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Envelope-associated folded chromosomes for Escherichia coli: variations under different physiological conditions.

机译:大肠杆菌的与信封相关的折叠染色体:在不同生理条件下的变异。

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摘要

The folded chromosome of Escherichia coli has been investigated under various lysis and physiological conditions. A new gradient system was devised that allows excellent separation between unlysed cells and envelope-associated and envelope-free chromosomes. Isotope incorporation experiments showed that the fraction often called "membrane-bound nucleoids" contains cell wall in addition to nucleic acids, membranes, and proteins. The amount of lysozyme added and the lysozyme digestion time were found to be important when comparing the rate of sedimentation of envelope-associated chromosomes obtained under various physiological conditions. Amino acid-starved cells were found to be much harder to lyse with lysozyme than exponentially grown cells, The difference in sedimentation coefficient of envelope-associated chromosomes described earlier (Ryder and Smith, 1974) was not detected when the latter two types of cells had been given equivalent, but not identical, lysozyme treatment such that detergent-mediated lysis proceeded at the same rate. Analysis of pulse- and uniformly labeled chromosomes from amino acid-starved cultures revealed no preferential labeling of either envelope-associated or -released nucleoids. Nor was there a difference in sedimentation coefficient between uniform and pulse-labeled envelope-associated nucleoids. These results are in disagreement with the models for chromosome replication of Worcel and Burgi (1974) and Ryder and Smith (1974), respectively. Growing cells on carbon sources poorer than glucose demonstrated that the replicating chromosomes sediment faster than the bulk of envelope-associated nucleoids. The slower the growth rate, the greater this difference became. An alternative hypothesis regarding chromosome replication and its association with the cell envelope is presented.
机译:已经在各种裂解和生理条件下研究了大肠杆菌的折叠染色体。设计了一种新的梯度系统,可以很好地分离未裂解的细胞与包膜相关的染色体和无包膜的染色体。同位素掺入实验表明,通常被称为“膜结合核苷”的部分除核酸,膜和蛋白质外还包含细胞壁。当比较在各种生理条件下获得的包膜相关染色体的沉降速率时,发现溶菌酶的添加量和溶菌酶的消化时间很重要。发现氨基酸饥饿的细胞比用指数生长的细胞更难用溶菌酶裂解。当后两种类型的细胞被裂解后,先前描述的包膜相关染色体的沉降系数差异(Ryder和Smith,1974)没有被检测到。给予相同但不相同的溶菌酶处理,以使去污剂介导的裂解以相同速率进行。对来自缺乏氨基酸的培养物的脉冲和均一标记的染色体的分析表明,与包膜相关或释放的类核素均未得到优先标记。均匀和脉冲标记的包膜相关核苷之间的沉降系数也没有差异。这些结果分别与Worcel和Burgi(1974)以及Ryder和Smith(1974)的染色体复制模型不一致。在比葡萄糖更差的碳源上生长的细胞表明,复制染色体的沉积速度快于与包膜相关的核苷的堆积速度。增长率越慢,差异越大。提出了关于染色体复制及其与细胞包膜的关联的另一种假设。

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