithm to correctly focus computation on interacting targets. We include experimental results on a challenging simulation sequence. We test the accuracy of the algorithm using two sensor modalities, video, and laser range data. We also show the algorithm exhibits real time performance on a conventional PC.

}, keywords = {algorithms, Artificial Intelligence, Image Enhancement, Image Interpretation, Computer-Assisted, Information Storage and Retrieval, Movement, Pattern Recognition, Automated, Reproducibility of Results, Sensitivity and Specificity, Subtraction Technique}, issn = {0162-8828}, doi = {10.1109/TPAMI.2006.247}, author = {Khan, Zia and Balch, Tucker and Dellaert, Frank} } @article {49750, title = {MCMC Data Association and Sparse Factorization Updating for Real Time Multitarget Tracking with Merged and Multiple Measurements}, journal = { IEEE Transactions on Pattern Analysis and Machine Intelligence}, volume = {28}, year = {2006}, month = {12/2006}, pages = {1960-1972}, author = {Zia Khan and Tucker Balch and Frank Dellaert} } @article {38371, title = {Metagenomic Analysis of the Human Distal Gut Microbiome}, journal = {ScienceScienceScienceScience}, volume = {312}, year = {2006}, type = {10.1126/science.1124234}, abstract = {The human intestinal microbiota is composed of 1013 to 1014 microorganisms whose collective genome ({\textquotedblleft}microbiome{\textquotedblright}) contains at least 100 times as many genes as our own genome. We analyzed \~{}78 million base pairs of unique DNA sequence and 2062 polymerase chain reaction{\textendash}amplified 16S ribosomal DNA sequences obtained from the fecal DNAs of two healthy adults. Using metabolic function analyses of identified genes, we compared our human genome with the average content of previously sequenced microbial genomes. Our microbiome has significantly enriched metabolism of glycans, amino acids, and xenobiotics; methanogenesis; and 2-methyl-d-erythritol 4-phosphate pathway{\textendash}mediated biosynthesis of vitamins and isoprenoids. Thus, humans are superorganisms whose metabolism represents an amalgamation of microbial and human attributes.}, isbn = {0036-8075, 1095-9203}, author = {Gill, Steven R. and M. Pop and DeBoy, Robert T. and Eckburg, Paul B. and Turnbaugh, Peter J. and Samuel, Buck S. and Gordon, Jeffrey I. and Relman, David A. and Fraser-Liggett, Claire M. and Nelson, Karen E.} } @article {49847, title = {M-GCAT: interactively and efficiently constructing large-scale multiple genome comparison frameworks in closely related species}, journal = {BMC bioinformatics}, volume = {7}, year = {2006}, pages = {433}, author = {Todd Treangen and Messeguer, Xavier} } @proceedings {38378, title = {Microbial diversity in the era of genomics}, volume = {66}, year = {2006}, month = {2006}, author = {Rita R. Colwell} } @article {38387, title = {Molecular Characterization of Serine-, Alanine-, and Proline-Rich Proteins of Trypanosoma cruzi and Their Possible Role in Host Cell Infection}, journal = {Infect. Immun.Infect. Immun.}, volume = {74}, year = {2006}, type = {

10.1128/IAI.74.3.1537-1546.2006

}, abstract = {We previously reported the isolation of a novel protein gene family, termed SAP (serine-, alanine-, and proline-rich protein), from Trypanosoma cruzi. Aided by the availability of the completed genome sequence of T. cruzi, we have now identified 39 full-length sequences of SAP, six pseudogenes and four partial genes. SAPs share a central domain of about 55 amino acids and can be divided into four groups based on their amino (N)- and carboxy (C)-terminal sequences. Some SAPs have conserved N- and C-terminal domains encoding a signal peptide and a glycosylphosphatidylinositol anchor addition site, respectively. Analysis of the expression of SAPs in metacyclic trypomastigotes by two-dimensional electrophoresis and immunoblotting revealed that they are likely to be posttranslationally modified in vivo. We have also demonstrated that some SAPs are shed into the extracellular medium. The recombinant SAP exhibited an adhesive capacity toward mammalian cells, where binding was dose dependent and saturable, indicating a possible ligand-receptor interaction. SAP triggered the host cell Ca2+ response required for parasite internalization. A cell invasion assay performed in the presence of SAP showed inhibition of internalization of the metacyclic forms of the CL strain. Taken together, these results show that SAP is involved in the invasion of mammalian cells by metacyclic trypomastigotes, and they confirm the hypothesis that infective trypomastigotes exploit an arsenal of surface glycoproteins and shed proteins to induce signaling events required for their internalization.}, author = {Baida, Renata C. P. and Santos, Marcia R. M. and Carmo, Mirian S. and Yoshida, Nobuko and Ferreira, Danielle and Ferreira, Alice Teixeira and El Sayed, Najib M. and Andersson, Bj{\"o}rn and da Silveira, Jose Franco} } @conference {49564, title = {Multitarget Tracking with Split and Merged Measurements}, booktitle = {2005 IEEE Computer Society Conference on Computer Vision and Pattern Recognition (CVPR{\textquoteright}05)2005 IEEE Computer Society Conference on Computer Vision and Pattern Recognition (CVPR{\textquoteright}05)}, year = {2006}, publisher = {IEEE}, organization = {IEEE}, address = {San Diego, CA, USA}, doi = {10.1109/CVPR.2005.245}, url = {http://ieeexplore.ieee.org/lpdocs/epic03/wrapper.htm?arnumber=1467323}, author = {Khan, Z. and Balch, T. and Dellaert, F.} } @article {38363, title = {Magic bullets and golden rules: data sampling in molecular phylogenetics}, journal = {Zoology (Jena)Zoology (Jena)}, volume = {108}, year = {2005}, type = {10.1016/j.zool.2005.09.006}, abstract = {Data collection for molecular phylogenetic studies is based on samples of both genes and taxa. In an ideal world, with no limitations to resources, as many genes could be sampled as deemed necessary to address phylogenetic problems. Given limited resources in the real world, inadequate (in terms of choice of genes or number of genes) sequences or restricted taxon sampling can adversely affect the reliability or information gained in phylogenetics. Recent empirical and simulation-based studies of data sampling in molecular phylogenetics have reached differing conclusions on how to deal with these problems. Some advocated sampling more genes, others more taxa. There is certainly no {\textquoteright}magic bullet{\textquoteright} that will fit all phylogenetic problems, and no specific {\textquoteright}golden rules{\textquoteright} have been deduced, other than that single genes may not always contain sufficient phylogenetic information. However, several general conclusions and suggestions can be made. One suggestion is that the determination of a multiple, but moderate number (e.g., 6-10) of gene sequences might take precedence over sequencing a larger set of genes and thereby permit the sampling of more taxa for a phylogenetic study.}, author = {Michael P. Cummings and Meyer, A.} } @article {49752, title = {MCMC-Based Particle Filtering for Tracking a Variable Number of Interacting Targets}, volume = {27}, year = {2005}, pages = {1805-1918}, author = {Zia Khan and Tucker Balch and Frank Dellaert} } @article {49562, title = {MCMC-based particle filtering for tracking a variable number of interacting targets.}, volume = {27}, year = {2005}, month = {2005 Nov}, pages = {1805-19}, abstract = {

We describe a particle filter that effectively deals with interacting targets--targets that are influenced by the proximity and/or behavior of other targets. The particle filter includes a Markov random field (MRF) motion prior that helps maintain the identity of targets throughout an interaction, significantly reducing tracker failures. We show that this MRF prior can be easily implemented by including an additional interaction factor in the importance weights of the particle filter. However, the computational requirements of the resulting multitarget filter render it unusable for large numbers of targets. Consequently, we replace the traditional importance sampling step in the particle filter with a novel Markov chain Monte Carlo (MCMC) sampling step to obtain a more efficient MCMC-based multitarget filter. We also show how to extend this MCMC-based filter to address a variable number of interacting targets. Finally, we present both qualitative and quantitative experimental results, demonstrating that the resulting particle filters deal efficiently and effectively with complicated target interactions.

}, keywords = {algorithms, Animals, Artificial Intelligence, Computer simulation, HUMANS, Image Enhancement, Image Interpretation, Computer-Assisted, Information Storage and Retrieval, Markov chains, Models, Biological, Models, Statistical, Monte Carlo Method, Motion, Movement, Pattern Recognition, Automated, Subtraction Technique, Video Recording}, issn = {0162-8828}, doi = {10.1109/TPAMI.2005.223}, author = {Khan, Zia and Balch, Tucker and Dellaert, Frank} } @article {38376, title = {Method of DNA extraction and application of multiplex polymerase chain reaction to detect toxigenic Vibrio cholerae O1 and O139 from aquatic ecosystems}, journal = {Environmental MicrobiologyEnvironmental Microbiology}, volume = {5}, year = {2003}, type = {10.1046/j.1462-2920.2003.00443.x}, abstract = {Vibrio cholerae is a free-living bacterium found in water and in association with plankton. V. cholerae non-O1/non-O139 strains are frequently isolated from aquatic ecosystems worldwide. Less frequently isolated are V. cholerae O1 and V. cholerae O139, the aetiological agents of cholera. These strains have two main virulence-associated factors, cholera toxin (CT) and toxin co-regulated pilus (TCP). By extracting total DNA from aquatic samples, the presence of pathogenic strains can be determined quickly and used to improve a microbiological risk assessment for cholera in coastal areas. Some methods suggested for DNA extraction from water samples are not applicable to all water types. We describe here a method for DNA extraction from coastal water and a multiplex polymerase chain reaction (PCR) for O1 and O139 serogroups. DNA extraction was successfully accomplished from 117 sea water samples collected from coastal areas of Per{\'u}, Brazil and the USA. DNA concentration in all samples varied from 20~ng to 480~{\textmu}g~{\textmu}l-1. The sensitivity of the DNA extraction method was 100 V. cholerae cells in 250~ml of water. The specificity of multiplex O1/O139 PCR was investigated by analysing 120 strains of V. cholerae, Vibrio and other Bacteria species. All V. cholerae O1 and O139 tested were positive. For cholera surveillance of aquatic environments and ballast water, total DNA extraction, followed by V. cholerae PCR, and O1/O139 serogroup and tcpA/ctxA genes by multiplex PCR offers an efficient system, permitting risk analysis for cholera in coastal areas.}, isbn = {1462-2920}, author = {Rivera, Irma N. G. and Lipp, Erin K. and Gil, Ana and Choopun, Nipa and Huq, Anwar and Rita R. Colwell} } @article {38368, title = {MDP-1 is a new and distinct member of the haloacid dehalogenase family of aspartate-dependent phosphohydrolases}, journal = {BiochemistryBiochemistry}, volume = {40}, year = {2001}, note = {http://www.ncbi.nlm.nih.gov/pubmed/11601995?dopt=Abstract}, abstract = {MDP-1 is a eukaryotic magnesium-dependent acid phosphatase with little sequence homology to previously characterized phosphatases. The presence of a conserved motif (Asp-X-Asp-X-Thr) in the N terminus of MDP-1 suggested a relationship to the haloacid dehalogenase (HAD) superfamily, which contains a number of magnesium-dependent acid phosphatases. These phosphatases utilize an aspartate nucleophile and contain a number of conserved active-site residues and hydrophobic patches, which can be plausibly aligned with conserved residues in MDP-1. Seven site-specific point mutants of MDP-1 were produced by modifying the catalytic aspartate, serine, and lysine residues to asparagine or glutamate, alanine, and arginine, respectively. The activity of these mutants confirms the assignment of MDP-1 as a member of the HAD superfamily. Detailed comparison of the sequence of the 15 MDP-1 sequences from various organisms with other HAD superfamily sequences suggests that MDP-1 is not closely related to any particular member of the superfamily. The crystal structures of several HAD family enzymes identify a domain proximal to the active site responsible for important interactions with low molecular weight substrates. The absence of this domain or any other that might perform the same function in MDP-1 suggests an "open" active site capable of interactions with large substrates such as proteins. This suggestion was experimentally confirmed by demonstration that MDP-1 is competent to catalyze the dephosphorylation of tyrosine-phosphorylated proteins.}, keywords = {Amino Acid Motifs, Amino Acid Sequence, Animals, Aspartic Acid, Catalytic Domain, HUMANS, Hydrolases, Mice, Molecular Sequence Data, Multigene Family, Mutagenesis, Site-Directed, Phosphoprotein Phosphatases, Protein Structure, Tertiary, Protein Tyrosine Phosphatases, Rats, Saccharomyces cerevisiae, sequence alignment, Sequence Homology, Amino Acid}, author = {J. Selengut} } @article {38369, title = {MDP-1: A novel eukaryotic magnesium-dependent phosphatase}, journal = {BiochemistryBiochemistry}, volume = {39}, year = {2000}, note = {http://www.ncbi.nlm.nih.gov/pubmed/10889041?dopt=Abstract}, abstract = {We report here the purification, cloning, expression, and characterization of a novel phosphatase, MDP-1. In the course of investigating the reported acid phosphatase activity of carbonic anhydrase III preparations, several discrete phosphatases were discerned. One of these, a magnesium-dependent species of 18.6 kDa, was purified to homogeneity and yielded several peptide sequences from which the parent gene was identified by database searching. Although orthologous genes were identified in fungi and plants as well as mammalian species, there was no apparent homology to any known family of phosphatases. The enzyme was expressed in Escherichia coli with a fusion tag and purified by affinity methods. The recombinant enzyme showed magnesium-dependent acid phosphatase activity comparable to the originally isolated rabbit protein. The enzyme catalyzes the rapid hydrolysis of p-nitrophenyl phosphate, ribose-5-phosphate, and phosphotyrosine. The selectivity for phosphotyrosine over phosphoserine or phosphothreonine is considerable, but the enzyme did not show activity toward five phosphotyrosine-containing peptides. None of the various substrates assayed (including various nucleotide, sugar, amino acid and peptide phosphates, phosphoinositides, and phosphodiesters) exhibited K(M) values lower than 1 mM, and many showed negligible rates of hydrolysis. The enzyme is inhibited by vanadate and fluoride but not by azide, cyanide, calcium, lithium, or tartaric acid. Chemical labeling, refolding, dialysis, and mutagenesis experiments suggest that the enzymatic mechanism is not dependent on cysteine, histidine, or nonmagnesium metal ions. In recognition of these observations, the enzyme has been given the name magnesium-dependent phosphatase-1 (MDP-1).}, keywords = {Amino Acid Sequence, Animals, Catalysis, Cations, Chromatography, Affinity, Cloning, Molecular, Cysteine, Enzyme Inhibitors, Histidine, Hydrogen-Ion Concentration, Magnesium, Mice, Molecular Sequence Data, Phosphoprotein Phosphatases, Protein Phosphatase 1, Rabbits, Sequence Analysis, Protein, Sequence Homology, Amino Acid, Substrate Specificity}, author = {J. Selengut and Levine, R. L.} } @article {38390, title = {More surprises from Kinetoplastida}, journal = {Proceedings of the National Academy of Sciences of the United States of AmericaProceedings of the National Academy of Sciences of the United States of America}, volume = {96}, year = {1999}, author = {Donelson, J. E. and Gardner, M. J. and Najib M. El-Sayed} } @inbook {49665, title = {Multiple mechanisms of immune evasion by African trypanosomes}, booktitle = {The Trypanosome Surface }, year = {1999}, pages = {71-91}, publisher = {De Boeck \& Larcier s.a.}, organization = {De Boeck \& Larcier s.a.}, address = {Brussels}, author = {Donelson, J.E. and Hill, K.L. and El-Sayed, N.M.A.} } @article {38392, title = {Multiple mechanisms of immune evasion by African trypanosomes}, journal = {Molecular and Biochemical ParasitologyMolecular and Biochemical Parasitology}, volume = {91}, year = {1998}, type = {16/S0166-6851(97)00209-0}, abstract = {During infection of a mammalian host, African trypanosomes are in constant contact with the host{\textquoteright}s immune system. These protozoan parasites are infamous for their ability to evade the immune responses by periodically switching their major variant surface glycoprotein (VSG), a phenomenon called antigenic variation. Antigenic variation, however, is likely to be only one of several mechanisms enabling these organisms to thrive in the face of the immune defenses. The ability to grow in high levels of interferon-gamma (IFN-[gamma]) and to avoid complement-mediated destruction may also facilitate the parasite{\textquoteright}s survival. In this review we summarize (i) the activation of trypanosome genes for three different VSGs during antigenic variation, (ii) the secretion of a trypanosome protein that induces host CD8+ T cells to produce IFN-[gamma], and (iii) the evidence for trypansome protein similar to a surface protease of Leishmania that plays a role in resistance to complement-mediated lysis.}, keywords = {Leishmania, Recombinant cloning, T cell, Trypanosomes, VSG genes}, isbn = {0166-6851}, author = {Donelson, John E. and Hill, Kent L. and Najib M. El-Sayed} } @article {49647, title = {Management of an enlarging aortic aneurysm in the presence of radiation induced retroperitoneal fibrosis.}, journal = {J Cardiovasc Surg (Torino)}, volume = {30}, year = {1989}, month = {1989 Mar-Apr}, pages = {233-5}, abstract = {

Despite a thoracoabdominal retroperitoneal approach to an enlarging symptomatic infrarenal aortic aneurysm, proximal aortic dissection was hazardous due to radiation induced retroperitoneal fibrosis. Iliac artery ligation and thoracic aorta to iliac artery bypass has resulted in successful management during 14 months of follow-up.

}, keywords = {Aged, Aorta, Abdominal, Aortic Aneurysm, Blood Vessel Prosthesis, HUMANS, Lymphoma, Male, Radiation Injuries, Retroperitoneal Fibrosis, Retroperitoneal Neoplasms, T-Lymphocytes}, issn = {0021-9509}, author = {Todd, G J and Schwartz, A and Rapoport, F} }