Identification and Analysis of Error Types in High-Throughput Genotyping
Kelly R. Ewen,Melanie Bahlo,Melanie Bahlo,Susan A. Treloar,Susan A. Treloar,Douglas F. Levinson,Bryan J. Mowry,John W. Barlow,Simon J. Foote,Simon J. Foote,Simon J. Foote +10 more
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TL;DR: The data suggest that Mendelian-inheritance-error checking is a worthwhile strategy for both types of genotyping data, whereas fine-mapping studies benefit more from concordance checking than do studies using commercial marker data.
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Abstract: Although it is clear that errors in genotyping data can lead to severe errors in linkage analysis, there is as yet no consensus strategy for identification of genotyping errors. Strategies include comparison of duplicate samples, independent calling of alleles, and Mendelian-inheritance-error checking. This study aimed to develop a better understanding of error types associated with microsatellite genotyping, as a first step toward development of a rational error-detection strategy. Two microsatellite marker sets (a commercial genomewide set and a custom-designed fine-resolution mapping set) were used to generate 118,420 and 22,500 initial genotypes and 10,088 and 8,328 duplicates, respectively. Mendelian-inheritance errors were identified by PedManager software, and concordance was determined for the duplicate samples. Concordance checking identifies only human errors, whereas Mendelian-inheritance-error checking is capable of detection of additional errors, such as mutations and null alleles. Neither strategy is able to detect all errors. Inheritance checking of the commercial marker data identified that the results contained 0.13% human errors and 0.12% other errors (0.25% total error), whereas concordance checking found 0.16% human errors. Similarly, Mendelian-inheritance-error checking of the custom-set data identified 1.37% errors, compared with 2.38% human errors identified by concordance checking. A greater variety of error types were detected by Mendelian-inheritance-error checking than by duplication of samples or by independent reanalysis of gels. These data suggest that Mendelian-inheritance-error checking is a worthwhile strategy for both types of genotyping data, whereas fine-mapping studies benefit more from concordance checking than do studies using commercial marker data. Maximization of error identification increases the likelihood of linkage when complex diseases are analyzed.
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Citations
Determining microsatellite genotyping reliability and mutation detection ability: an approach using small-pool PCR from sperm DNA.
TL;DR: Large multi-step mutations were observed, providing evidence for complex mutation processes at microsatellites and potentially violating key assumptions in the stepwise mutation model, and demonstrating the necessity of actively searching for large mutation events when investigating microsatellite evolution.
15
Estimation of genotyping error rate from repeat genotyping, unintentional recaptures and known parent-offspring comparisons in 16 microsatellite loci for brown rockfish (Sebastes auriculatus).
Maureen A. Hess,James G. Rhydderch,Larry L. LeClair,Raymond M. Buckley,Raymond M. Buckley,Mitsuhiro Kawase,Lorenz Hauser +6 more
TL;DR: The data suggest that repeat genotyping may underestimate true error rates and may not estimate locus‐specific error rates accurately, and is suggested to use methods for error estimation that correspond to the overall aim of the study.
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•Dissertation
Genetics of the scandinavian brown bear (Ursus arctos) : implications for biology and conservation
Eva Bellemain
- 01 Jan 2004
TL;DR: The software PARENTE was developed, to conduct parentage inference using molecular data from diploid codominant markers, and significantly improved microsatellite amplification and decreased error rates for fecal DNA in limiting conditions, to amplify DNA from noninvasive samples of brown bears.
Detection of multidrug-resistant Mycobacterium tuberculosis strains isolated in Brazil using a multimarker genetic assay for katG and rpoB genes
Luita Nice Café Oliveira,Jairo da Silva Muniz-Sobrinho,Luiz Alexandre Viana-Magno,Sônia Cristina Oliveira Melo,Antonio Macho,Fabrício Rios-Santos +5 more
TL;DR: Instead of using diagnostic kits detecting several mutations, a simple dual-marker panel is proposed to detect multidrug-resistant tuberculosis, with 86% sensitivity and 100% specificity, which would considerably decrease the processing costs while retaining diagnostic accuracy.
Development and characterization of novel tetranucleotide microsatellite markers in the noble crayfish (Astacus astacus) suitable for highly multiplexing and for detecting hybrids between the noble crayfish and narrow-clawed crayfish (A. leptodactylus)
TL;DR: The novel 19-plex microsatellite assay can be applied for genetic management of captive stocks of the noble crayfish and in studies requiring high genetic resolution, such as parentage assessment, relatedness analysis or strain identification.
14
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