首页> 美国卫生研究院文献>Journal of Bacteriology >Comparison In Vitro of a High- and a Low-Abundance Chemoreceptor of Escherichia coli: Similar Kinase Activation but Different Methyl-Accepting Activities
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Comparison In Vitro of a High- and a Low-Abundance Chemoreceptor of Escherichia coli: Similar Kinase Activation but Different Methyl-Accepting Activities

机译:大肠杆菌的高和低丰度化学感受器的体外比较:类似的激酶激活但不同的甲基接受活性。

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摘要

In Escherichia coli, high-abundance chemoreceptors are present in cellular amounts approximately 10-fold greater than low-abundance chemoreceptors. Cells containing only low-abundance receptors exhibit abnormally low tumble frequencies and do not migrate effectively in spatial gradients. These defects reflect an inherent activity difference between the two receptor classes. We used in vitro assays to investigate this difference. The low-abundance receptor Trg mediated an ∼100-fold activation of the kinase CheA, only twofold less than activation by the high-abundance receptor Tar. In contrast, Trg was less than 1/20 as active as Tar for in vitro methylation. As observed for high-abundance receptors, kinase activation by Trg varied with the extend of modification at methyl-accepting sites; low methylation corresponded to low kinase activation. Thus, in Trg-only cells, low receptor methylation would result in low kinase activation, correspondingly low content of phospho-CheY, and a decreased dynamic range over which attractant binding could modulate kinase activity. These features could account for the low tumble frequency and inefficient taxis exhibited by Trg-only cells. Thus, the crucial functional difference between the receptor classes is likely to be methyl-accepting activity. We investigated the structural basis for this functional difference by introducing onto the carboxy terminus of Trg a CheR-binding pentapeptide, usually found only at the carboxy termini of high-abundance receptors. This addition enhanced the in vitro methyl-accepting activity of Trg 10-fold.
机译:在大肠杆菌中,高丰度化学感受器的细胞数量约为低丰度化学感受器的10倍。仅包含低丰度受体的细胞表现出异常低的滚转频率,并且不能在空间梯度中有效迁移。这些缺陷反映了两种受体类别之间固有的活性差异。我们使用体外测定法研究了这种差异。低丰度受体Trg介导了CheA激酶的约100倍激活,仅比高丰度受体Tar的激活少两倍。相反,对于体外甲基化,Trg的活性不如Tar少1/20。正如对高丰度受体所观察到的,Trg激活的激酶随甲基接受位点修饰的扩展而变化。低甲基化对应于低激酶活化。因此,在仅Trg的细胞中,低受体甲基化将导致低激酶活化,相应地降低低磷CheY含量,以及降低的动态范围,在该动态范围上引诱剂结合可调节激酶活性。这些特征可以解释纯Trg电池所表现出的低滚转频率和低效率的滑行。因此,受体类别之间的关键功能差异可能是甲基接受活性。我们通过在Trg的羧基末端引入CheR结合五肽(通常仅在高丰度受体的羧基末端发现)来研究这种功能差异的结构基础。该添加将Trg的体外甲基接受活性提高了10倍。

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