Fragment -125/-112 bears putative NIT2 and
CdxA binding sites, whereas oligonucleotide from -243 to -229 could be involved in binding to a so far unknown protein. NIT2 modulates transcription of genes that encode enzymes involved in the catabolism of nitrogen sources during starvation [27]. selleck chemicals We have recently studied PbGP43 NIT2-binding sites and shown transcription modulation of the PbGP43 with find more primary nitrogen sources; however the participation of a NIT2 transcription factor binding to the putative motifs at -179, -117 and -73 was unlikely [22]. The core sequence of CdxA-binding element is A/TA/TTA/TA/CTA/G [28], thus allowing for several sequence possibilities. That probably explains why CdxA is one of the most frequently found promoter elements in human genes [29]. Transcription factor CdxA buy Roscovitine is a homeodomain protein originally described in the early stages of morphogenesis of chicken intestinal tract [30], but its role on regulation of fungal genes has apparently not been addressed. The P. brasiliensis genome does not show any protein with high identities with CdxA, although other homeobox proteins have been annotated. On the other hand, there is a slight similarity of P. brasiliensis proteins with Sox-5, whose DNA-binding motif is seen in non-overlapping fragments of the probes covering sequence form -134 and -103. To date, we have not been able to purify
and identify the DNA-binding proteins detected here. The probes tested are located close to PbGP43 transcription start sites and we understand from our previous work that the first -480 bp were sufficient to promote basal levels of gene transcription and also modulation with ammonium sulfate [22]. This fragment contains most of 1a region. When we blasted the overlap -125/-112 (14-mer) and -243/-229 (13-mer) oligonucleotides from EMSA-positive fragments with P. brasiliensis upstream intergenic regions http://www.broad.mit.edu/annotation/genome/paracoccidioides_brasiliensis/MultiHome.html,
exact matches IMP dehydrogenase were found generally at the 11-mer level in about 20 to 30 genes. Sequence CTGTTGATCTTTT has been found in P. brasiliensis homologous genes encoding beta-hexosaminidase and chitin synthase, but mostly in genes encoding predicted or hypothetical proteins. Concerning the mutated -125/-112 region, we detected identical fragments in the upstream region of one gene encoding beta-glucosidase. Therefore, although gp43 is a non-functional β-1,3-exoglucanase, its gene may have conserved transcription motifs characteristic of those related to carbohydrate metabolism, possibly within the binding sequences identified here. We presently showed negative modulation with glucose of PbGP43 from Pb3, Pb18 and Pb339 at similar rates, but the participation of the binding DNA sequences revealed here in this or other modulations is presently unknown and will have to be addressed using gene reporter experiments.