1a). As expected, the higher the similarity, the higher the signal intensity, which was consistent at every temperature. Signal intensity decreased with increasing hybridization temperature, with a 10-fold decrease in signal intensity observed from 55 to 75 °C for the perfect match group. The different responses to hybridization temperature are highlighted in Fig. 1b. The signal intensity from mismatches was considerably lower than that of perfect matches, and intensity relative to SAHA HDAC research buy the perfect match decreased with the increase in hybridization temperature. For example, the group with 85–90% similarity had 12%, 5%,
and 1% relative signal intensity compared with the perfect match at 65, 70, and 75 °C, respectively. Previously, long oligonucleotide probes (50–70mer) selleck screening library with around 85–90% of sequence similarity to targets were shown to have 10% relative signal intensity to perfect matches (He et al., 2005). Thus, the specificity of random genomic fragment probes is comparable to
long oligonucleotide probes. In addition, based on the data reported by Goris et al. (2007), most genomic fragment sequences between different species seem to share similarity lower than 90%, a finding consistent with this study. Therefore, our results indicate that the specificity of genomic fragment probes is potentially at species level. In this study, long DNA fragments (around 2000 bp) were selected
as probes because of their high sensitivity (Letowski et al., 2004). Long probes also contain more Demeclocycline sequence information, which makes them advantageous for analysis of microorganisms, many of which are unknown, in the environment (Yokoi et al., 2007; Tobino et al., 2011). Because random 2000-bp fragments may cover two adjacent genes partially, they may however hybridize with target DNA containing one of these genes, which will result in nonspecific signal. Here, target DNA was fragmented to 400 bp to, at least in part, address this concern. When using fragmented DNA, regions flanking the sequence that binds to the probe remain in solution and hence do not contribute to the signal. This situation is similar to what has been observed for whole genome probes, which can provide strain-level specificity even though a given probe (that is, genome) contains genes that are conserved among strains (Wu et al., 2004). However, fragmentation cannot prevent the hybridization of multiple fragments from different strains to the same probe, and hybridization signals obtained with DNA from diverse microbial communities should be interpreted with caution. In conclusion, our results show that the degree of specificity achievable by randomly generated genomic fragment probes on DNA arrays legitimizes their use for microbial diagnostics.