Role of CysE in Production of an Extracellular Signaling Molecule in Providencia stuartii and Escherichia coli: Loss of cysE Enhances Biofilm Formation in Escherichia coli

Gwen Sturgill; Christine M. Toutain; John Komperda; George A. OToole; Philip N. Rather

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Role of CysE in Production of an Extracellular Signaling Molecule in Providencia stuartii and Escherichia coli: Loss of cysE Enhances Biofilm Formation in Escherichia coli

机译：CysE在斯图亚特氏菌和大肠杆菌中的细胞外信号分子的生产中的作用：cysE的丧失增强了大肠杆菌中的生物膜形成。

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A mini-Tn5Cm insertion has been identified that significantly reduced the amount of an extracellular activating signal for a lacZ fusion (cma37::lacZ) in Providencia stuartii. The transposon insertion was located immediately upstream of an open reading frame encoding a putative CysE ortholog. The CysE enzyme, serine acetyltransferase, catalyzes the conversion of serine to O-acetyl-l-serine (OAS). This activating signal was also produced by Escherichia coli, and production was abolished in a strain containing a null allele of cysE. Products of the CysE enzyme (OAS, N-acetyl-l-serine [NAS], O-acetyl-l-threonine, and N-acetyl-l-threonine) were individually tested for the ability to activate cma37::lacZ. Only OAS was capable of activating the cma37::lacZ fusion. The ability of OAS to activate the cma37::lacZ fusion was abolished by pretreatment at pH 8.5, which converts OAS to NAS. However, the activity of the native signal in conditioned medium was not decreased by treatment at pH 8.5. In contrast, conditioned medium prepared from cells grown at pH 8.5 exhibited a 4- to 10-fold-higher activity, relative to pH 6.0. Additional genes regulated by the CysE-dependent signal and OAS were identified in P. stuartii and E. coli. The response to the extracellular signal in E. coli was dependent on CysB, a positive activator that requires NAS as a coactivator. In E. coli, a cysE mutant formed biofilms at an accelerated rate compared to the wild type, suggesting a physiological role for this extracellular signal.

机译：已经确定了mini-Tn 5Cm 插入可显着减少 lacZ 融合（ cma37 :: lacZ ）在 Providencia stuartii 中。转座子插入位于编码假定的CysE直向同源物的开放阅读框的紧邻上游。 CysE酶丝氨酸乙酰转移酶催化丝氨酸转化为 O -乙酰基-1-丝氨酸（OAS）。该激活信号也是由大肠杆菌产生的，而在含有cysE空等位基因的菌株中的产生被取消了。 CysE酶的产物（OAS， N -乙酰基-1-丝氨酸[NAS]， O -乙酰基-1-苏氨酸和 N （乙酰基-1-苏氨酸）分别测试了激活 cma37 :: lacZ 的能力。只有OAS能够激活 cma37 :: lacZ 融合体。 pH 8.5预处理可消除OAS激活 cma37 :: lacZ 融合体的能力，将OAS转化为NAS。但是，在pH 8.5处理不会降低条件培养基中天然信号的活性。相反，由在pH 8.5下生长的细胞制备的条件培养基相对于pH 6.0表现出高4至10倍的活性。在 P中鉴定了受CysE依赖性信号和OAS调节的其他基因。 stuartii 和 E。大肠杆菌。对 E中细胞外信号的反应。大肠杆菌依赖于CysB，CysB是一种需要NAS作为共激活因子的阳性激活因子。在 E中。大肠杆菌（一种 EsE 突变体）与野生型相比以更快的速度形成生物膜，表明该细胞外信号具有生理作用。 展开▼

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《Journal of bacteriology》 |2004年第22期|共8页

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Gwen Sturgill; Christine M. Toutain; John Komperda; George A. OToole; Philip N. Rather;
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6. Role of CysE in Production of an Extracellular Signaling Molecule in Providencia stuartii and Escherichia coli: Loss of cysE Enhances Biofilm Formation in Escherichia coli [O] . Gwen Sturgill, Christine M. Toutain, John Komperda, 2004

机译：CysE在斯图亚特氏菌和大肠杆菌中的细胞外信号分子的生产中的作用：cysE的丧失增强了大肠杆菌中的生物膜形成。

7. Role of CysE in Production of an Extracellular Signaling Molecule in Providencia stuartii and Escherichia coli: Loss of cysE Enhances Biofilm Formation in Escherichia coli [O] . Sturgill, Gwen, Toutain, Christine M., Komperda, John, 2004

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Role of CysE in Production of an Extracellular Signaling Molecule in Providencia stuartii and Escherichia coli: Loss of cysE Enhances Biofilm Formation in Escherichia coli

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