首页> 外文OA文献 >Dual role of the PhoP approximately P response regulator: Bacillus amyloliquefaciens FZB45 phytase gene transcription is directed by positive and negative interactions with the phyC promoter.
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Dual role of the PhoP approximately P response regulator: Bacillus amyloliquefaciens FZB45 phytase gene transcription is directed by positive and negative interactions with the phyC promoter.

机译:PhoP大约P响应调节剂的双重作用:解淀粉芽孢杆菌FZB45植酸酶基因转录是通过与phyC启动子的正向和负向相互作用进行的。

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摘要

Several Bacillus strains secrete phytase, an enzyme catalyzing dephosphorylation of myo-inositol hexakisphosphate (phytate). We identified the phyC (phytase) gene from environmental Bacillus amyloliquefaciens FZB45 as a member of the phosphate starvation-inducible PhoPR regulon. In vivo and in vitro assays revealed that PhoP approximately P is essential for phyC transcription. The transcriptional start site was identified downstream of a sigmaA-like promoter region located 27 bp upstream of the probable translation ATG start codon. Inspection of the phyC promoter sequence revealed an unusual structure. The -35 and -10 regions are separated by a window of 21 bp. A pair of tandemly repeated PhoP TT(T/A/C)ACA binding boxes was located within and upstream of the -35 consensus promoter region. A single PhoP box was found within the -10 consensus promoter region. DNase I footprinting experiments performed with isolated PhoP confirmed that PhoP approximately P binds at two sites overlapping with the phyC -35 and -10 consensus promoter region. While binding of dimeric PhoP approximately P at -35 is essential for activation of the phyC promoter, binding of PhoP approximately P at -10 suppresses promoter activity. A sixfold enhancement of phyC gene expression was registered after T:G substitution of nucleotide -13 (mutant MUT13), which eliminates PhoP binding at the single PhoP box without impairing the -10 consensus sequence. Moreover, MUT13 also expressed phyC during phosphate-replete growth, suggesting that the repressing effect due to binding of PhoP approximately P at -10 was abolished. A model is presented in which transcription initiation of phyC is positively and negatively affected by the actual concentration of the PhoP approximately P response regulator.
机译:几种芽孢杆菌属菌株分泌肌醇六磷酸酶,一种催化肌醇六磷酸(肌醇六磷酸)去磷酸化的酶。我们从环境中的解淀粉芽孢杆菌FZB45中鉴定了phyC(植酸酶)基因为磷酸饥饿诱导型PhoPR调节剂的成员。体内和体外测定表明,PhoP大约为phyC转录所必需。在可能的翻译ATG起始密码子上游27bp处的sigmaA样启动子区域的下游鉴定了转录起始位点。 phyC启动子序列的检查揭示了一个异常的结构。 -35和-10区域之间的间隔为21 bp。一对串联重复的PhoP TT(T / A / C)ACA结合盒位于-35共有启动子区域内和上游。在-10个共有启动子区域内发现了一个PhoP框。用分离的PhoP进行的DNase I足迹实验证实,PhoP大约P在与phyC -35和-10共有启动子区域重叠的两个位点结合。虽然在-35处约P的二聚体PhoP结合对于phyC启动子的激活是必不可少的,但在-10处约P的PhoP结合则抑制了启动子活性。在核苷酸-13的T:G取代后(突变MUT13),phyC基因表达增强了6倍,这消除了单个PhoP盒中的PhoP结合,而不会损害-10共有序列。此外,MUT13在磷酸盐充分生长期间也表达了phyC,这表明由于PhoP在-10附近结合P所引起的阻抑作用被消除。提出了一个模型,其中phyC的转录起始受到PhoP近似P反应调节剂实际浓度的正负影响。

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