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Fragment assembly with short reads

by: Mark Chaisson, Pavel Pevzner, Haixu Tang
Bioinformatics In Bioinformatics, Vol. 20, No. 13. (1 September 2004), pp. 2067-2074, doi:10.1093/bioinformatics/bth205  Key: citeulike:384489

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Abstract

Motivation: Current DNA sequencing technology produces reads of about 500–750 bp, with typical coverage under 10×. New sequencing technologies are emerging that produce shorter reads (length 80–200 bp) but allow one to generate significantly higher coverage (30× and higher) at low cost. Modern assembly programs and error correction routines have been tuned to work well with current read technology but were not designed for assembly of short reads.Results: We analyze the limitations of assembling reads generated by these new technologies and present a routine for base-calling in reads prior to their assembly. We demonstrate that while it is feasible to assemble such short reads, the resulting contigs will require significant (if not prohibitive) finishing efforts.Availability: Available from the web at http://www.cse.ucsd.edu/groups/bioinformatics/software.html


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