首页> 美国卫生研究院文献>The Journal of Biophysical and Biochemical Cytology >Direct biochemical measurements of microtubule assembly and disassembly in Chinese hamster ovary cells. The effect of intercellular contact cold D2O and N6O2-dibutyryl cyclic adenosine monophosphate
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Direct biochemical measurements of microtubule assembly and disassembly in Chinese hamster ovary cells. The effect of intercellular contact cold D2O and N6O2-dibutyryl cyclic adenosine monophosphate

机译:在中国仓鼠卵巢细胞中微管组装和拆卸的直接生化测量。细胞间接触感冒D2O和N6O2-二丁酰基环状腺苷单磷酸的影响

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摘要

A study was undertaken to develop a means of quantitating the amount of tubulin present as a soluble pool and as intact microtubules in cultured Chinese hamster ovary cells. A procedure was developed in which these cells grown on monolayer culture in Petri dishes were placed in a "microtubule stabilizing medium" (MTM) consisting of 50% glycerol, 10% dimethylsulfoxide and sodium phosphate magnesium buffer, as described previously by Filner and Behnke. These cells then were homogenized and the homogenate was spun in the ultracentrifuge. Colchicine binding activity was then determined in the supernates and the pellets. The values, when compared with total colchicine binding activity present in replicate homogenates, were used to determine the percentage of tubulin present as intact microtubules. A statistical analysis of thin sections of cells treated with MTM revealed no statistically significant difference between MTM-treated cells and untreated controls. It was further discovered that the relative amount of colchicine binding activity recovered in the high speed pellet varied dramatically, depending upon the cell number of the culture being studied. Preconfluent cultures showed very low colchicine binding activity averaging less than 5%, while confluent and postconfluent cultures often possessed as high as 25% of their total colchicine binding activity in pelletable material. Although cold and D2O treatment had little or no effect on these values, N6,O2'-dibutyryl cyclic adenosine monophosphate increased them. It is hoped that this study will serve as the basis for a reliable quantitative procedure for measuring microtubule polymerization and depolymerization in vivo.
机译:进行了一项研究,以开发一种定量的方法来定量培养的中国仓鼠卵巢细胞中可溶性蛋白池和完整微管中微管蛋白的含量。如先前由Filner和Behnke所述,开发了一种程序,其中将这些细胞在培养皿中在单层培养上生长的细胞置于由50%甘油,10%二甲基亚砜和磷酸钠镁缓冲液组成的“微管稳定培养基”(MTM)中。然后将这些细胞匀浆,并在超速离心机中离心匀浆。然后测定上清液和沉淀中的秋水仙碱结合活性。当与重复匀浆中存在的总秋水仙碱结合活性比较时,该值用于确定以完整微管形式存在的微管蛋白的百分比。对经MTM处理的细胞薄片的统计分析表明,经MTM处理的细胞与未经处理的对照之间没有统计学上的显着差异。进一步发现,在高速沉淀物中回收的秋水仙碱结合活性的相对量变化很大,这取决于所研究的培养物的细胞数。融合前的培养物显示秋水仙碱的结合活性非常低,平均少于5%,而融合和融合后的培养物在可沉淀的物料中通常拥有高达其秋水仙碱总结合活性的25%。尽管冷和D2O处理对这些值影响很小或没有影响,但是N6,O2'-二丁酰基环状腺苷单磷酸酯会增加这些值。希望这项研究将为测量体内微管聚合和解聚的可靠定量程序奠定基础。

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