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对影响细胞社会行为的培养上清液中的因子进行表征。

Characterization of factor(s) in culture supernatants affecting cell social behavior.

作者信息

Weston J A, Yamada K M, Hendricks K L

出版信息

J Cell Physiol. 1979 Sep;100(3):445-56. doi: 10.1002/jcp.1041000308.

Abstract

Treatment of embryonic chick heart fibroblast cultures with 0.2 M urea reversibly increases cellular overlap. The increase in cellular overlapping over that in control cultures may be quantitated by the overlap ratio (R), the ratio of the number of superimposed nuclei observed, to the number expected to occur when cells are assumed to be distributed randomly over the culture substratum (R = observed/expected overlaps). Reversal of the urea-induced increase in R is blocked by 0.2 micrograms/ml cycloheximide. In the presence of cycloheximide, normal (low) overlap ratios are restored to urea-treated cultures by adding non-dialyzable material recovered by washing fibroblast monolayers with serum-free medium. The overlap ratio assay revealed no effect of supernatant material added either to urea-treated cultures in the continued presence of urea, or to untreated cultures. Although unfiltered supernatants were shown by SDS-polyacrylamide gel electrophoresis to contain fibronectin (CSP; LETS; MWappar. = 220,000 d) and smaller proteins, the ability to reverse the urea-induced increase in overlap ratio was present in Diaflo and Millipore filtrates of culture supernatants in which fibronectin was greatly depleted or absent. In contrast, purified fibronectin preparations failed to lower urea-induced increases in overlap-ratio. Partially purified, biologically active supernatants, prepared from 14C-leucine or 125I-labeled cultures, contained several macromolecules smaller than fibronectin that were labeled by both radioisotopes. In particular, one band (MWappar. = 58--60,000 d) was present in polyacrylamide gels of active supernatant and also depleted in gels of homogenates from urea-treated cultures. These results indicate that external macromolecules other than fibronectin are synthesized by cultured fibroblasts and can affect cell social behavior or culture morphology.

摘要

用0.2M尿素处理鸡胚心脏成纤维细胞培养物会可逆地增加细胞重叠。与对照培养物相比,细胞重叠的增加可通过重叠率(R)来定量,重叠率是观察到的叠加核的数量与假设细胞随机分布在培养底物上时预期出现的数量之比(R = 观察到的重叠数/预期重叠数)。0.2微克/毫升的环己酰亚胺可阻止尿素诱导的R增加的逆转。在存在环己酰亚胺的情况下,通过添加用无血清培养基洗涤成纤维细胞单层回收的不可透析物质,可使尿素处理的培养物恢复正常(低)重叠率。重叠率测定显示,无论是在持续存在尿素的情况下添加到尿素处理的培养物中,还是添加到未处理的培养物中的上清液物质均无影响。虽然SDS-聚丙烯酰胺凝胶电泳显示未过滤的上清液含有纤连蛋白(CSP;LETS;表观分子量 = 220,000 d)和较小的蛋白质,但在纤连蛋白大量减少或不存在的培养上清液的Diaflo和Millipore滤液中存在逆转尿素诱导的重叠率增加的能力。相反,纯化的纤连蛋白制剂未能降低尿素诱导的重叠率增加。从14C-亮氨酸或125I标记的培养物中制备的部分纯化的生物活性上清液含有几种比纤连蛋白小的大分子,这两种放射性同位素均对其进行了标记。特别是,在活性上清液的聚丙烯酰胺凝胶中存在一条带(表观分子量 = 58 - 60,000 d),并且在尿素处理的培养物的匀浆凝胶中也减少了。这些结果表明,培养的成纤维细胞合成了除纤连蛋白以外的外部大分子,并且这些大分子可以影响细胞的社会行为或培养形态。

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