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在晶状节杆菌的杆状细胞和球状细胞长期饥饿期间内源性代谢的细胞内底物。

Intracellular substrates for endogenous metabolism during long-term starvation of rod and spherical cells of Arthrobacter crystallopoietes.

作者信息

Boylen C W, Ensign J C

出版信息

J Bacteriol. 1970 Sep;103(3):578-87. doi: 10.1128/jb.103.3.578-587.1970.

DOI:10.1128/jb.103.3.578-587.1970
PMID:5474876
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC248129/
Abstract

Cells of Arthrobacter crystallopoietes, harvested during growth as spheres and as rods, were starved by shaking at 30 C in phosphate buffer for 30 days, during which time they maintained 100% viability. Changes in cellular components and the activity of specific enzyme pathways were monitored. A glycogen-like polysaccharide comprised 40% of the dry weight of growing spherical cells and 10% of the dry weight of rod cells. This material was utilized at approximately the same rate, on a percentage basis, during starvation of both cell forms. The rods degraded intracellular protein at approximately twice the rate of the spheres. At the end of 30 days, the rods had degraded 40% and the spheres 20% of their initial content of protein. Ribonucleic acid (RNA) was degraded significantly more rapidly in the rods. After 30 days starvation, 85 and 32% of the initial RNA of rods and spheres, respectively, had been depleted. Magnesium ion followed this same general pattern; the rods lost 65% and the spheres 45% of their initial content during 28 days of starvation. Deoxyribonucleic acid increased by 20% during the first few hours of starvation of both cell forms and then remained constant. The ability of glucose-, succinate-, and 2-hydroxypyridine (2-HP)-grown cells to oxidize glucose remained constant during 14 days of starvation. The ability of succinate-grown cells to oxidize succinate decreased rapidly during the first few hours of starvation to a rate which remained constant for 14 days. Cells adapted to growth on 2-HP completely lost their ability to oxidize this substrate after 3 days starvation.

摘要

在生长过程中收获的球形和杆状的晶状节杆菌细胞,在30℃的磷酸盐缓冲液中振荡饥饿30天,在此期间它们保持100%的活力。监测细胞成分的变化和特定酶途径的活性。一种类糖原多糖占生长中的球形细胞干重的40%,占杆状细胞干重的10%。在两种细胞形式饥饿期间,这种物质以大致相同的速率(按百分比计算)被利用。杆状细胞降解细胞内蛋白质的速率约为球形细胞的两倍。在30天结束时,杆状细胞降解了其初始蛋白质含量的40%,球形细胞降解了20%。核糖核酸(RNA)在杆状细胞中的降解速度明显更快。饥饿30天后,杆状细胞和球形细胞分别有85%和32%的初始RNA被耗尽。镁离子也遵循相同的总体模式;在28天的饥饿期间,杆状细胞失去了其初始含量的65%,球形细胞失去了45%。在两种细胞形式饥饿的最初几个小时内,脱氧核糖核酸增加了20%,然后保持不变。在14天的饥饿期间,以葡萄糖、琥珀酸和2-羟基吡啶(2-HP)培养的细胞氧化葡萄糖的能力保持不变。以琥珀酸培养的细胞氧化琥珀酸的能力在饥饿的最初几个小时内迅速下降到一个在14天内保持不变的速率。适应在2-HP上生长的细胞在饥饿3天后完全失去了氧化这种底物的能力。

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