首页> 美国卫生研究院文献>Journal of Bacteriology >Formation of cell wall polymers by reverting protoplasts of Bacillus licheniformis.
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Formation of cell wall polymers by reverting protoplasts of Bacillus licheniformis.

机译:通过回复地衣芽孢杆菌的原生质体形成细胞壁聚合物。

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摘要

The biosynthesis of peptidoglycan and teichoic acid by reverting protoplasts of Bacillus licheniformis 6346 His-, in cubated at 35 C on medium containing 2.5% agar, is detectable after 40 min. The amount of N-acetyl-[1-14C]glucosamine incorporated into peptidoglycan and teichoic acid on continued incubation doubles at the same rate as the incorporation of [3H]tryptophan into protein. At the early stages of reversion the average glycan chain length, measured by the ratio of free reducing groups of muramic acid and glucosamine to total muramic acid present, is very short. As reversion proceeds, the average chain length increases to a value similar to the found in the wall of the parent bacillus. The extent of cross-linkage found in the peptide side chains of the peptidoglycan also increases as reversion proceeds. At the completion of reversion the wall material synthesized has similar characteristics to those of the walls of the parent bacilli, containing peptidoglycan and teichoic and teichuronic acids in about the same proportions. Soluble peptidoglycan can be isolated from the reversion medium, amounting to 30% of the total formed after 3 h of incubation and 8% after 12 h. This amount was reduced by the presence in the medium of the walls of an autolysin-deficient mutant; they were not formed at all by reverting protoplasts of the autolysin-deficient mutant itself. Analysis of the soluble material provided additional evidence for their being autolytic products rather than small unchanged molecules. When protoplasts were incubated on medium containing only 0.8% agar, 53 to 67% of the peptidoglycan formed after 3 h of incubation was soluble, and 21% after 12 h. Fibers that appeared to be sheared from the protoplasts at intermediate stages of reversion on medium containing 2.5% agar were similar in composition to the bacillary walls.
机译:通过还原地衣芽孢杆菌6346 His-的原生质体在35℃下于含有2.5%琼脂的培养基中温育,可以检测肽聚糖和磷壁酸的生物合成。在连续孵育过程中,掺入肽聚糖和磷壁酸的N-乙酰基-[1-14C]氨基葡萄糖的量以与[3H]色氨酸掺入蛋白质的速率相同的速度增加一倍。在还原的早期阶段,平均聚糖链长度很短,该平均聚糖链是通过山酸和葡萄糖胺的游离还原基团与所存在的全部山酸之比来衡量的。随着还原的进行,平均链长增加到类似于亲本芽孢杆菌壁中发现的值。随着还原的进行,在肽聚糖的肽侧链中发现的交联程度也增加。还原完成后,所合成的壁材料具有与亲本细菌壁相似的特性,其中包含肽聚糖,回潮酸和四氢尿酸的比例大致相同。可以从还原培养基中分离出可溶性肽聚糖,其含量为孵育3小时后形成的总量的30%,占12小时后形成的总量的8%。通过在培养基中存在自溶素缺陷型突变体减少了该量;它们根本不是通过还原自身溶素缺陷型突变体本身的原生质体形成的。对可溶物质的分析为它们是自溶产物而不是小的不变分子提供了更多证据。当原生质体在仅包含0.8%琼脂的培养基上孵育时,孵育3小时后形成的53%至67%的肽聚糖是可溶的,而在12小时后溶解为21%。在含有2.5%琼脂的培养基上,在回复的中间阶段,似乎从原生质体上剪下的纤维的成分与细菌壁相似。

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