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Characterization of the l-alanine exporter AlaE of Escherichia coli and its potential role in protecting cells from a toxic-level accumulation of l-alanine and its derivatives

机译:大肠杆菌的l-丙氨酸输出蛋白AlaE的表征及其在保护细胞免受l-丙氨酸及其衍生物毒性水平累积的潜在作用

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摘要

We previously reported that the alaE gene of Escherichia coli encodes the l-alanine exporter AlaE. The objective of this study was to elucidate the mechanism of the AlaE exporter. The minimum inhibitory concentration of l-alanine and l-alanyl-l-alanine in alaE-deficient l-alanine-nonmetabolizing cells MLA301ΔalaE was 4- and >4000-fold lower, respectively, than in the alaE-positive parent cells MLA301, suggesting that AlaE functions as an efflux pump to avoid a toxic-level accumulation of intracellular l-alanine and its derivatives. Furthermore, the growth of the alaE-deficient mutant derived from the l-alanine-metabolizing strain was strongly inhibited in the presence of a physiological level of l-alanyl-l-alanine. Intact MLA301ΔalaE and MLA301ΔalaE/pAlaE cells producing plasmid-borne AlaE, accumulated approximately 200% and 50%, respectively, of the [3H]l-alanine detected in MLA301 cells, suggesting that AlaE exports l-alanine. When 200 mmol/L l-alanine-loaded inverted membrane vesicles prepared from MLA301ΔalaE/pAlaE were placed in a solution containing 200 mmol/L or 0.34 μmol/L l-alanine, energy-dependent [3H]l-alanine accumulation occurred under either condition. This energy-dependent uphill accumulation of [3H]l-alanine was strongly inhibited in the presence of carbonyl cyanide m-chlorophenylhydrazone but not by dicyclohexylcarbodiimide, suggesting that the AlaE-mediated l-alanine extrusion was driven by proton motive force. Based on these results, physiological roles of the class="small-caps">l-alanine exporter are discussed.
机译:我们之前曾报道过,大肠杆菌的alaE基因编码l-丙氨酸输出者AlaE。这项研究的目的是阐明AlaE出口商的机制。与alaE阳性亲代细胞MLA301相比,在alaE缺失的l-丙氨酸非代谢细胞MLA301ΔalaE中,l-丙氨酸和l-丙氨酰基-1-丙氨酸的最低抑制浓度分别低4倍和> 4000倍。 AlaE用作外排泵,以避免细胞内1-丙氨酸及其衍生物的毒性水平积累。此外,在生理水平的1-丙氨酰基-1-丙氨酸存在下,强烈抑制了源自1-丙氨酸代谢菌株的alaE缺陷型突变体的生长。完整的MLA301ΔalaE和MLA301ΔalaE/ pAlaE细胞产生质粒携带的AlaE,在MLA301细胞中检测到的[ 3 H] 1-丙氨酸分别累积约200%和50%,这表明AlaE输出l-丙氨酸。当将由MLA301ΔalaE/ pAlaE制备的200 mmol / L加载有l-丙氨酸的倒膜囊泡置于含有200 mmol / L或0.34μmol/ L的l-丙氨酸的溶液中时,能量依赖性[ 3 H在任一情况下都发生] 1-丙氨酸积累。 [ 3 H] 1-丙氨酸的这种能量依赖的上坡积累在羰基氰化物间氯苯hydr存在下受到强烈抑制,但不被二环己基碳二亚胺抑制,这表明驱动了AlaE介导的1-丙氨酸挤出通过质子动力。基于这些结果,讨论了 class =“ small-caps”> l -丙氨酸出口者的生理作用。

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