| Literature DB >> 22567329 |
Abstract
Yersinia enterocolitica is an important zoonotic pathogen that can cause yersiniosis in humans and animals. Food has been suggested to be the main source of yersiniosis. It is critical for the researchers to be able to detect Yersinia or any other foodborne pathogen with increased sensitivity and specificity, as well as in real-time, in the case of a foodborne disease outbreak. Conventional detection methods are known to be labor intensive, time consuming, or expensive. On the other hand, more sensitive molecular-based detection methods like next generation sequencing, microarray, and many others are capable of providing faster results. DNA testing is now possible on a single molecule, and high-throughput analysis allows multiple detection reactions to be performed at once, thus allowing a range of characteristics to be rapidly and simultaneously determined. Despite better detection efficiencies, results derived using molecular biology methods can be affected by the various food matrixes. With the improvements in sample preparation, data analysis, and testing procedures, molecular detection techniques will likely continue to simplify and increase the speed of detection while simultaneously improving the sensitivity and specificity for tracking pathogens in food matrices.Entities:
Year: 2011 PMID: 22567329 PMCID: PMC3335726 DOI: 10.4061/2011/310135
Source DB: PubMed Journal: J Pathog ISSN: 2090-3057
Current software applications for microarray data analysis.
| Software | Application | Provider | Platform | Web link |
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| Array Designer | Primer design for microarray construction | Premier Biosoft International | Windows |
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| ArrayMiner | Analysis tool for microarray gene expression data | Optimal Design | Mac OS |
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| ArrayTrack | Database solution for managing, analyzing, and interpreting microarray gene expression data | National Center for Toxicological Research | Web-based | |
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| ArrayVision | Automated analysis of macro- and microarrays | GE Healthcare | Windows |
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| BAMarray | Detecting differentially expressed genes from microarray data using Bayesian analysis | Case Western Reserve University | Mac OS |
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| BASE | Database solution for the massive amounts of data generated by microarray analysis | Lund University | Web-based |
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| Cluster | Perform a variety of types of cluster analysis and other types of processing on large microarray datasets | University of Tokyo | Mac OS |
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| GenePattern | Gene expression analysis tools | Broad Institute, MIT | Web-based |
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| GeneSifter | Tools for exploring the statistically significant interplay of the data with factors of biological relevance to understand the expression pattern in microarray data. | Geospiza Inc. | Web-based |
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| GenMAPP | Tools for visualizing data from gene expression experiments in the context of biological pathways. | Gladstone Institute, University of California at San Francisco | Windows |
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| GenMaths XT | Analysis of high density microarrays and gene chips | Applied Maths | Windows |
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| Genowiz | A comprehensive multi platform software for microarray data analysis | Ocimum Biosolutions | Mac OS | |
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| Microarray tools | Including: a Comparative Genomic Hybridization (CGH) and expression microarray data analysis, data management and export system | J. Craig Venter Institute | Windows |
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| Partek Genomics Suite | Statistical analysis and data mining tools to facilitate powerful and intuitive exploratory data analysis | Partek Incorporated | Windows |
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| TreeArrange and Treeps | Software for displaying and manipulating hierarchical clustered data | University of Waterloo | Windows |
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| waviCGH | For the analysis and visualization of array-CGH data | Spanish National Cancer Center, Bioinformatics Unit | Web-based |
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Comparison of major next generation DNA sequencing technologies and conventional sequencing.
| Platform | Application | Sequencing chemistry | Read length (bases) | Throughput per run (Gb) | Read per run (million) | Throughput per 24 hr (Gb) | Raw accuracy Range (%) | Cost Pe Mb ($) |
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| ABI 3730 | (1) Complement | Sanger Dideoxy | 800 | 0.00008 | 0.000096 | 0.00064 | 99.0 to 99.999 | 4000 |
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| ABI SOLID 5500 | (1) Whole genome SNP discovery; | Sequencing by ligation | 60 × 2 | 310 | 5167 | 45 | 99.0 to 99.9 | 0.05 |
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| Illumina HiSeq | (1) Whole genome SNP discovery; | Sequencing by synthesis | 100 × 2 | 600 | 6000 | 75 | 96.2 to 99.7 | 0.02 |
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| Life Technologies Ion Torrent | (1) Whole methylome resequencing; | pH meter | 200 | 0.2 | 1 | 2.4 | >99.0 | 0.5 |
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| Roche 454 | (1) | Pyrosequencing | 600 | 0.8 | 1 | 0.5 | 96.0 to 97.0 | 8 |
Software applications for NGS analysis.
| Software | Categories | Sequencing file format compatibility | Created by | Operating platform | Web link |
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| ABySS | Assembly | FASTA | Jared Simpson et al. | Mac OS |
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| Edena | Assembly | FASTQ | David Hernandez | Windows |
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| Exonerate | Alignment | FASTA | Guy Slater and Ewan Birney | Windows |
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| Maq | Alignment | FASTA | Heng Li | Windows |
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| Mosaik | Alignment | FASTA | Michael Stromberg and Gabor Marth | Mac OS |
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| Phrap/ | Alignment | FASTA | Phil Green, Brent Ewing and David Gordon | Mac OS |
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| PyroBayes | Base Caller | SFF | Aaron Quinlan et al. | Linux |
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| SHARCGS | Assembly | Illumina Bustard & Gerald | Juliane Dohm et al. | Linux |
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| SHRiMP | Alignment | FASTA | Michael Brudno and Stephen Rumble | Mac OS |
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| SOAP | Alignment Burrows-Wheeler | Illumina Bustard & Gerald | Ruiqing Li et al. | Unix |
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| SSAHA2 | Alignment Smith-Waterman | FASTA | The Wellcome Trust Sanger Institute | Mac OS |
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| SSAKE | Assembly | FASTA | Rene Warren et al. | Linux |
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| VCAKE | Assembly k-mer extension | FASTA | William Jeck et al. | Mac OS |
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| Velvet | Assembly | FASTA | Daniel Zerbino et al. | Mac OS |
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