454 Antibody Sequencing - Error Characterization and Correction

Overview

Journal BMC Res Notes

Publisher Biomed Central

Specialties Biology
General Medicine

Date 2011 Oct 14

PMID 21992227

Citations 12

Authors

Ponraj Prabakaran

Emily Streaker

Weizao Chen

Dimiter S Dimitrov

Affiliations

Soon will be listed here.

Abstract

Background: 454 sequencing is currently the method of choice for sequencing of antibody repertoires and libraries containing large numbers (106 to 1012) of different molecules with similar frameworks and variable regions which poses significant challenges for identifying sequencing errors. Identification and correction of sequencing errors in such mixtures is especially important for the exploration of complex maturation pathways and identification of putative germline predecessors of highly somatically mutated antibodies. To quantify and correct errors incorporated in 454 antibody sequencing, we sequenced six antibodies at different known concentrations twice over and compared them with the corresponding known sequences as determined by standard Sanger sequencing.

Results: We found that 454 antibody sequencing could lead to approximately 20% incorrect reads due to insertions that were mostly found at shorter homopolymer regions of 2-3 nucleotide length, and less so by insertions, deletions and other variants at random sites. Correction of errors might reduce this population of erroneous reads down to 5-10%. However, there are a certain number of errors accounting for 4-8% of the total reads that could not be corrected unless several repeated sequencing is performed, although this may not be possible for large diverse libraries and repertoires including complete sets of antibodies (antibodyomes).

Conclusions: The experimental test procedure carried out for assessing 454 antibody sequencing errors reveals high (up to 20%) incorrect reads; the errors can be reduced down to 5-10% but not less which suggests the use of caution to avoid false discovery of antibody variants and diversity.

Citing Articles

Bioinformatic Analysis of Natively Paired VH:VL Antibody Repertoires for Antibody Discovery.

Fahad A, Madan B, DeKosky B Methods Mol Biol. 2022; 2552:447-463.

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Combined Influence of B-Cell Receptor Rearrangement and Somatic Hypermutation on B-Cell Class-Switch Fate in Health and in Chronic Lymphocytic Leukemia.

Petrova V, Muir L, McKay P, Vassiliou G, Smith K, Lyons P Front Immunol. 2018; 9:1784.

PMID: 30147686 PMC: 6095981. DOI: 10.3389/fimmu.2018.01784.

The analysis of clonal expansions in normal and autoimmune B cell repertoires.

Hershberg U, Luning Prak E Philos Trans R Soc Lond B Biol Sci. 2015; 370(1676).

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Immunoglobulin class-switched B cells form an active immune axis between CNS and periphery in multiple sclerosis.

Palanichamy A, Apeltsin L, Kuo T, Sirota M, Wang S, Pitts S Sci Transl Med. 2014; 6(248):248ra106.

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Analysis of plant microbe interactions in the era of next generation sequencing technologies.

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