Improving read lengths by recomputing the matrices of Model 377 DNA Sequencers.

Correcting data shifts in gel files created by Model 377 DNA Sequencers.

Aligning Flowgrams to DNA Sequences

A read from 454 or Ion Torrent sequencers is natively represented as a flowgram, which is a sequence of pairs of a nucleotide and its (fractional) intensity. Recent work has focused on improving the accuracy of base calling (conversion of flowgrams to DNA sequences) in order to facilitate read mapping and downstream analysis of sequence variants. However, base calling always incurs a loss of in...

Acceleration of short and long DNA read mapping without loss of accuracy using suffix array

UNLABELLED HPG Aligner applies suffix arrays for DNA read mapping. This implementation produces a highly sensitive and extremely fast mapping of DNA reads that scales up almost linearly with read length. The approach presented here is faster (over 20× for long reads) and more sensitive (over 98% in a wide range of read lengths) than the current state-of-the-art mappers. HPG Aligner is not only ...

Rescuing corrupted gel files from Model 377 and 373 DNA Sequencers.

Automated DNA sequencing requires the intensive use of computers to handle the large amount of data taken. When a computer failure occurs and the data are no longer accessible, all the expense and effort that went into the sequencing experiment is lost. By using the data storage architecture of Macintosh computers to our advantage, we may prevent this loss in the case of automatic sequencers fr...

High-quality automated DNA sequencing primed with hexamer strings.

The finishing phase of genome sequencing projects is expensive, in part, because of the cost of de novo synthesis of custom primers and the management burden associated with obtaining and using them for primer walking. One approach to reduce these high costs is the use of a presynthesized library of short oligonucleotides (8-10 bases) rather than long primers. The use of such a library eliminat...