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在添加了MEM+和B27的神经基础培养基混合物中海马体和皮质神经元的存活情况。

Survival of hippocampal and cortical neurons in a mixture of MEM+ and B27-supplemented neurobasal medium.

作者信息

Xie C, Markesbery W R, Lovell M A

机构信息

Sanders-Brown Center on Aging, University of Kentucky, Lexington, KY 40536-0230, USA.

出版信息

Free Radic Biol Med. 2000 Mar 1;28(5):665-72. doi: 10.1016/s0891-5849(99)00268-3.

DOI:10.1016/s0891-5849(99)00268-3
PMID:10754261
Abstract

Serum-free B-27 supplemented neurobasal (NB) and a 10% fetal bovine serum-supplemented Eagle's minimum essential medium (MEM+) are used to culture rat embryonic hippocampal neurons for different purposes. Although NB medium leads to enhanced cell survival, it contains biological antioxidants and is not suitable for the study of free radical damage and oxidation in cultured neurons. MEM+ without additional antioxidants has been used widely in the study of free radical damage and oxidation, although it does not support optimum neuronal survival in culture. Serum in MEM+ leads to enhanced cell survival but also promotes glial cell proliferation. In this study, we used a new combination medium (NM-2) that consists of both NB and MEM+ for growing primary hippocampal and cortical neuronal cultures. NM-2 enhanced neuronal survival 78.9% for dissociated neurons at a density of 50 cells/mm(2) and 83.1% for 100 cells/mm(2), while decreasing glial cell proliferation to 2-3% and completely inhibiting oligodendrocytes. The NM-2 minimized the effectiveness of antioxidants in the medium to the neurotoxin 4-hydroxynonenal. It also decreased neuronal clumping and provided a more even distribution of neurons. Neurons survived for 4 weeks in NM-2 without changing the original medium. NM-2 provides a good environment for studies of free radical damage and oxidation of neurons. The combination incorporates the best of both NB and MEM+ that results in high neuron survival rate, low glial cell proliferation, reduced antioxidant level, and provides relatively pure cultures of hippocampal and cortical neurons.

摘要

无血清添加B-27的神经基础培养基(NB)和添加10%胎牛血清的伊格尔最低必需培养基(MEM+)被用于不同目的的大鼠胚胎海马神经元培养。尽管NB培养基能提高细胞存活率,但它含有生物抗氧化剂,不适合用于研究培养神经元中的自由基损伤和氧化。不含额外抗氧化剂的MEM+已广泛用于自由基损伤和氧化研究,尽管它不能支持培养神经元的最佳存活。MEM+中的血清能提高细胞存活率,但也会促进胶质细胞增殖。在本研究中,我们使用了一种由NB和MEM+组成的新型复合培养基(NM-2)来培养原代海马和皮质神经元。对于密度为50个细胞/mm²的解离神经元,NM-2使神经元存活率提高了78.9%,对于100个细胞/mm²的神经元,存活率提高了83.1%,同时将胶质细胞增殖降低到2 - 3%,并完全抑制少突胶质细胞。NM-使培养基中抗氧化剂对神经毒素4-羟基壬烯醛的作用最小化。它还减少了神经元聚集,使神经元分布更均匀。神经元在NM-2中可存活4周而无需更换原始培养基。NM-2为神经元自由基损伤和氧化研究提供了良好的环境。这种组合融合了NB和MEM+的优点,导致高神经元存活率、低胶质细胞增殖、降低抗氧化剂水平,并提供相对纯净的海马和皮质神经元培养物。

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