| Literature DB >> 29654355 |
Kana Ishikawa1, Emi Kunitake1,2, Tomomi Kawase1, Motoki Atsumi1, Yuji Noguchi1, Shuhei Ishikawa1, Masahiro Ogawa3, Yasuji Koyama3, Makoto Kimura1, Kyoko Kanamaru1, Masashi Kato1,4, Tetsuo Kobayashi5.
Abstract
The paralogous transcription factors AraR and XlnR in Aspergillus regulate genes that are involved in degradation of cellulose and hemicellulose and catabolism of pentose. AraR and XlnR target the same genes for pentose catabolism but target different genes encoding enzymes for polysaccharide degradation. To uncover the relationship between these paralogous transcription factors, we examined their contribution to regulation of the PCP genes and compared their preferred recognition sequences. Both AraR and XlnR are involved in induction of all the pentose catabolic genes in A. oryzae except larA encoding L-arabinose reductase, which was regulated by AraR but not by XlnR. DNA-binding studies revealed that the recognition sequences of AraR and XlnR also differ only slightly; AraR prefers CGGDTAAW, while XlnR prefers CGGNTAAW. All the pentose catabolic genes possess at least one recognition site to which both AraR and XlnR can bind. Cooperative binding by the factors was not observed. Instead, they competed to bind to the shared sites. XlnR bound to the recognition sites mentioned above as a monomer, but bound to the sequence TTAGSCTAA on the xylanase promoters as a dimer. Consequently, AraR and XlnR have significantly similar, but not the same, DNA-binding properties. Such a slight difference in these paralogous transcription factors may lead to complex outputs in enzyme production depending on the concentrations of coexisting inducer molecules in the natural environment.Entities:
Keywords: AraR; Aspergillus oryzae; Pentose catabolism; XlnR
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Year: 2018 PMID: 29654355 DOI: 10.1007/s00294-018-0837-5
Source DB: PubMed Journal: Curr Genet ISSN: 0172-8083 Impact factor: 3.886