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芳香锚定第二跨膜螺旋的残基组成决定了大肠杆菌天冬氨酸/麦芽糖化学感受器 Tar 的信号转导特性。

The residue composition of the aromatic anchor of the second transmembrane helix determines the signaling properties of the aspartate/maltose chemoreceptor Tar of Escherichia coli.

机构信息

Department of Biology, Texas A&M University, College Station, Texas 77843, United States.

出版信息

Biochemistry. 2012 Mar 6;51(9):1925-32. doi: 10.1021/bi201555x. Epub 2012 Feb 27.

DOI:10.1021/bi201555x
PMID:22339259
Abstract

Repositioning of the tandem aromatic residues (Trp-209 and Tyr-210) at the cytoplasmic end of the second transmembrane helix (TM2) modulates the signal output of the aspartate/maltose chemoreceptor of Escherichia coli (Tar(Ec)). Here, we directly assessed the effect of the residue composition of the aromatic anchor by studying the function of a library of Tar(Ec) variants that possess all possible combinations of Ala, Phe, Tyr, and Trp at positions 209 and 210. We identified three important properties of the aromatic anchor. First, a Trp residue at position 209 was required to maintain clockwise (CW) signal output in the absence of adaptive methylation, but adaptive methylation restored the ability of all of the mutant receptors to generate CW rotation. Second, when the aromatic anchor was replaced with tandem Ala residues, signaling was less compromised than when an Ala residue occupied position 209 and an aromatic residue occupied position 210. Finally, when Trp was present at position 209, the identity of the residue at position 210 had little effect on baseline signal output or aspartate chemotaxis, although maltose taxis was significantly affected by some substitutions at position 210. All of the mutant receptors we constructed supported some level of aspartate and maltose taxis in semisolid agar swim plates, but those without Trp at position 209 were overmethylated in their baseline signaling state. These results show the importance of the cytoplasmic aromatic anchor of TM2 in maintaining the baseline Tar(Ec) signal output and responsiveness to attractant signaling.

摘要

串联芳香残基(色氨酸 209 和酪氨酸 210)在第二跨膜螺旋(TM2)的细胞质末端的重定位调节大肠杆菌天冬氨酸/麦芽糖化学感受器(Tar(Ec))的信号输出。在这里,我们通过研究 Tar(Ec)变体文库的功能,直接评估芳香锚定残基组成的影响,该文库具有位置 209 和 210 处的 Ala、Phe、Tyr 和 Trp 的所有可能组合。我们确定了芳香锚定的三个重要特性。首先,位置 209 处的色氨酸残基对于在没有适应性甲基化的情况下保持顺时针(CW)信号输出是必需的,但适应性甲基化恢复了所有突变受体产生 CW 旋转的能力。其次,当芳香锚被串联 Ala 残基取代时,信号传递的损害程度小于 Ala 残基占据位置 209 且芳香残基占据位置 210 时。最后,当位置 209 存在色氨酸时,位置 210 的残基的身份对基线信号输出或天冬氨酸趋化性几乎没有影响,尽管麦芽糖趋化性受到位置 210 中的一些取代的显著影响。我们构建的所有突变受体都在半固体琼脂泳动平板中支持一定水平的天冬氨酸和麦芽糖趋化性,但在基线信号状态下,位置 209 没有色氨酸的那些受体过度甲基化。这些结果表明 TM2 细胞质芳香锚在维持 Tar(Ec)的基线信号输出和对吸引物信号的响应性方面的重要性。

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The residue composition of the aromatic anchor of the second transmembrane helix determines the signaling properties of the aspartate/maltose chemoreceptor Tar of Escherichia coli.芳香锚定第二跨膜螺旋的残基组成决定了大肠杆菌天冬氨酸/麦芽糖化学感受器 Tar 的信号转导特性。
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