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[神经组织细胞中DNA合成刺激剂的研究]

[Study of DNA synthesis stimulators in nerve tissue cells].

作者信息

Vitvitskiĭ V N

出版信息

Biokhimiia. 1985 Oct;50(10):1616-20.

PMID:4074773
Abstract

Ontogenetic changes in DNA synthesis in different divisions and regions of the brain occur via different mechanisms, which is conditioned by changes in the composition and properties of corresponding mediators. Tissue extracts obtained from the parts of brain characterized by intensive cell division (cortex of 15-17-day-old embryos or cerebellum of 8-10-day-old animals) can stimulate the incorporation of labeled precursors into brain cell DNA in both neonatal and adult rats. Using desalting at increasing concentrations of ammonium sulfate, gel filtration on sephadexes and isoelectrofocusing, three fractions of DNA synthesis stimulators whose isoelectric points lie at acidic, neutral and alkaline regions of pH, were isolated. A method is described, which can be employed for isolation in a pure state and determination of some physico-chemical properties of an acid activator. The latter is a low molecular weight peptide causing marked stimulation of [3H]thymidine incorporation into nervous tissue cell DNA in an in vitro system, when taken at a concentration of about 1 microgram/ml.

摘要

大脑不同分区和区域中DNA合成的个体发育变化通过不同机制发生,这取决于相应介质的组成和性质的变化。从以细胞密集分裂为特征的脑区(15 - 17日龄胚胎的皮质或8 - 10日龄动物的小脑)获得的组织提取物,能够刺激新生大鼠和成年大鼠的脑细胞DNA中标记前体的掺入。通过在不断增加的硫酸铵浓度下脱盐、在葡聚糖凝胶上进行凝胶过滤以及等电聚焦,分离出了三种DNA合成刺激剂组分,其等电点位于pH的酸性、中性和碱性区域。描述了一种可用于以纯态分离并测定一种酸性激活剂某些物理化学性质的方法。后者是一种低分子量肽,当以约1微克/毫升的浓度使用时,在体外系统中能显著刺激[3H]胸苷掺入神经组织细胞DNA。

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