In DNA barcoding, the DNA degradation of old museum specimens has been limited full-length (658bp) sequencing. The challenges associated with the retrieval and authentication of degraded DNA extracts from fossil and old museum specimens were principally limited to analyze the relatively short sequences (<300 bp). Furthermore, almost protocols in other to analyzed the degraded DNA contained the cloning process after PCR causing the time-consuming and the rising costs. To overcome these problematic circumstances, we tried a modified method to analyze full-length of DNA barcoding region in 30~60 year-old butterfly specimens (225 samples in 28 species), using direct sequencing after PCR with species-specific overlapping primer sets per each species. As a result, all of 28 species have been successfully analyzed, although 178 samples (79%) are completely generated barcoding sequences ranged from 640 to 658 bp and 47 samples (21%) are partially sequenced ranged from 100 to 500 bp. Thus, the result showed that the direct PCR sequencing using the overlapping primer sets per species appears to have great potential efficiency for analysis of degraded DNA without incorrect sequences.

• Taeman Han(Department of Agricultural Biology, National Academy of Agricultural Science)
• Tae Hwa Kang(Department of Agricultural Biology, National Academy of Agricultural Science)
• Oh Chang Kwon(Department of Agricultural Biology, National Academy of Agricultural Science)
• Young Bo Lee(Department of Agricultural Biology, National Academy of Agricultural Science)
• Mi Ae Kim(Department of Agricultural Biology, National Academy of Agricultural Science)
• Hae Chul Park(Department of Agricultural Biology, National Academy of Agricultural Science)