e , the flanking 5′ and 3′ base did not coincide with a gene pred

e., the flanking 5′ and 3′ base did not coincide with a gene prediction), and (3) they had no overlap with repeat regions. 94 TARs that did not coincide with the predicted gene set were chosen for experimental validation by RT-PCR. 79

of these TARs were detected in a first-pass analysis with a single primer pair, giving a validation rate of 84%. A representative sampling of RT-PCR results is shown in Figure 5. Figure 5 Novel transcripts check details are validated by RT-PCR. RT-PCR products for primer pairs targeting TYR1 (positive control) and 22 novel transcripts detected on the whole genome tiling arrays. A standard DNA ladder flanks each gel. “”RT”" indicates whether reverse transcriptase was added to the cDNA synthesis reaction. To determine

whether the novel loci correspond to conserved sequences in other genomes and, if so, if these homologous loci have been independently annotated as transcribed (i.e., if they are merely unannotated in G217B), we searched for conserved sequences in other dimorphic fungal pathogens Kinase Inhibitor Library chemical structure within the order Onygenales (4 strains of H. capsulatum, 2 strains of Blastomyces dermatitidis, 3 strains of Paracoccidioides brasiliensis, and the reference strain of Coccidioides immitis). A BLASTX search of the isolated novel sequences against the predicted protein sets yielded a number of hits in other genomes (173 of the isolated novel sequences had hits in at least one non-G217B H. capsulatum gene set, and 63 of these

had hits in at least one non-H. capsulatum gene set). Z-IETD-FMK chemical structure To increase the sensitivity of this search, we performed an INPARANOID-based[12] mapping of syntenic loci that flanked each novel locus (Figure 6). Genes in 20 kb windows on either side of the novel TAR could be independently mapped to orthologs on a common contig in at least 8 other genomes for 217 of old the isolated novel sequences. Of the 173 isolated novel sequences with BLASTX hits, 156 could be mapped to syntenic loci, and, for 150 of these, the BLASTX hit coincided with the mapped locus. A TBLASTX (translated nucleotide vs. translated nucleotide) comparison of the isolated novel sequence to the mapped locus yielded a significant alignment (e ≤ 10-6) for at least 4 H. capsulatum strains in 210 cases, for both B. dermatitidis strains in 80 cases, for at least two P. brasiliensis strains in 31 cases, and for the reference C. immitis strain in 7 cases. In general, the TBLASTX results were consistent with evolutionary distance from G217B (e.g. sequences conserved between H. capsulatum and B. dermatitidis were also conserved among H. capsulatum strains). Figure 6 Syntenic loci were mapped using an INPARANOID-based strategy. As described in the results section, syntenic loci were defined as non-G217B contigs containing INPARANOID-based orthologs (y-axis) of genes within 20 kb of novel TARs (x-axis).

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