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Characterization of an NaCl-sensitive Staphylococcus aureus mutant and rescue of the NaCl-sensitive phenotype by glycine betaine but not by other compatible solutes.

机译:NaCl敏感的金黄色葡萄球菌突变体的表征和甘氨酸甜菜碱而不是其他相容性溶质的NaCl敏感表型的挽救。

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摘要

To further study mechanisms of coping with osmotic stress-low water activity, mutants of Staphylococcus aureus with transposon Tn917-lacZ-induced NaCl sensitivity were selected for impaired ability to grow on solid defined medium containing 2 M NaCl. Southern hybridization experiments showed that NaCl-sensitive mutants had a single copy of the transposon inserted into a DNA fragment of the same size in each mutant. These NaCl-sensitive mutants had an extremely long lag phase (60 to 70 h) in defined medium containing 2.5 M NaCl. The osmoprotectants glycine betaine and choline (which is oxidized to glycine betaine) dramatically shortened the lag phase, whereas L-proline and proline betaine, which are effective osmoprotectants for the wild type, were ineffective. Electron microscopic observations of the NaCl-sensitive mutant under NaCl stress conditions revealed large, pseudomulticellular cells similar to those observed previously in the wild type under the same conditions. Glycine betaine, but not L-proline, corrected the morphological abnormalities. Studies of the uptake of L-[14C]proline and [14C]glycine betaine upon osmotic upshock revealed that the mutant was not defective in the uptake of either osmoprotectant. Comparison of pool K+, amino acid, and glycine betaine levels under NaCl stress conditions in the mutant and the wild type revealed no striking differences. Glycine betaine appears to have additional beneficial effects on NaCl-stressed cells beyond those of other osmoprotectants. The NaCl stress protein responses of the wild type and the NaCl-sensitive mutant were characterized and compared by labeling with L-[35 S]methionine and two-dimensional gel electrophoresis. The synthesis of 10 proteins increased in the wild type in response to NaCl stress, whereas the synthesis of these 10 proteins plus 2 others increased in response to NaCl stress in the NaCl-sensitive mutant. Five proteins, three of which were NaCl stress proteins, were produced in elevated amounts in the NaCl-sensitive mutant under unstressed conditions compared to the wild type. The presence of glycine betaine during NaCl stress decreased the production of three NaCl stress proteins in the mutant versus one in the wild type.
机译:为了进一步研究应对渗透胁迫-低水分活性的机制,选择了具有转座子Tn917-lacZ诱导的NaCl敏感性的金黄色葡萄球菌突变体,以削弱其在含有2 M NaCl的固体培养基上的生长能力。 Southern杂交实验表明,对NaCl敏感的突变体具有单个拷贝的转座子,插入每个突变体大小相同的DNA片段中。这些对NaCl敏感的突变体在含有2.5 M NaCl的特定培养基中具有极长的滞后阶段(60至70 h)。渗透保护剂甘氨酸甜菜碱和胆碱(被氧化为甘氨酸甜菜碱)大大缩短了滞后阶段,而L-脯氨酸和脯氨酸甜菜碱(对野生型有效的渗透保护剂)无效。在NaCl胁迫条件下对NaCl敏感突变体的电子显微镜观察显示,大型假多细胞细胞类似于先前在相同条件下在野生型中观察到的细胞。甘氨酸甜菜碱,但不是L-脯氨酸,纠正了形态异常。对L- [14C]脯氨酸和[14C]甘氨酸甜菜碱在渗透性冲击后的吸收研究表明,该突变体在两种渗透保护剂的吸收中均无缺陷。在突变体和野生型中,在NaCl胁迫条件下,库K +,氨基酸和甘氨酸甜菜碱水平的比较没有显着差异。甘氨酸甜菜碱似乎对NaCl胁迫的细胞具有其他渗透保护剂以外的其他有益作用。通过用L- [35S]蛋氨酸标记和二维凝胶电泳对野生型和NaCl敏感突变体的NaCl胁迫蛋白应答进行了表征和比较。在NaCl敏感突变体中,响应于NaCl胁迫,野生型中10种蛋白质的合成增加,而响应于NaCl胁迫,这10种蛋白质和2种其他蛋白质的合成增加。与野生型相比,在无胁迫条件下,NaCl敏感突变体中产生了五种蛋白质,其中三种是NaCl胁迫蛋白质,产量升高。在NaCl胁迫期间,甘氨酸甜菜碱的存在降低了突变体中三种NaCl胁迫蛋白的产生,而野生型中则为一种。

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