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Appl. Environ. Microbiol., 06 1997, 2338-2346, Vol 63, No. 6
GA Komatsoulis and MS Waterman
A new computational method (chimeric alignment) has been developed to
detect chimeric 16S rRNA artifacts generated during PCR amplification from
mixed bacterial populations. In contrast to other nearest-neighbor methods
(e.g., CHECK_CHIMERA) that define sequence similarity by k- tuple matching,
the chimeric alignment method uses the score from dynamic programming
alignments. Further, the chimeric alignments are displayed to the user to
assist in sequence classification. The distribution of improvement scores
for 500 authentic, nonchimeric sequences and 300 artificial chimeras
(constructed from authentic sequences) was used to study the sensitivity
and accuracy of both chimeric alignment and CHECK_CHIMERA. At a constant
rate of authentic sequence misclassification (5%), chimeric alignment
incorrectly classified 13% of the artificial chimeras versus 14% for
CHECK_CHIMERA. Interestingly, only 1% of nonchimeras and 10% of chimeras
were misclassified by both programs, suggesting that optimum performance is
obtained by using the two methods to assign sequences to three classes:
high-probability nonchimeras, high-probability chimeras, and sequences that
need further study by other means. This study suggests that k- tuple-based
matching methods are more sensitive than alignment-based methods when there
is significant parental sequence similarity, while the opposite becomes
true as the sequences become more distantly related. The software and a
World Wide Web-based server are available at
http://www-hto.usc.edu/software/mglobal CHI.
Copyright © 1997, American Society for Microbiology
A new computational method for detection of chimeric 16S rRNA artifacts generated by PCR amplification from mixed bacterial populations
Department of Mathematics, University of Southern California, Los Angeles 90089-1113, USA. gkoma@hto.usc.edu
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