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鼠型斑疹伤寒立克次体和小蛛立克次体在经辐射的L细胞中的代谢

Metabolism of Rickettsia typhi and Rickettsia akari in irradiated L cells.

作者信息

Weiss E, Newman L W, Grays R, Green A E

出版信息

Infect Immun. 1972 Jul;6(1):50-7. doi: 10.1128/iai.6.1.50-57.1972.

Abstract

L cells that had been exposed to 3,000 r of (60)Co the previous day were used to study the growth and metabolism of Rickettsia typhi and R. akari. Viable (unirradiated) L cells were used to study the effect of rickettsial infection on host-cell metabolism. Monolayers were infected with a rickettsial multiplicity of 1.2 and given Eagle's minimal essential medium containing 25 mmN-2-hydroxyethylpiperazine-N'-2'-ethanesulfonic acid buffer and 10% calf serum. At various intervals, cycloheximide (2 mug/ml) was added to one set of cultures, to inhibit eukaryotic protein and deoxyribonucleic acid (DNA) metabolism; phosphate-buffered saline (PBS) was added to another set. After 1 hr, the cultures received a mixture of 15 (14)C-labeled amino acids or adenine-8-(14)C. The cultures were harvested 16 hr later and were tested for incorporation of labeled carbon into the fraction precipitated by cold trichloroacetic acid. Viable cells were exposed to thymidine-2-(14)C for 2-hr periods. Infectivity of R. typhi increased to a peak of 150 to 400 hemolytic units/culture on day 4; the titer remained approximately the same on days 5 and 6, and declined rapidly on day 7. Total amino acid incorporation was about the same in infected and uninfected cultures up to day 6, but metabolic activity was reduced to a negligible level on day 7 in infected cells. Cycloheximide-resistant activity was higher in the infected cultures, with a peak equivalent to one-half the total activity at day 4 to 5. Total as well as cycloheximide-resistant adenine incorporation was higher in the infected cells between days 3 and 5 after infection, with a peak at day 3 to 4. Somewhat similar results were obtained with R. akari, except that the cycle of infection and of cycloheximide-resistant activity proceeded and was completed more rapidly. (14)C-DNA of both rickettsiae was isolated from infected cultures that had received labeled adenine. With labeled thymidine, which was not incorporated by the rickettsiae, it was shown that R. typhi and R. akari differ considerably in their effects on the host cell. R. typhi elicited moderate inhibition, whereas R. akari infection led to a complete inhibition of thymidine incorporation by the third day, at the time of highest rickettsial activity. It is concluded that rickettsiae have the necessary enzymes for protein and nucleic acid synthesis, but, thus far, these enzymes have been activated or induced only in an intracellular environment.

摘要

使用前一天接受过3000伦琴(60)钴照射的L细胞来研究鼠型斑疹伤寒立克次体和小蛛立克次体的生长与代谢。使用活的(未照射的)L细胞来研究立克次体感染对宿主细胞代谢的影响。将单层细胞以1.2的立克次体感染复数进行感染,并给予含有25 mM N-2-羟乙基哌嗪-N'-2'-乙磺酸缓冲液和10%小牛血清的伊格尔最低必需培养基。在不同时间间隔,向一组培养物中加入环己酰亚胺(2微克/毫升),以抑制真核蛋白质和脱氧核糖核酸(DNA)代谢;向另一组培养物中加入磷酸盐缓冲盐水(PBS)。1小时后,培养物接受15种(14)C标记氨基酸或腺嘌呤-8-(14)C的混合物。16小时后收获培养物,并检测标记碳掺入冷三氯乙酸沉淀部分的情况。将活细胞暴露于胸苷-2-(14)C中2小时。鼠型斑疹伤寒立克次体的感染力在第4天增加到峰值,为150至400个溶血单位/培养物;在第5天和第6天滴度大致相同,在第7天迅速下降。在第6天之前,感染和未感染的培养物中总氨基酸掺入量大致相同,但在第7天,感染细胞中的代谢活性降低到可忽略不计的水平。感染培养物中环己酰亚胺抗性活性较高,在第4至5天达到相当于总活性一半的峰值。感染后第3至5天,感染细胞中总腺嘌呤掺入量以及环己酰亚胺抗性腺嘌呤掺入量均较高,在第3至4天达到峰值。用小蛛立克次体获得了 somewhat 类似的结果,只是感染周期和环己酰亚胺抗性活性的进程和完成速度更快。两种立克次体的(14)C-DNA均从接受标记腺嘌呤的感染培养物中分离得到。用未被立克次体掺入的标记胸苷表明,鼠型斑疹伤寒立克次体和小蛛立克次体对宿主细胞的影响有很大差异。鼠型斑疹伤寒立克次体引起中度抑制,而小蛛立克次体感染在第三天,即立克次体活性最高时,导致胸苷掺入完全抑制。结论是立克次体具有蛋白质和核酸合成所需的酶,但到目前为止,这些酶仅在细胞内环境中被激活或诱导。 (注:“somewhat”翻译为“ somewhat”,可能是原文有误,猜测可能是“somewhat”,意为“有点,稍微” )

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/de7a/422489/44adb4322ef9/iai00271-0065-a.jpg

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