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在体外培养Krebs II腹水细胞期间内质网膜轮廓的时间依赖性改变。

Time-dependent alteration in endoplasmic reticulum membrane profiles during in vitro incubation of Krebs II ascites cells.

作者信息

Fjose A, Pryme I F

出版信息

Mol Cell Biochem. 1983;56(2):131-6. doi: 10.1007/BF00227213.

Abstract

Krebs II ascites cells were harvested from the mouse peritoneum 6-8 days after inoculation and incubated in vitro in roller suspension culture for up to 22 hr. Within 2 hr of incubation a large portion of the cells entered S phase as judged by the incorporation of 3H-thymidine into DNA. The incorporation of radioactive precursors into phospholipid, protein and RNA increased rapidly during in vitro incubation indicating a high degree of macromolecular synthesis. The rates of incorporation were maximal within 4 hr of incubation. When cells labeled with 3H-choline were disrupted by nitrogen cavitation and endoplasmic reticulum (ER) membranes analyzed for subfractions on discontinuous sucrose gradients, it was observed that only small amounts of radioactivity could be detected in the HR region after 1/2 hr incubation while 63.2% of total radioactivity in ER membranes appeared in the LR fraction. Between 8-18 hr there was a considerable increase in the amount of HR membranes. Of the total radioactivity in ER membranes that in the HR fraction increased from 16.9% to 53.9% during this period. There were only small changes in the amounts of radioactivity in LR and S membranes between 8 and 18 hr. The results suggest a time-dependent appearance of ER membrane subfractions during a 22 hr period of in vitro incubation of Krebs II ascites cells.

摘要

接种后6 - 8天从小鼠腹膜收集克雷布斯II腹水细胞,并在体外进行滚瓶悬浮培养长达22小时。培养2小时内,通过3H - 胸腺嘧啶核苷掺入DNA判断,大部分细胞进入S期。在体外培养期间,放射性前体掺入磷脂、蛋白质和RNA的量迅速增加,表明大分子合成程度很高。掺入速率在培养4小时内达到最大值。当用3H - 胆碱标记的细胞通过氮空化破碎,内质网(ER)膜在不连续蔗糖梯度上分析亚组分时,观察到培养半小时后在HR区域仅能检测到少量放射性,而内质网膜中63.2%的总放射性出现在LR组分中。在8 - 18小时之间,HR膜的量有相当大的增加。在此期间,内质网膜中HR组分的总放射性从16.9%增加到53.9%。在8至18小时之间,LR和S膜中的放射性量仅有微小变化。结果表明,在克雷布斯II腹水细胞体外培养22小时期间,内质网膜亚组分呈时间依赖性出现。

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