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从大鼠脑中纯化的可溶性硫酸软骨素蛋白聚糖的核心蛋白可阻断PC12D细胞的细胞周期。

Core proteins of soluble chondroitin sulfate proteoglycans purified from the rat brain block the cell cycle of PC12D cells.

作者信息

Katoh-Semba R, Oohira A

机构信息

Department of Perinatology, Institute for Developmental Research, Aichi Prefecture Colony, Japan.

出版信息

J Cell Physiol. 1993 Jul;156(1):17-23. doi: 10.1002/jcp.1041560104.

DOI:10.1002/jcp.1041560104
PMID:8314855
Abstract

The effects of soluble chondroitin sulfate proteoglycans (CSPGs) purified from the rat brain on proliferation of and neurite outgrowth from PC12D cells (Katoh-Semba et al., J Neurosci Res 17:36, 1987) were investigated. When PC12D cells are cultured under standard conditions, they proliferate with a doubling time of about 2 days, irrespective of the presence or absence of NGF. However, the addition of a mixture of several types of purified soluble brain CSPG (50 nmol uronic acid/ml) to the culture medium prevented the increase in the number of PC12D cells as well as the nerve growth factor (NGF)-induced neurite extension. The dose for 50% inhibition (ID50) was 1.6 nmol/ml for cell proliferation and 2.7 nmol/ml for neurite elongation. The increase in cell number seemed to stop around 6 h after exposure to culture medium supplemented with brain-derived CSPGs, and even substratum-attached CSPGs were able to exert such inhibitory effects. Only brain-type CSPGs, not a cartilage-derived CSPG (PGH) or a hyaluronate-binding PGH, had such inhibitory effects. Furthermore, these inhibitory activities were associated only with the core proteins of brain-derived CSPGs, and not with polysaccharide chains from brain-derived CSPGs. Incorporation of [3H]thymidine into DNA did not decrease for at least the first 12 h. Consequently, the amount of DNA per cell after 48 h of culture was about twofold higher in cells treated with brain CSPGs than in nontreated cells after exposure to the medium with CSPGs. Microspectrophotometry revealed that the population of cells with a high DNA content was greater in the culture treated with brain-derived CSPGs than in the control culture. These findings indicate that purified soluble brain CSPGs block the cell cycle of PC12D cells at the G2 phase with resultant cessation of cell proliferation and the inhibition of neurite outgrowth.

摘要

研究了从大鼠脑中纯化的可溶性硫酸软骨素蛋白聚糖(CSPGs)对PC12D细胞增殖及神经突生长的影响(Katoh-Semba等人,《神经科学研究杂志》17:36,1987年)。当PC12D细胞在标准条件下培养时,无论有无神经生长因子(NGF),它们都会以约2天的倍增时间进行增殖。然而,向培养基中添加几种纯化的可溶性脑CSPG混合物(50 nmol糖醛酸/毫升)可阻止PC12D细胞数量的增加以及神经生长因子(NGF)诱导的神经突延伸。细胞增殖的50%抑制剂量(ID50)为1.6 nmol/毫升,神经突伸长的ID50为2.7 nmol/毫升。暴露于添加了脑源性CSPGs的培养基后约6小时,细胞数量的增加似乎停止,甚至附着于基质的CSPGs也能发挥这种抑制作用。只有脑型CSPGs具有这种抑制作用,软骨来源的CSPG(PGH)或透明质酸结合PGH则没有。此外,这些抑制活性仅与脑源性CSPGs的核心蛋白有关,而与脑源性CSPGs的多糖链无关。至少在最初12小时内,[3H]胸苷掺入DNA的量并未减少。因此,培养48小时后,用脑CSPGs处理的细胞中每细胞的DNA量比暴露于含CSPGs培养基中的未处理细胞高约两倍。显微分光光度法显示,用脑源性CSPGs处理的培养物中DNA含量高的细胞群体比对照培养物中的更大。这些发现表明,纯化的可溶性脑CSPGs在G2期阻断PC12D细胞的细胞周期,导致细胞增殖停止和神经突生长受到抑制。

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